Refine
Year of publication
Document Type
- Article (16363)
- Part of Periodical (2825)
- Working Paper (2365)
- Preprint (2319)
- Doctoral Thesis (2082)
- Book (1738)
- Conference Proceeding (1235)
- Part of a Book (1071)
- Report (471)
- Review (166)
Language
- English (30833) (remove)
Keywords
- taxonomy (752)
- new species (451)
- morphology (180)
- Deutschland (142)
- Syntax (126)
- Englisch (120)
- distribution (118)
- biodiversity (104)
- inflammation (101)
- Deutsch (98)
Institute
- Medizin (5467)
- Physik (4299)
- Wirtschaftswissenschaften (1941)
- Frankfurt Institute for Advanced Studies (FIAS) (1883)
- Biowissenschaften (1574)
- Informatik (1522)
- Center for Financial Studies (CFS) (1506)
- Biochemie und Chemie (1097)
- Sustainable Architecture for Finance in Europe (SAFE) (1085)
- House of Finance (HoF) (718)
The aim of the meeting is to expose this current topic for critical discussion with international speakers and participants and to find solutions which optimize the integration of information services into university structures. Presentations and discussions will consider: * integrated versus cooperative models * single-unit operations, central or de-centralized faculty organisations * outsourcing services versus own organisation/effort * institutional repository versus discipline-based repository * information supply in the era of "Google print" »The Integration of Information Services into University Structures« Symposium will be taking place simultaneously with the Frankfurt Book Fair, the largest book-related event in the world attracting annually 286,621 people (2006) , thus giving participants who arrive early the chance to combine attendance at both the Book Fair and Symposium. A cultural event and dinner in one of Frankfurt's historical rooms on Friday will be a social highlight! A contingency of hotel rooms has been reserved on a »first come, first served basis« outside Frankfurt at non-Book Fair prices. More information on request.
The mission of the Harvard Judaica Collection is to comprehensively document Jewish history and civilization in all places and periods. To accomplish its mission, the Judaica Collection collects materials in all languages and in all formats—books, pamphlets, periodicals, newspapers, sound recordings, and videos, posters, broadsides, and photographs. A particular focus is the Library’s Documenting Israel program, which covers all aspects of Israeli life and culture in great depth; Harvard has the largest collection of Israeli publications and Israel-related materials outside the State of Israel. The Harvard Judaica Collection also attempts to have comprehensive coverage of the publications of Jewish communities throughout the globe, including a significant collection of publications from countries across Europe. Collecting these materials requires cooperation with a wide array of institutions and individuals around the world.
The LOCKSS (Lots of Copies Keep Stuff Safe) Alliance is an international community of about 100 libraries and partners like OCLC. For almost a decade the LOCKSS open source model has been tested for its robustness against attack and for its ability to migrate formats. LOCKSS »boxes« at 150 institutions in more than 20 countries comprise a peer-to-peer system that automatically cross-checks content to ensure the accuracy and completeness of all member archives. Eighty publishers, including large publishers like Oxford University Press, are now participating in LOCKSS or actively preparing to add their journals to the program.
U. S. library resources on South Asia that were built around the limited needs of a handful of Sanskritics before World War II have made a long journey during the past half century. Since the inception of the Library of Congress Cooperative South Asia Acquisition Program (formerly called "PL-480" program), in 1962, libraries have built significant collections with financial support from governmental agencies and philanthropic foundations, to support teaching and research in all areas of social sciences and humanities. These collections have been supplemented by efforts to build retrospective collections and to microfilm rare materials in British and South Asian libraries and archives. Today, in cooperation with South Asian libraries, several projects are underway to preserve and digitize rapidly deteriorating materials so that these riches can be shared with the global scholarly community through electronic means.
To stimulate further discussion, I would like to briefly tackle the following questions: * How can one become informed about what is going on in German Studies in the US? * What kinds of American guides to German resources are available? * What kinds of German Studies resources are being produced in the US? * What do we know about how scholars are using (or not) these guides and resources?
The enhancing importance of digital documents has effected activities on how to deal with them. One line came from the more general field of "scientific publishing", which was handled in detail by DINI (Deutsche Initiative für Netzwerkinformation). But for this initiative long- time archiving was only one field of many and was not their primary focus. DINI first of all concentrated on the elaboration of effective and standardized methods and tools for publishing and related services on the basis of open access policy via the use of institutional repositories. The second line of projects came from the more general view of maintaining cultural heritage also in a digital world. Especially under the patronage of the Ministry of Education and Research important projects were being financed. Strategic solutions including archives, libraries, and museums are discussed and elaborated within NESTOR, where more technical solutions based on the term of practicability are developed within KOPAL. KOPAL brought together the industry (IBM) with a public- funded technical center (GWDG) and two libraries (DNB and SUB Göttingen). Within this project a general software implementation, which took into consideration all necessary international standards, could be finished last month and has been now for about two weeks. Based on early results within NESTOR it seemed important too, to strengthen all activities by giving them a legal basis. Therefore when the law changed concerning the German National Library from June 22nd this year (DNBG), the library was authorized with all the necessary instruments to collect digital documents in "non-physical" form as well. With this law at the moment Germany is in the rare position of being one of the few countries where the collection of network publications is part of the whole legal deposit strategy.
In the year 2000 the Deutsche Initiative für Netzwerkinformation (DINI) / German Coalition of Network Information was founded: 10 theses "Changes in information infrastructure – challenges to universities and their information and communications facilities" is the DINI’s founding charter (s. http://www.dini.de).
Thesis 4 states: "The universities need to establish information management structures to integrate departments. University managements, departments and central institutions ought to prepare a university development plan for the areas of information, communication and multimedia." ...
The basic argument the canonical and apocryphic theologies of the South Indian Tamil Shrivaishnavas grow worm over since centuries is the question: Has God set into motion the process of salvation in order to save mankind - the anthropocentric tradition is teaching -, or in order to save himself, the way a theocentric soteriology would teach. To answer this question we have to examine particularly the theocentric religion of salvation because it was held apocryphic by the anthropocentic orthodoxy and has therefore to be reconstructed from sources that are all concealed anthropocentrically. ...
Charity has a long tradition in the Christian religion. From the early beginning there was some organized charity. In the Acts of the Apostles we read about socalled diakonoi being responsible for the needy Christians. During the whole church history there was the rule that 1/3 of the tithe, the decima pars, the religious tax, had to be spend for the poor people of a parish. Of course, there was much misuse of that portion; the tithe became private and the new owners of the tax mostly living far away were not interested in supporting the poor people. Yet, the Christian people organized additional charity. It is very important to see that religious mentality was very helpful for that ...
Jonathan Wagner has written a monograph on a migration movement that was in many ways a peripheral one. From a Canadian perspective, Germans accounted for a relatively minor share of immigrants, compared to former residents of the British Isles, of eastern or southern Europe. Seen from Germany, Canada was one of many destinations for migrants who wished to leave the country and were prepared to travel over long distances, but were, for whatever reason, not attracted by the United States, the destination for the overwhelming majority of transcontinental emigrants. Nevertheless, the movement from Germany to Canada was significant in absolute and often symbolic terms. The way Wagner tells it, the story of German-Canadian migration was a tale of parallel experiences: both Germany and Canada experienced federation and increasing international autonomy from the 1860s; both were ruled by domineering conservative figures presiding over de facto liberalization in the 1870s; both participated in the First World War, and both went through traumatic economic crises in the interwar period. ...
The volume consists of eight essays with a precise focus: the study of the "dynamics of social exclusion" as reflected in data available for 1994 to 1996, when a detailed survey of a sample of households in EU countries, the "European Community Households Panel," was conducted. On the basis of these data, the authors document the extent and prevalence of poverty generally and specifically in regard to particular risk groups defined in terms of age, health and personal circumstances (young adults, lone parents, people with sickness or disability and retirees).[1] The analysis was carried out for five countries: Austria, Germany, Greece, Portugal and the United Kingdom, which were taken to be representative of the extremes of EU membership: north and south; wealthy and poor; large and small. The essays discuss income poverty (measured as incomes at 40, 50 or 60 percent of median incomes) as well as housing problems, access to basic necessities like food and utilities, access to consumer durables and social interactions. The essays document not only that the extent of poverty varies between countries--a well-known fact--but also that its causes and effects continue to differ even in an increasingly united western Europe. Austria had the lowest proportion of the population in poor households (17 percent--compared to 18 percent in Germany, 21 percent in the United Kingdom and Greece, and 24 percent in Portugal). While sickness and disability were likely to impoverish individuals in all the countries studied, this was particularly true of Austria, Germany and the United Kingdom (that is, northern Europe); retirement was more likely to result in income poverty in the south. The north-south divide was less relevant for parents; single income households with children were particularly likely to suffer from income poverty in the United Kingdom, Germany and Portugal. Poverty was more likely to be persistent than merely a brief phase in the life cycle. Persistence rates of income poverty were around 80 percent in Greece and Britain, above 70 percent in Portugal and above 60 percent in Germany and Austria. But the effects were rather different. In the United Kingdom, high persistence rates of income poverty coincided with low persistence rates (34 percent) of amenities deprivation, whereas the persistence of necessities deprivation was relatively low in Greece at 39 percent. The volume was conceived as a contribution to policy decision-making in the aftermath of the 2000 Lisbon Declaration, which focused (among other things) on poverty and encouraged member states to set more concrete targets for dealing with social exclusion. Some member states did so; Britain, for example--a country where income poverty was particularly likely to result in deprivation of basic necessities--vowed to abolish "poverty" by 2020. The volume is a treasure-trove of data and empirical analysis; it makes essential, though at times rather trying, reading for anyone interested in the extent of social exclusion, and the likelihood of falling into or escaping from it. It also provides ample proof--if any were needed--that governments seeking to combat social exclusion have to set different priorities, because they are not attacking the same phenomenon. Unfortunately, the empirical as well as the more conceptual contributions reveal some of the approach's and the book's shortcomings.[2] The book's very advantage--providing a precise research agenda--is also a drawback. With its focus on three years, and on the life-cycle rather than more stable factors such as ethnicity, occupation or regional origin, the volume presents a particular image of the risk (and duration) of deprivation, which may be more or less comprehensive for different countries. The narrow temporal focus makes one wonder whether measuring poverty's "persistence" of poverty makes much sense for such a relatively short time. Such doubt is enhanced when considering some of the oddities in the results: how did households that remained poor in the United Kingdom manage to get their hands on consumer durables? (The same question could be asked for the sudden increase in access to necessities in Greek households.) Illustrating the empirical findings with more concrete examples would have been helpful, particularly when they are counterintuitive, for instance the statement that patterns of poverty in eastern and western Germany were converging in spite of the continuing divergence in unemployment patterns. Another question--admittedly suggested by events of the last several years--is whether ethnicity, regional origins or occupations are not more important in determining the extent and duration of social exclusion than life cycle. These factors were not, and partly could not be, measured on the basis of the data used, but have moved to the center of policy debates today. This matter relates to another issue the book does not address: who is to blame for poverty, and what roles have governments and the European Union assumed in determining poverty patterns and trends? Have past policy choices--for instance, cutting benefits; increasing "flexibility" in labor markets; encouraging the emigration of jobs (such things the European Union is frequently accused of doing)--made a difference? Is combating poverty a serious policy agenda, or merely window-dressing to make the "reforms" that were key to the Lisbon agenda for modernizing the EU more palatable? Europe seems to be facing an internal contradiction between the agenda of competition and privatization (which results in higher access costs to essential services for "low value" customers) and the agenda of abolishing poverty. This contradiction is partly sustained by U.K. data. Which element is and should be more important to the European Union or national governments is hotly debated, but of course serious contributions to the debate require a comprehensive review of the present state of affairs through the type of careful studies of which this volume is an excellent example.
Douglas G. Morris's excellent book poses a broad question: what happened to the rule of law in Germany after 1919? How severe was the collapse of judicial impartiality and competence? Can one doubt whether the Weimar Republic ever qualified as a republic, "if a necessary part of a republic is a judiciary committed to democratic ideals and impartial justice" (p. 1)? That there was a collapse in judicial impartiality is hardly in doubt. As early as 1922, Emil Julius Gumbel provided statistical proof: between late 1918 and summer 1922, a total of 354 political murders committed by perpetrators affiliated with the political right had been punished with one life sentence plus 90 years and 2 months imprisonment; in 326 cases, there had been no punishment at all. By contrast, the 22 murders committed by left-wing sympathizers in the same period had been punished with 10 death sentences, 3 life sentences and 248 years and 9 months imprisonment; only 4 perpetrators escaped (p. 1). To be sure, this statistic may indicate more about the political leanings of police officials and prosecutors investigating cases than of judges who rule on the evidence put before them, but the divergence in sentencing remains remarkable. Morris reformulates this insight to ask how Germany's judges, trained to apply the law in an impartial and technically correct manner, could become raving political partisans willing to twist the law in favor of a particular political position. He does not seek to provide a comprehensive answer, but focuses on cases which involved Max Hirschberg, a Jewish attorney who practiced in Munich from 1911 to 1934, when he escaped to Italy. Hirschberg moved on to the United States in 1939, where he died in 1964. Hirschberg was not only involved in the major political trials of the day in 1920s and early 1930s Munich, but also developed a systematic interest in judicial error, which culminated in a major work on Das Fehlurteil im Strafprozeß, published in 1960. Morris is interested primarily in how trials were conducted. This in-depth analysis is divided into three blocks: political trials in 1922 and 1925, when Germany's war guilt and the causes of defeat were treated in libel suits and criminal prosecutions; non-political cases in which Hirschberg succeeded in having judicial errors reversed; finally, political cases linked with the rise of the Nazi party from 1926. In each case, Morris offers a clear exposition of the facts and substantial as well as legal issues in the case, a step-by-step analysis of trials and appeals processes, and an evaluation of the outcome. The main lines of argument which emerge from these analyses are, first, that some problems were peculiar to Bavaria. The main issue was the existence of people's courts, introduced during Bavaria's brief socialist phase to provide swift justice. The people's courts did not just increase judges' freedom of action by abolishing procedural safeguards, but also protected judges from professional scrutiny and criticism because there were to be no appeals. One of Hirschberg's major victories in the cases of the early 1920s was successful lobbying for their reintroduction. Second, Munich's judges may have been particularly traumatized by the brief revolutionary episode (and by the political preferences of Bavaria's ministries, which were systematically anti-Republican); moreover, they were called upon to decide a stream of political trials, some of which--notably libel trials--effectively sought the impossible, namely a definitive judicial ruling on the validity of a certain interpretation of history or a personal political position. Third, in spite of significant personal variations in style and substance, even after the reintroduction of appeals judges tended to use their freedom of maneuver in an anti-left-wing (which implicitly meant pro-National Socialist) sense. However, until 1933, this state of affairs did not challenge the ties which bound the profession. The Bavarian ministry of justice failed in its attempts to have Hirschberg disbarred in the early 1920s. Even when Hirschberg was released from so-called protective custody in 1934, most of his colleagues rallied round the decorated war veteran, allowing him to retain an access to the court building that was denied most Jewish attorneys. Finally, the problems of the justice system affected non-political cases as well, which may have deepened distrust of Republican institutions. The meticulously researched book benefits immensely from its author's experience as a practicing attorney familiar with courtroom drama and legal technicalities, which are vividly recreated and succinctly explained. The focus on Hirschberg illustrates both the immense obstacles a defense attorney faced and the victories an exceptionally gifted attorney could still win. Even though the courtroom perspective disregards some of the motivations which have their roots outside court--be it the social structure of and career perspectives in Munich's legal profession or political pressures on judges--these are not the main focus of Morris's research. Finally, one could argue about the optimist portrayal of pre-1918 German justice in politically sensitive cases. The clear focus on Weimar trials ensures that the book is no biography. Although Morris includes brief chapters on Hirschberg's youth and his years in exile, not much information is offered on Hirschberg's private life, the economics of his legal practice or his time in exile. But this decision does not diminish Morris's achievement in providing a fascinating insight into the workings of Weimar justice.
The articles in this volume represent anthropological approaches to the study of external and internal boundaries in Europe. The authors raise fascinating methodological and empirical questions by approaching European societies from the perspective of a discipline usually working on the basis of greater cultural distance between scholars and the objects of their research. Moreover, the volume tackles a subject usually understood as a political project and a political problem, E.U. Europe, in an original non-political-science perspective. The volume's case studies are all based on bottom-up views of Europe, with fieldwork the methodology of choice. The first articles focus on institutions. Cris Shore and Daniela Baratieri's article focuses on the ambivalent results of attempts by European schools, which cater mainly to Eurocrats in Brussels and Luxemburg, to replace nationalism with a sense of European identity or nationhood, while Gregory Feldman discusses Estonian programs for the integration of Russian-speakers and Davide Però addresses the position of Italy's left-wing parties and public to the "new immigration." While these essays argue that "Europe" may not be as destructive to national (institutional) boundaries or the nation state as is often supposed, the next block of articles tackles migration across boundaries in a more conventional perspective, focusing on particular immigrant groups. Helen Kopnina discusses Russians in London and Amsterdam, while Christina Moutsou focuses upon immigrants in Brussels and Jacqueline Waldren examines Bosnians in Mallorca. To me, the case study of Turkish migrants in West Berlin by Sabine Mannitz is particularly intriguing, because it uses the peculiar experience of a lesson on Jews' fate in the Holocaust in which the teacher cast immigrants as permanent outsiders in Germany to explore pupils' sense of boundaries, and the East-German West-German divide appeared to loom much larger for immigrants than that between foreigners and Germans. The last section focuses on concrete and contested boundaries in European states and towns: William F. Kelleher, Jr. discusses Northern Ireland, Greek towns are the focus of Venetia Evergeti and Eleftheria Deltsou's article and South Tyrol is examined by Jaro Stacul. The volume makes for diverse and diversifying reading, and can only be highly recommended to anyone interested in innovative perspectives on the fate of the European project.
That God has to become man in order to reveal the being of God to mankind is a belief not only held by Christianity. In Bhagavata Purana, one of the holy scriptures of Hinduism, God Vishnu speaks the sentence quoted above when he is incarnated as Krishna. In a world getting ever smaller, awareness of other religions gains more and more importance. It is my purpose to show what contribution the theological field I represent, ecclesiastical history or historical theology,1 may make towards getting to know other religions and seeking dialogue with them. I will use the worship of Krishna in the following text to exemplify my propositions. My explanations are set out in five parts: (I) two traditions of how God became man; (II) the problem and purpose of inter-religious encounter; (III) historical theology as history; (IV) historical theology as theology; (V) thoughts about dialogue with other religions as an encounter between two things of comparable significance.
In Germany, theological studies on the Hindu religion of the International Soci-ety of Krishna Consciousness and its Vaishnava theology are still only just be-ginning. Previously this relevant task was left mostly to religio-political polemics, resulting in a politically highly problematic research deficit which seriously impeded the necessary social and clerical confrontation with these new religious impulses in the German society. But theological passiveness and polemic activ-ism actually reduce the chances for religiously relevant analyses and socially acceptable solutions of philosophical and spiritual problems. Ignorance rather than dialogue, and polemics inimical to dialogue, have directly or indirectly stabilised the destructive forces in the new religious communities for decades, and consequently favoured a diminution and isolation of reformative tendencies. Due to an increasing respect for the freedom of religion as a human right, the profane alliance of the aggressive forces of both sides has recently ended, and a public, and differentiating, discussion of participants and persons concerned has cautiously started, reinforcing a freer and more competent inter-civil dialogue about spiritual affairs. Clear signs may be seen, not only of a reform within the ISKCON religion, but also in the churches setting about discussing the multi-religious topic on a higher level. A so-called broader theological research, partly transcending the border-lines of Christianity, is developing in the universities, and the free science of religion in Germany is receiving a surprising impetus. It was the suppression of the science of religion that had been impeding a constructive discussion in society of the new religious situation in Germany. The rejection of an inter-civil dialogue of spiritual affairs, however, contradicts an effective democracy which subsists on the continuous confrontation of free citizens with their common culture, especially with the ultimate questions of human existence. But the success of this inter-civil confrontation is solely guaranteed if the participants in the dialogue respect their mutual freedom as citizens and take the mutual dialogue among citizens for granted. This is the only way to attain a reasonable range of solutions concerning the ends of our existence and its proper means. As a contribution to this inter-civil dialogue a theological analysis is to be made of the religious culture practised by citizens of this country engaged in the ISK-CON religion and from there desiring to exert an impact on our civil culture. I. Subject and Aim of Diacritical Theology Because of the diffuse understanding of theology it is necessary to explain what it is, where it should and should not be engaged. Theology is not a religious ideology of a particular community that argues the interests of social organisations, but a universal science. It is not limited to a certain religious culture or form of society but is committed to its specific subject (1). Such an autonomous theology has the task of discrimen inter legem et evangelium—the diacritical analysis of Law and Gospel according to the description of its function by Martin Luther. We will follow these basic categories of diacritical theology and explain them here (2).
As both time and space at hand for this presentation is limited, therefore instead of a longer introductory note, here a move is made to deal with the given subject straight. In the second section the background both historical and theological is discussed, which win state the position of the inter-religious dialogue in India. The third section will deal with the involvement and experiences of the Roman Catholic and Protestant churches in the field of inter-religious dialogue. The fourth section deals with other living religions specially Islam. Finally in section five concluding remarks are given in the form of reflections and in section six, the notes and references are listed.
In recent years the role of 'religion' has generally been considered in the negative term, specially in India. Today, it may be a Kashmir or Punjab problem in North India, but all such problems are attributed to 'religion'. But that is when 'religion' is used at the higher level either by a state or sub-state, or by larger religious communities to protect their special interests. One such good example is of the Babri-Ramjanambhoomi conflict, over a Mosque and Temple, between the two larger communities of India, namely the Muslims and the Hindus. A recent film 'Bombay' in Hindi has well projected this problem from this angle. But then there is also the 'religion' of people, which operates at the lower or local levels, the level of ordinary people, where it plays the role of establishing relations, more correctly it helps building a larger community positively. This lecture deals with the latter form or level of religion. This lecture is based upon the actual case studies. Though these case studies belong to North West India, yet the application of these are applicable generally to the rest of India also. For the sake of convenience this lecture is divided into two parts. In part one, two cases, one from rural and the other from urban areas, dealing with the theme of 'relations in religion' are given, and in part two, some comments, along with a few views of others are offered, and at the end, in the form of concluding remarks a summary of the whole lecture is given.
The Christian culture experienced a deep-going change with the uprising of the Civil Society ("Bürgerliche Gesellschaft"), the industrialization of economic production, the urbanization of life-style and the individualization of religiosity in the 19th century. The Christian formation of inner- and outer-world in those days became obsolete. From this conflict the civil or modern Christianity origi-nated. In a painful changing process most of the people of this new society have newly interpreted religion, moral and ritual of traditional Christianity and cre-ated to their new conditions of life new institutional forms of transmission and realization of Christian cultural heritage. Under the recourse of the Reformato-rian heritage the modern Christianity developed the religious-moral doctrine: A true Christian is before all a citizen who is living in the midst of the world self-determinate and socially engaged fulfilling all his worldly duties; the modern Christian has to get this motivation for a world-oriented existence on his own responsibility because religion is not restricted anymore. ...
Many religious people believe that the integration of world society is of the greatest importance for mankind. They think that the religions of the world should strive to attain this goal through multi-religious agreement, through inter-religious dialogue, even through the merger of their organisations. Religious unification is supposed to be an effective instrument to encourage world society and to guarantee social peace. Religious differentiation, however, is dubious to these people. It would lead to social splintering and would ultimately be anti-social and extremely dangerous, especially to the economic unification of the world. The people who advocate religious unification look upon the progressing cultural, political and economic unification of the world as a model for religious unity. Therefore, many religious people believe that a unified global religion, or at least a union of world religions, should be implemented today. Options of this kind, however, are utopian in the extreme - confronting the ever-expanding conflicts between the established international religious organisations. Pragmatists who espouse the doctrine of religious unification therefore propagate the following fundamental tenets: 1. All religious people believe in the same god or whatever the ultimate reality may be called. 2. Each religion may believe in the ultimate reality in its own way. 3. No religious community is allowed to make converts. 4. Everybody should remain in his original religious community forever. These tenets are in reality nothing but a kind of a cartel agreement. And this agreement should establish an inter-religious combine, which had to stop competition between the religious organisations and to prevent the individual to leave his original religion. The basic supposition of this concept, however, is that religion today has mainly to be seen as an organised, congregational and institutionalised one. And because of this historical error they are only interested to keep the status quo of the established religious organisations. The propagation of that cartel agreement is rooted in the fear, that the established religions wouldn't survive the radical religious revolution at the end of the 20th century.
Modern Hindus use the term 'Hindu' in a positive sense. It is no more a derogatory appellation used by foreigners and oppressors, but a powerful self chosen name. The historically most valid ideologue of that positive Hindu understanding is Narendra Nath Datta (1863-1902). This highly talented son of a regarded lawyer family in Calcutta became disciple of Ramakrishna, the flaming son and priest of the goddess Kali and greatest religious virtuoso in the 19th century. Becoming a sannyasin Narendra received the title and name Swami Vivekananda; after the death of his master he set up the famous Ramakrishna Order. ...
Das genetische Material der Zellen besteht aus Molekülketten der Desoxyribonukleinsäure (DNA), die ein Träger der Erbinformation ist. In normalen Körperzellen wird die Erbinformation der DNA in eine andere Molekülkette, die sogenannte Ribonukleinsäure (RNA), übersetzt. Die RNA reguliert die Bildung von neuem Protein in der Zelle. Dass die RNA nicht bloß ein „Stempel“ ist, der die Informationen der DNA weitervermittelt, darin sind sich die Experten heute einig. RNA-Moleküle können Informationen speichern, katalytische Aktivitäten entfalten, sich perfekt tarnen, und sie regulieren auch als Produkt ihre eigene Synthese. Manche Viren enthalten ebenfalls RNA (oder DNA) und können so den Produktionsapparat der Zelle täuschen. Erkenntnisse über die Wechselwirkung dieser RNA mit natürlichen und synthetischen Liganden können zur Suche nach potentiellen Wirkstoffen beitragen. Nukleinsäuren sind lineare Biopolymere von grundlegenden Untereinheiten, die Nukleotide genannt werden und aus Adenin (A), Cytosin (C), Guanin (G), Urazil (U), und Thymin (T) zusammengesetzt sind. Sie sind jedoch in der Lage sich zu falten und so eine Doppel-Helixstruktur auszubilden. Diese besteht größtenteils aus den bekannten "Watson-Crick-Basenpaaren" (G-C und A-U oder A-T), die zur Stabilität der Struktur beitragen, sowie aus den weniger stabilen G-U-Paaren. Durch die Wechselwirkung zwischen verschiedenen Sekundärstrukturelementen entstehen Tertiärstrukturelemente, deren Struktur und Dynamik oft nur schwer experimentell zu bestimmen sind. Fortschritte in der RNA-Strukturanalyse wurden durch Röntgenkristallographie und Kernresonanzspektroskopie (NMR) möglich. Durch die Röntgenkristallographie wurden viele RNA-Eigenschaften festgestellt. Allerdings besteht keine Kristallstruktur für alle mögliche Einzelnfaser-RNA-Haarnadeln, weil diese immer dazu neigen, in eine linearen doppelte Faserform zu kristallisieren, die geringe biologische Bedeutung hat. Außerdem wurde mit Hilfe der NMR-Spektroskopie das dynamische Verhalten von RNA, z.B. Entfaltungsprozesse bei ansteigender Temperatur, beobachtet. Jedoch erlauben diese experimentellen Daten oft keine direkte mikroskopische Beschreibung der molekularen Prozesse. Molekulardynamik (MD)-Simulationen von biologischen Systemen ermöglichen es hingegen, diese Prozesse in atomischem Detail zu untersuchen. Die MD-Simulation beschreibt ein molekulares System auf atomarer Ebene mit Hilfe der klassischen Mechanik. Kräfte werden von empirischen Potentialen abgeleitet. Sie liefern zeitabhängige Trajektorien, die sich aus den Newton'schen Bewegungsgleichungen ergeben. Durch verbesserte Computerleistung, bessere Kraftfelder, und neu entwickelte genauere Methoden stimmen heutzutage MD-Simulationen von RNA mit experimentellen Daten immer besser überein. In meiner Doktorarbeit wurden MD-Simulationen durchgeführt um die Dynamik, die Struktur und insbesondere die Stabilität von RNA-Hairpins theoretisch zu beschreiben, um so ein erweitertes Verständnis für die dynamischen Vorgänge zu erhalten. Auch der SFB 579 der Universität Frankfurt beschäftigt sich mit RNA-Systemen. Erforscht wird unter anderem der D-Loop des Coxsackievirus B3 (CVB3), der Virenmyocarditis verursacht. Die Interpretation dieser experimentellen Daten wird durch MD-Simulation möglich. In dieser Arbeit wurden das GROMACS Software-Paket und das AMBER Kraftfeld verwendet, um das strukturelle, dynamische und thermische Verhalten der RNA-Hairpins mit Hilfe von MD-Simulationen auf atomarer Ebene zu untersuchen. Betrachtet wurden die 14-mer RNA-Hairpins, uCACGg und cUUCGg. Die verfügbaren NMR-Strukturen zeigen, dass das uCACGg-Tetraloop auffallend ähnlich in der gesamten Geometrie und den Wasserstoffbindungen zu der experimentellen Struktur des cUUCGg-Tetraloop ist, obwohl die schließende Basenpaarsequenz der beiden Tetraloops unterschiedlich sind. Trotz beachtlicher struktureller Ähnlichkeit unterscheiden sich allerdings die uCACGg und cUUCGg Tetraloops in Funktionalität und Thermostabilität. Zunächst orientiert sich unser erstes Bemühen an der Frage nach einem guten Modell für RNA-Hairpins und Simulationsbedingungen, um die zu untersuchenden RNA-Hairpins in Wasser möglichst realitätsnah zu simulieren. Erstens werden drei Versionen des biomolekularen AMBER-Kraftfelds geprüft, indem man die 60 ns Simulationen des 14-mer uCACGg-Hairpins durchführt. Die simulierten strukturellen Eigenschaften und Atomfluktuationen zeigen hohe Ähnlichkeiten in den drei Kraftfeldern. Darüber hinaus stimmen die von MD-Simulationen berechneten Atomkernabstände mit den experimentellen NMR-Daten gut überein. Die gute Übereinstimmung zwischen den Simulationen und den strukturellen NMR Daten belegt die Fähigkeit des AMBER-Kraftfelds zur Beschreibung der strukturellen Eigenschaft von kleinen RNA-Hairpins. Anschließend werden die Einflüsse der Methoden, welche die langreichweitigen, elektrostatischen Wechselwirkungen beschreiben, auf die strukturellen Eigenschaften untersucht. Insbesondere werden die Ergebnisse der Reaktionfeld-Methode mit denen der Particle Mesh Ewald (PME)-Methode verglichen. Es zeigt sich, dass die PME-Methode die elektrostatischen Wechselwirkungen am besten beschreibt, auch wenn die Simulationen der beiden Methoden Ähnlichkeit in der Struktur-Stabilität und der Atomfluktuation bei niedriger Natriumkonzentration aufweisen. Drittens wird der Kationseffekt auf die RNA-Stabilität untersucht. Betrachtet wurden zwei unterschiedliche Kationen (ein- und zweiwertig) und verschiedene Konzentrationen. Die Simulationen weisen darauf hin, dass sich die Metallionen in der Affinität zum RNA-Hairpin unterscheiden, wenn Na+ und/oder Mg2+ als Gegenionen verwendet werden. Weiterhin wird gezeigt, dass sich die bevorzugten Positionen der Na+-Ionen in der großen Furche (major groove) des RNA-Hairpins befinden. Insbesondere die Anlagerungsort der Na+-Ionen liegen in der Nähe des schließenden Basenpaar U5-G10. Im Vergleich zu Na+-Ionen lagern sich Mg2+-Ionen sowohl an die RNA-Basen U3, A4-U11, und die Phosphat-Gruppe, als auch an das schließenden Basenpaar U5-G10 an. Bestätigt werden die Modelle und Simulationsbedingungen durch den Vergleich von Parametern, die sowohl experimentell als auch durch Simulationen ermittelt werden können. Ferner erlauben MD-Simulationen Einblick in das System, indem sie detallierte Konformations- und andere Verteilungen liefern. In der vorliegenden Arbeit wurden die Einflüsse der Loopsequenz und des schließenden Basenpaares auf die Verteilung der Konformationen, der internen Bewegungen, und auf die Thermostabilität von zwei RNA-Hairpins mit Hilfe dieser Modelle untersucht. Zunächst wurden die strukturellen Eigenschaften bei Raumtemperatur ausgewertet. Die starken strukturellen Ähnlichkeiten und die gute Übereinstimmung mit NMR-Daten bestätigen die Hypothese, dass die zwei Tetraloops zur gleichen “erweiterten” RNA-Familie gehören. Diese zwei Hairpins haben ähnliche Lösemittelzugängliche Oberflächen (solvent accessible surface), wobei deren Lösemittel zugänglichen funktionellen Gruppen unterschiedlich sind. Weiterhin weist das uCACGg-Hairpin eine stärkere Tendenz auf Wasserstoffe abzugeben als das cUUCGg-Hairpin, was in den unterschiedlichen Bindungsaffinitäten zwischen diesen Hairpins und der viralen Protease begründet liegt. Darüber hinaus wurde der Faltungs- und Entfaltungsprozess mit Hilfe der Replica-Exchange-Molekulardynamik-Simulationen untersucht. Diese Untersuchung zielt auf das bessere Verständnis der unterschiedlichen Thermostabilität der Hairpins, indem sie die möglichen Zwischenprodukte im atomaren Detail liefern. Sowohl experimentell als auch von den MD-Simulationen ergibt sich eine Differenz in den Schmelztemperaturen der beiden Hairpins von ungefähr 20 K. Allerdings sind die von MD beobachteten Schmelztemperaturen 20 % höher als die von Experiment zu ansehende Wert. Die Ergebnisse machen deutlich, dass die Schmelztemperaturdifferenz nicht auf die Unterschiede in der Sequenz, in der Struktur, oder in der Dynamik der Loops zurückführen sind, sondern auf die Unterschiede der Basenpaaren in den Stämmen. Weiterhin wird gezeigt, dass sich das uCACGg-Hairpin einerseits kooperativ entfaltet, und die Entfaltung des cCACGg-Hairpins anderseits weniger kooperativ stattfindet. Um die schnelle interne Dynamik der uCACGg- und cUUCGg-Hairpins zu untersuchen, erlauben die Simulationen von 50 ns eine akurate Beschreibung der schnellen internen Bewegung der RNA-Hairpin, obwohl der den Hairpins zugängliche Konformationsraum nicht vollständig abgedeckt wird. Die NMR-Relaxationsparameter, die mit Hilfe der MD-Simulationen zurückgerechnet wurden, bestätigen das Modell und die Simulationsbedingungen der MD-Simulationen. Im Hinblick auf die Übereinstimmung kann man den besten Ansatz zur Berechnung der NMR-Ordnungsparameter bestimmen. In dieser Arbeit wurden drei verschiedene Ansätze angewandt, nämlich das Fitting von 100 ps auf modellfreiem Ansatz nach Lipari-Szabo, equilibrium average, und das Gaussian Axial Fluctuation (GAF)-Modell. Die zwei letzteren können nur qualitativ mit den experimentellen Daten übereinstimmen. Die NMR-Ordnungsparameter können mit Hilfe des Modells von Lipari-Szabo richtig ermittelt werden, wenn sich die interne Bewegung in kleineren Zeitskalen als zur Gesamtbewegung vollzieht. Vorausetzung für die Berechnung dieses Modells ist aber, dass das Fitting der internen Korrelationsfunktionen nur auf den ersten Teil von 100 ps der Korrelationsfunktionen eingesetzt wird. Die berechneten Ordnungsparameter deuten auf ein unterschiedliches Verhalten der beiden Hairpins besonders im Loop-Bereich hin. Die konformationelle Umordnung, die beim UUCG-Loop beobachtet wurde, tritt beim CACG-Loop nicht ein. Zusammenfassend lässt sich sagen, dass es durch den Einsatz von MD Simulationen ermöglicht wird, die strukturellen und dynamischen Eigenschaften der RNA-Systeme auf atomarer Ebene zu untersuchen. Als Schlussfolgerung zeigt diese Doktorarbeit, dass sich die Studie der konformationell Dynamik der RNA-Systeme durch die Kombination aus MD-Simulation und NMR-Spektroskopie sowie der Leistungsfähigkeit der MD-Simulationen, die die interne Bewegungen deutlich beschreiben können, untersuchen lässt.
Two types of proteins transport ions across the membrane – ion channels and ion pumps. Ion pumps transport ions against their electrochemical gradient by co-transporting another ion or a substrate molecule through a concentration gradient or by coupling this process to an energy source like ATP. Those that couple ATP hydrolysis to ion transport are called ion motive ATPases and can be classified as ‘V’, ‘F’ and ‘P’ types. In this thesis, two sub-classes of P-type ATPases, PIIIA and PIB were studied. Attempts were made to over-express and crystallize the plant proton pump AHA2 (a PIIIA-ATPase). Also, the two putative copper transporting ATPases, CtrA3 (CopB-like) and CtrA2 (CopA-like) from Aquifex aeolicus (both PIB pumps) were over-expressed in E. coli and characterized. PIIIA-type pumps transport protons across the membrane and are found exclusively in plants and fungi, and probably some archaea. One of the most characterized proton pump biochemically is the A. thaliana proton pump AHA2. An 8Å projection map of this enzyme is already available (Jahn 2001). PIBATPases, also called CPX type pumps transport heavy metal ions such as Cu+, Cu2+, Zn2+, Pb2+, Cd2+, Co2+ across biological membranes and play an important role in homeostasis and biotolerance of these metals. CopA and CopB are two such proteins that transport copper across cell membrane found in many prokaryotes. CopB-like proteins are found almost exclusively in bacteria, with CPH sequence motif, while CopA-like proteins have CPC sequence motif, also found in eukaryotic copper transporters including human ATP7A and ATP7B. CopB extrudes Cu2+ across the membrane. CopA is activated by and transports Cu+ but the direction of transport is debated. Attempts were made to over-express the plant proton pump AHA2 in yeast Pichia pastoris. However, the yeast expressed only a truncated protein, which could not be used for further studies. It can be concluded that P. pastoris strain SMD1163 is not a good host for expression of AHA2. Focus was then shifted to AHA2 that has been over-expressed and purified from S. cerevisiae strain RS72. Growth and purification protocols had to be changed from published methods because of laboratory constraints and this probably had an effect on the protein produced. The protein purified from S. cerevisiae could not be crystallized reproducibly for structural studies by electron microscopy. CtrA3 was expressed in E. coli and purified using Ni2+-NTA matrix. Like CopB of A. fulgidus (Mana Capelli 2003), it was active only in the presence of Cu2+ and to some extent in Ag+. The protein was maximally active at 75°C, at pH 7 and in presence of cysteine. Lipids were essential for the activity of CtrA3. However, when the protein was purified in Cymal-6, CtrA3 could not hydrolyze ATP, even when lipids were added to the reaction mixture. For reconstitution of CtrA3 into liposomes for 2D crystallization, several lipids were tested. To screen the lipids compatible for protein incorporation, CtrA3 was dialyzed with different lipids at a high lipid-to-protein ratio of 10:1 and centrifuged by sucrose density gradient. Protein incorporated in lipids localized with liposome fraction in the gradient. Most of the CtrA3 was incorporated into DPPC with no aggregation. This lipid was used for reconstitution of CtrA3 at low LPRs, and at an LPR of 0.3-0.5, the protein formed 2D crystals. A NaCl concentration of 50mM was necessary for the formation of crystals. However, salt removal by dialysis prior to harvesting was essential for obtaining wellordered lattices of CtrA3. Addition of preservatives like trehalose and tannin or direct plunging in liquid ethane for cryo-microscopy destroyed the crystal lattice. Similar to CtrA3, the gene responsible for expression of CtrA2 was amplified from genomic DNA of A. aeolicus and expressed in E. coli and purified by Ni2+-NTA. Functional characterization of CtrA2 was done by analyzing ATP hydrolysis activity of the enzyme. Similar to CopA of A. fulgidus (Mandal 2002), CtrA2 was activated in the presence of Ag+ and to some extent, Cu+. It is possible that both the copper ATPases of A. aeolicus have different ion selectivity- CtrA3, specific for Cu2+ and CtrA2, specific for Cu+. Maximal activity of CtrA2 was also at 75°C. Cysteine was essential for activity of CtrA2, but the protein was not dependent on addition of lipids for activation. Reconstitution of CtrA2 was done similar to CtrA3 for screening of lipids for 2D crystallization. Of the lipids tested, DOPC reconstituted the protein best. However, screening at low LPRs did not yield any crystals. Even though both CtrA3 and CtrA2 are similar heavy metal transporting Ptype ATPases from the same organism and have 36% identity, they behaved completely different in their expression levels in E. coli, purification profiles, activity and reconstitution in lipids.
Purification and characterization of heterologously produced cannabinoid receptor 1 and G proteins
(2007)
G protein coupled receptors form the largest group of transmembrane proteins, which are involved in signal transduction and are targeted directly or indirectly by 40-50% of the drugs in the market. Even though a lot of biochemical and pharmacological information was acquired for these receptors in the past decades, structural information is still insufficient. G protein coupled receptors are expressed in a very minute scale in the tissues. Purification of G protein coupled receptors, in amounts needed for structural studies, from native tissue is tedious and almost impossible. To overcome this first hurdle of insufficient protein, several heterologous protein expression systems are being used. Another difficulty in structural determination of a G protein coupled receptor is that it is a membrane protein. Membrane proteins are difficult targets for structural studies. One of the possible reasons is the little hydrophilic surface area on the membrane protein, reducing the chances of crystal contact between the molecules. The present work is an attempt to investigate possible ways to overcome these problems. Aim of the project was to use G proteins to increase the hydrophilic area of the G protein coupled receptor. G protein is a physiological partner to the G protein coupled receptor which makes the complex functionally relevant. In the present work five G alpha proteins were purified to homogeneity by a two step purification using metal affinity and ion-exchange chromatography. The G alpha subunits purified were tested for their detergent susceptibility. It was found that only some G proteins were active in the presence of detergent. Observation from contemporary reports also suggest that the G alpha proteins expressed in Escherichia coli, alone may not be sufficient to bind to the G protein coupled receptors in solution. So the project was extended towards expressing a G protein coupled receptor which was reported to exist in a complex with the G proteins, in the cells. Purifying such a functional complex could be more beneficial to use for crystallization. Cannabinoid receptors were chosen for heterologous expression and purification. Production of recombinant cannabinoid receptor 2 was investigated in Pichia pastoris. The protein obtained was highly heterogenous. There were several oligomeric forms as well as degradation products in the cell membranes. Most of the protein was lost in the purification steps leading to a poor yield. Several oligomeric forms and other impurities were still present in the protein sample after purification. Alternatively, a baculovirus mediated insect cell expression system was investigated, to produce the receptors. Cannabinoid receptor 1 was investigated in insect cell expression system because of its better biochemical understanding and pharmacological importance than cannabinoid receptor 2. Cannabinoid receptor 1 was produced in two forms, a full length and a distal carboxy terminal truncated version. All the several gene constructs made could be expressed in the Spodoptera frugiperda (Sf9) insect cells. Expression levels (Bmax) for the constructs with a decahistidine tag at the amino terminus and Strep-tagII at the carboxy terminus were 40 pmol/mg and 53 pmol/mg respectively, for full length and truncated versions. These expression levels are 2 fold higher than the levels reported till now in the literature. As was quite evident from previous experiences of other research groups, purification of this receptor was a challenge. Protein purified from immobilized metal affinity chromatography (Ni-nitrilo tri acetate)(Ni-NTA) was not even 50% pure. A second purification by immobilized monomeric avidin or Streptactin agarose, making use of Biotag and StreptagII respectively, drastically reduced the protein recovery. Later on, purification of receptor was investigated on different metal chelating resins. His-Select, a Ni-NTA based matrix from Sigma, with much lesser density than Ni-NTA from Qiagen, showed a better purification profile. Purification was optimized to get 80% homogeneity but with low yield (20%). Further efforts are needed to improve the yield and purity of the receptor, to use it for crystallization. Cannabinoid receptors are known to exist in a precoupled form to G proteins in the cells. The existence of such precoupled forms of the receptor was investigated using the fluorescence techniques. Guanosine-5-triphosphate binding assay on the cell membranes, in the absence of agonists confirmed the active precoupled form of the receptor. It was found that it is possible to co-immunoprecipitate the complex. These results show that the truncated cannabinoid receptor can be produced in functional form in insect cells in much higher yields than reported. This receptor exists as a complex with G proteins even in the absence of ligands. It was also shown that the receptor/G protein complex can be coimmunoprecipitated. Further work is required to investigate the possibility of purifying this complex to use it for co-crystallization.
G-protein coupled receptors (GPCRs) comprise the largest superfamily of cell surface receptors and possess a signature motif of seven transmembrane helices. The endothelin B (ETB) receptor is a member of rhodopsin like GPCR family. It plays an important role in vasodilation and is found in the membranes of the endothelial cells enveloping blood vessels. Knowledge of the three-dimensional structure of G-protein coupled receptors in general would significantly add to our understanding of their molecular mechanisms and would be useful in the search for new specific drugs. However, three-dimensional structural analysis will require milligram quantities of pure and homogeneous protein. This dissertation is a study of the production, biochemical characterization and preliminary structural studies of the human ETB G-protein coupled receptor. The present work aimed at elucidating the structure and mechanistic details of function of the receptor by using a combination of X-ray crystallographic and NMR methods for collecting structural data. To obtain homogenous and monodisperse receptor protein preparation for structural and functional studies, we implemented the baculovirus expression system for the production of ETB receptor for the present work. The two step affinity purification ensured capture of full-length receptor. Silver stained SDS-PAGE of the purified receptor-ligand complex indicated greater than 90% protein purity. Based on previous reports, we used the high affinity ligand (endothelin -1) binding to the receptor for co-crystallization of receptor-ligand complex by locking the receptor in the activated conformation. As a prerequisite for 3D crystallization trials, the stability of the detergent solubilized receptor-ligand complex was assessed with respect to pH, temperature and time. Receptor-ligand complex did not show any degradation and aggregation over 6 days at 4°C and 18°C. Interestingly, change of pH suggested that receptor-ligand complex is unstable at lower pH due to possible charge induced conformational changes. In our work, we introduced the idea of using fluorophore labeled ligand for simple visual recognition of the receptor-ligand complex during purification and crystallization. On the other hand, we alternatively used biotinylated endothelin-1 to produce an adequate amount of ligand bound receptor complex, thus ensuring homogeneity of the purified complex for use in structural studies. Thus far, preliminary crystals have been obtained for both the unlabelled ET-1 and fluorophore labeled ET-1 complexed with ETB receptor. Moreover, we performed the systematic investigation of the protein/peptide binding partner for the receptor-ligand complex with the chief aims of stabilizing structure and increasing the possibilities of 3D-crystal contacts. Thus subsequent to formation of receptor-ligand complex, the additional in vitro formation of a ternary arrestin-receptor-ligand complex was also attempted for use in structural studies. We successfully demonstrated that arrestin mutant (R169E) forms a tight complex with ETB receptor regardless of its phosphorylation state. A second approach to get insight into the ETB receptor ligand binding site relied on the use of spin isotope labeled ET-1 ligand peptide by employing solid state MAS NMR method. Preliminary data provided compelling evidence that the C-terminal region of the peptide is immobilized in an ordered environment and presumably bound to the receptor. This indicates that the approach is feasible, although there are difficulties in sample preparation for further spectral measurements and data collection which are currently being discussed in ongoing investigations. At this point of our research work, we initiated a collaborative effort to obtain high yields of pure, active receptor without post translational modifications, from an E. coli cell lysate based in vitro expression system. We successfully optimized the production of homogenous and monodisperse endothelin B receptor in mg amounts. Thus this could potentially provide an alternative source of high quality receptor production in large quantities for immediate crystallization trials. Thus we hope that the results from these investigations can be applied in a more general sense to the production and crystallization of other G protein-coupled receptors.
Report of the botanist
(1872)
Background and Purpose of this Meeting With an opening reception sponsored by Thomson Scientific on the evening of Thursday, October 5, the University Library of Frankfurt and the German-North American Resources Partnership (GNARP) and will be hosting an important two-day conference this Autumn in Frankfurt, Germany: »The World According to GNARP: Prospects for Transatlantic Library Partnership in the Digital Age« Sessions at this meeting will explore the wealth of library resources - archival, print, and digital - available to students and researchers (in Germany and the United States) in five selected subject areas: North American Studies, German Studies, Judaica, Africana, and South Asia/India, highlighting both existing avenues (and obstacles) for transatlantic resource sharing along with future prospects. In addition, several other important topics will be highlighted through individual presentations and panel discussions: the future of German as a language of the sciences; existing and planned electronic journal archives in Germany and the U.S.; print and digital repositories; and a special panel on »comparative cataloging cultures« on both sides of the Atlantic. The »World According to GNARP« conference will be taking place simultaneously with the Frankfurt Book Fair, the largest book-related event in the world, attracting annually 285,000 visitors (2005), thus giving participants who arrive early the chance to combine attendance at both the Book Fair and Conference. A cultural event and dinner in Frankfurt are planned for Friday 6th October.
The rate of species extinctions due to anthropogenic activities has dramatically increased within the past few centuries (Dirzo & Raven, 2003; Novacek & Cleland, 2001). Although the mechanisms and ultimate causes leading to the extinction of species remain largely unclear (Frankham et al., 2002), five threats to global biodiversity have frequently been referred to as the most important: habitat destruction and fragmentation, global climate change, hunting and overuse of food resources, biological invasions and environmental pollution (Dudgeon et al., 2006; Lewis, 2006; Novacek & Cleland, 2001). Different research fields, as conservation biology, ecology and ecotoxicology, investigate the effects of these factors on organisms and found strong evidence for their negative impact on regional and global biodiversity.
In most cases, natural populations will be impacted not only by one threat, but rather a combination of them (Buckley & Roughgarden, 2004; Kappelle et al., 1999). Multiple environmental stress factors can have cumulative negative effects on the survival of populations (Sih et al., 2004). To understand, how natural populations respond to combinations of different stress factors is thus of crucial importance in order to understand our present and future impact on all scales of biodiversity (Warren et al., 2001).
The effects of anthropogenically introduced chemicals on organisms and ecosystems are investigated in the field of ecotoxicology. Research in this area has led to a large body of information concerning the impact of chemical stress on the fitness of model species in the laboratory. In contrast to this, there is an obvious lack of knowledge on the effects of contaminants on natural populations and communities (Bickham et al., 2000; Bourdeau et al., 1990). For instance, ecotoxicologists have just started to investigate the impact of environmental pollution on the genetic variability of natural populations (Bickham et al., 2000; Whitehead et al., 2003). Genetic variation provides the raw material for populations in order to adapt to changing environmental conditions and is thus the substrate for evolution and long-term survival of populations and species (Frankham, 2005). The amount of genetic variation in populations is positively correlated with the effective population size (Frankham, 1996). Habitat destruction and fragmentation has divided the ranges of many species into small and isolated refuges. Without migration from adjacent habitats, isolated populations will decrease in their level of genetic diversity through random loss of alleles (Hedrick, 2000). Frankham (1995) for instance, showed that 32 of the 37 endangered species (which occur in small populations per definition) of different animals and plant taxa display reduced levels of heterozygosity compared to closely related and more frequent species.
In strongly human impacted landscapes, both factors, environmental pollution and habitat destruction, can be expected to occur frequently together. It is thus of crucial importance to investigate the impact of reduced genetic diversity and inbreeding on the response to chemical stress. In addition, chemical exposure has frequently been discussed to have an impact on the extent of genetic variability in exposed populations (Guttman, 1994; Staton et al., 2001; van Straalen & Timmermans, 2002). However, evidence for this 'genetic erosion hypothesis' remained scarce to date, most likely because of the difficulty to single out the impact of pollution stress from a background of multiple factors which influence patterns of genetic variability in natural populations (Belfiore, 2001; Staton et al., 2001; van Straalen & Timmermans, 2002).
The Frankfurt University Library possesses one of the outstanding Africana Collections in continental Europe; its regional anddisciplinary scope is unique in Germany. Today about 5,000 new acquisitions a year have accumulated over 200,000 items on Africa south of the Sahara. Some 50,000 historical and rare photographs are fully digitized and freely accessible. Together with a collection of around 18,000 books stemming from the collections of the German Colonial Society at the end of the 19th and the beginning of the 20th century they constitute the historical foundations of the collection. Recently the University Library Frankfurt and the library of the GIGA Institute of African Affairs, Hamburg, started the project ilissAfrica (internet library sub-Saharan Africa), a central subject gateway for online resources and a powerful tool for bibliographic research. These new services will be indispensable for researchers and librarians of African Studies and will promote African studies worldwide.
A commentary on the Synopsis Fungorum in America Boreali Media Degentium, by L. D. de Schweinitz
(1856)
Experimente zum radiativen Elektroneneinfang (REC, Radiative Electron Capture), der Zeitumkehrung der Photoionisation, wie er in Stößen hochgeladener, relativistischer Schwerionen mit leichten Gasatomen auftritt, ermöglicht einen einzigartigen Zugang zum Studium der Photonen-Materie-Wechselwirkung im Bereich extrem starker Coulombfeldern. So ist die REC-Strahlung im relativistischen Bereich zum einen geprägt durch das Auftreten von höheren elektrischen und magnetischen Multipolordnungen und zum anderen durch starke Retardierungseffekte. In Folge dessen wurde der REC-Prozeß in den vergangen Jahren sehr detailliert untersucht, wobei sich die experimentelle und theoretische Forschung auf die Emissionscharakteristik der REC-Photonen konzentrierte, wie z.B. auf Untersuchungen von Winkelverteilungen und Linienprofilen. Mittlerweile kann der REC-Prozeß als ein - selbst für die schwersten Ionen - wohlverstandener Effekt angesehen werden. Allerdings entzog sich den Experimenten bislang eine zur Beschreibung der Photonenmission wesentlich Größe, näamlich die Polarisation der Strahlung. Die lineare Polarisation der REC-Strahlung, wie sie in Stößen zwischen leichten Atomen und den schwersten, hochgeladenen Ionen vorhergesagt wird, war der Gegenstand der vorliegende Arbeit, in der es erstmals gelang, die diese für den konkreten Fall des Einfangs in die K-Schale von nackten Uranionen nachzuweisen und im Detail zu untersuchen. Die hierzu notwendigen experimentellen Untersuchungen erfolgten am Speicherring ESR der GSI-Darmstadt für das Stoßsystem U92+ -> N2 und für Projektilenergien, die im Bereich zwischen 98 und 400 MeV/u lagen. Besonders hervorzuheben ist der Einsatz eines segmentierten Germaniumdetektors, der speziell für den Nachweis linear polarisierter Strahlung im Energiebereich oberhalb 100 keV entwickelte wurde. Die lineare Polarisation der Strahlung wurde hierbei durch eine Analyse der Comptonstreuung innerhalb des Detektors gewonnen. Die durch eine präzise Analyse der Comptonstreuverteilungen gewonnenen Daten zeigen eine ausgeprägte lineare Polarisierung der REC-Strahlung in der Streuebene, die zudem eine starke Abhängigkeit als Funktion der Stoßenergie und des Beobachtungwinkels aufweist. Der detaillierte Vergleich mit nicht-relativistischen und relativistischen Vorhersagen ermöglichte darüberhinaus den Nachweis für das Auftreten starker relativistischer Effekte, die sich allerdings depolarisierend auswirken. Das Experiment wurde am internen Target des ESR-Speicherrings durchgeführt, wobei der Photonennachweis mittels mehrerer Ge(i)-Detektoren erfolgte, die die Ionen-Target-Wechselwirkungszone unter Beobachtungswinkeln zwischen nahe Null und 150 Grad einsahen. Alle Photonendetektoren wurden in Koinizidenz mit einem Teilchendetektor betrieben, um so die volle Charakteristik des REC-Prozesses zu erfassen, also den Einfang eines Targetelektrons in die nackten Uranionen (U92+) unter Emission eines Photons. Für den Polarisationsnachweis entscheidend war der Einsatz eines Germanium-Pixel-Detektors, der abwechselnd unter den Winkeln von 60 und 90 Grad betrieben wurde. Dieser Detektor verfügt über eine 4x4 Pixelmatrix (Pixelgröße: 7x7 mm), wobei die elektronische Information jedes Pixels (Energiesignale und schnelle Zeitsignale) separat registriert und aufgezeichnet wurde. Hierdurch war es möglich Ereignisse, die koinzident in zwei Pixeln erfolgten, zu detektieren und zu analysieren. Dies ist die eigentliche Voraussetzung für den Nachweis der linearen Polarisation bei hohen Photonenenergien, bei dem die Abhängigkeit des differenziellen Wirkungsquerschnitts für Comptonstreuung von der linearen Polarisation der einfallenden Photonen ausgenutzt wird (siehe Klein-Nishina Formel Eq. 2.7). Der Nachweis der Comptonstreuung erfolgt hierbei durch die Detektion des Compton-Rückstoßelektrons (deltaE) und des gestreuten Comptonphotons (hw'), die jeweils separat, aber koinzident in zwei unterschiedlichen Segmenten des Detektors nachgewiesen werden. Hier sei betont, dass für Germanium bereits ab Photonenenergien von ca. 160 keV die Absorption der Strahlung durch den Compton-Effekt über die Photoabsorption dominiert und somit das Ausnutzen des Compton-Effekts prinzipiell eine sehr effektive Technik ist. Der Auswertung der Datenfkam wesentlich zugute, dass der Germanium-Detektor über eine im Vergleich zu Szintillations- oder Gaszählern gute Energieauflösung von ca. 1.8 keV bei 122 keV verfügt. Somit kann durch Bilden der Summenenergie hw = hw' + deltaE für koinzidente Ereignisse die Energie des einfallenden Photons (hw) rekonstruieren werden und als zwingende Bedingung dafür herangezogen werden, dass es sich bei dem Ereignis im Detektor um ein Compton-Event gehandelt hat. Für den Fall linearer Polarisation ist eine wesentliche Aussage der Klein-Nishina-Formel, dass die maximale Intensität für die Compton gestreuten Photonen senkrecht zur Polarisationsebene zu erwarten ist. Tatsächlich zeigen bereits die während des Experiments aufgenommenen Rohdaten für den Fall der untersuchten REC-Strahlung, die durch den Einfang in die K-Schale des Projektils entsteht, dass es sich hierbei um eine stark polarisierte Strahlung handelt, wobei eine erhöhte Intensität für Comptonstreuung senkrecht zur Stoßebene (für den REC-Prozeß definiert durch die Ionenstrahlachse und den Impuls des REC-Photons) festgestellt wurde (vgl. Fig. 7.3). Zur genauen qualitativen Analyse der Meßdaten wurden alle möglichen Pixelkombinationen der (4x4) Detektorgeometrie ausgewertet, wobei jedoch koinzidente Ereignisse benachbarter Segmente ausgeschlossen wurden, um den hier vorhandenenen Einfluß elektronischer Übersprecher zu eliminieren. Zudem erfolgte die Analyse der Daten unter Berücksichtigung verschiedenster Effekte, die einen Einfluß auf die Nachweiseffizienzen für die Compton gestreuten Photonen haben könnten. An prominenter Stelle ist hier die Korrektur zu nennen, die durch die Detektordicke von 1,5 cm und der Pixelgröße von 7x7 cm2 hervorgerufen wird. Zu betonen ist hier, dass für die Auswertung nur relative Effizienzen eine Rolle spielen und so der Einfluß systematischer Fehler, hervorgerufen durch Effizienzkorrekturen, stark reduziert werden konnte (für eine so gewonnene, vollständige Compton-Streuverteilung sei auf Abbildung 9.1 verwiesen, in der die Intensitätsverteilung für Compton-Streuung dargestellt ist). Es sei auch hervorgehoben, dass der Nachweis der Polarisation durch Messungen von vollständigen Compton-Intensitätverteilung im Detektor erfolgte, was das hier diskutierte Experiment wesentlich von konventionellen Polarisationsexperimenten für harte Röntgen- und gamma-Strahlung unterscheidet. Üblicherweise wird in diesen Experimenten die Comptonstreuung ausschließlich in der Reaktionsebene und senkrecht dazu nachgewiesen. Generell weisen die in der vorliegenden Arbeit gewonnen Compton-Streuverteilungen für den K-REC-Prozeß ein ausgeprägtes Maxium senkrecht zur Reaktionsebene auf und bestätigen somit den bereits aus den Rohdaten abgeleiteten Befund, dass die Polarisationsebene der KREC Strahlung in der Reaktionsebene des Stosses liegt. In der Tat kann dieser Befund für alle Energien und Beobachtungswinkel bestätigt werden, die in dem hier diskutierten Experiment verwendet wurden. Hier sei zudem darauf hingewiesen, dass es durch die Erfassung der vollständigen Compton-Streuverteilung möglich war, die Orientierung der Polarisationsebene in Bezug auf die Stoßebene mit hoher Präzision zu erfassen. So konnte z.B. bei der Stossenergie von 400 MeV/u und dem Winkel von 90 Grad, die Orientierung der Comptonstreuverteilung in Bezug auf die Stoßebene zu ph=90 Grad bestimmt werden. Dieser Befund könnte für die Planung zukünftiger Experimente zum Nachweis polarisierter Ionenstrahlen entscheidend sein, da eine Abweichung von der ph = 90 Grad Symmetrie nur durch das Vorhandensein polarisierter Teilchen erklärt werden kann. Dieser Effekt, der in neuesten theoretischen Behandlungen im Detail untersucht wurde, stellt gleichsam einen neuen Zugang zur Bestimmung des Polarisationsgrads der Projektile dar. Hierdurch wird die Stärke der hier angewandten Technik verdeutlicht, die auf dem Einsatz eines ortsempfindlichen Germanium-Pixel- Detektors beruht. Die Bestimmung des genauen Polarisationsgrades für die K-REC-Strahlung erfolgte durch eine X2-Anpassung der Klein-Nishina-Formel an die experimentellen Daten. Die hieraus resultierenden Daten zeigen für alle Strahlenergien und Beobachtungsgwinkel eine starke Polarisation von etwa 80%, wobei die experimentelle Unsicherheit im 10% Bereich liegt. Letztere ist im wesentlichen auf die statistische Genauigkeit zurückzuführen. Die Daten wurden zudem eingehend mit theoretischen Vorhersagen verglichen. Die Theorie stützt sich auf eine vollständige relativistische Beschreibung des REC-Prozesses unter Verwendung exakter Wellenfunktionen für das Kontinuum und den 1s Zustand in wasserstoffartigem Uran. Typischer weise mußten bei den Rechnungen sowohl elektrische wie auch magnetische Multipolterme bis hin zu L=20 verwendet werden, um Konvergenz zu erreichen. Der Vergleich zeigt eine hervorragende Übereinstimmung zwischen Experiment und Theorie. Zudem verdeutlicht der Vergleich mit der ebenfalls diskutierten Vorhersage der nicht-relativistischen Dipolnäherung die Bedeutung relativistischer Effekte (vor allem das Auftreten höherer elektrischer und magnetischer Multipole), die für die Emission der REC-Strahlung bei hohen, relativistischen Energien und hohem Z charakteristisch sind. Offensichtlich wirken sich diese Effekte stark depolarisierend aus. Dass in der Tat eine Zunahme der depolarisierenden Effekte mit einer Zunahme der Strahlenergie verbunden ist, wird auch durch die Daten dokumentiert, die für den Beobachtungswinkel von 60 Grad als Funktion des Projektilenergie untersucht wurden. Die in der vorliegenden Arbeit gewonnenen Resultate für die Polarisation der REC-Strahlung ebenso wie die neuartige Experimenttechnik, die hierbei zum Einsatz kam, lassen für die nahe Zukunft eine Serie von weiteren Polarisations-Experimenten erwarten. Hierbei könnte der REC-Strahlung und deren Polarisation als Mittel zur Diagnostik und zum Nachweis des Polarisationsgrades gespeicherter Ionenstrahlen eine Schlüsselrolle zukommen. Als Detektorsysteme werden hierzu zwei-dimensionale Germanium- und Silizium-Streifen-Detektoren zum Einsatz kommen bzw. Kombinationen aus zweidimensionalen Silizium- und Germanium-Detektoren, sogenannte Compton-Teleskope. Diese Compton-Polarimeter, die gegenwärtig für neue Experimentvorhaben am ESR-Speicherring entwickelt werden, verfügen über eine wesentlich verbesserte Ortsauflösung (z.B. 1x1 mm2) und somit über eine wesentlich gesteigerte Nachweiseffizienz für die Comptonstreuung (ein bis zwei Größenordnungen). Hierdurch sollte es möglich sein, den für Polarisationexerperimente zugänglichen Energiebereich wesentlich auszudehnen, sodass selbst die charakteristische Strahlung der Schwerionen (ca. 50 bis 100 keV) für solche Experimente zugänglich wird.
Physical soil properties feature high spatial variabilities which are known to affect geophysical measurements. However, these variations are not considered in most cases. The challenging task is to quantify the influence of soil heterogeneities on geophysical data. This question is analysed for DC resistivity and GPR measurements which are frequently used for near-surface explorations. To determine the pattern of electric soil properties in situ with the required high spatial resolution, geophysical measuring techniques are methodically enhanced. High-resolution dipole-dipole resistivity measurements are used to determine the electric conductivity distribution of the topsoil. Due to the small electrode separations, the actual electrode geometry has to be considered and an analytic expression for geometric factors is derived instead of assuming point electrodes. Two methods are used to determine soil permittivity with GPR:(i) the coefficient of reflection at the interface air-soil is measured with an air-launched horn antenna, (ii) the velocity of the groundwave is measured with a new setup using two receiver antennas enhancing the lateral resolution from in the best case 0.5 m for standard techniques to approximately 0.1 m with the new technique. With the optimised measuring techniques, the electric properties of sandy soils are determined in the field. Conductivity and permittivity show high spatial variability with correlation lengths of a few decimetres. Geostatistical simulation techniques are used to generate synthetic random media featuring the same statistical properties as in the field. FD calculations are carried out with this media to provide realistic synthetic data of resistivity and GPR measurements. Conductivity variations as determined in the field generate significant variations of simulated Schlumberger sounding curves resulting in uncertainties of the inverted models. Even in pedologically homogeneous sandy soil, moisture pattern and resulting permittivity variations cause strong GPR diffractions as demonstated by FD calculations. This influences the detectability of small objects such as e.g. landmines or of large reflectors as e.g. the groundwater table. Conductivity variations as typical for soils showed to have a minor effect on GPR measurements than variations of permittivity. In summary, geostatistical analysis and simulation provide a powerful tool to simulate geophysical measurements under field conditions including soil heterogeneity which can be used to quantify the uncertainty of field measurements by geologic noise.
The present publication is intended to be a monograph on the family of Burmanniaceae. It is divided into three parts: General Part, Critical Part and Taxonomical Part. The first part, General Part, contains general remarks on the taxonomy, distribution and use of the family. The second part, Critical Part, contains general and geobotanical remarks on the genera of the family, whereas the third part, the Taxonomical Part, gives the determination keys to the tribes, subtribes, genera, sections, subsections and species, the description of these groups with literature, distribution and the indications of the types. New varieties, species and larger groups are described in the taxonomical part in foot-notes.
Shaped by some of the most dramatic tectonic events of the Cenozoic, the parts of southern and eastern Asia that have become known as the Oriental faunal region comprise vast areas of great geological complexity and ecological diversity. One of the four major groups of terrestrial elapid snakes in this region is the genus Bungarus. These nocturnal and predominantly ophiophagous snakes are widely known as kraits and are an important cause of snakebite mortality throughout their wide range that extends from Afghanistan to Vietnam and eastern China, and south to the Indonesian islands of Java and Bali. Although present on Borneo, kraits have not been found on any island of the Philippines, nor on Lesser Sunda Islands east of Bali. Despite their medical significance and the great importance of Bungarus toxins as tools in neuropharmacology, krait systematics and taxonomy have remained largely unstudied. Twelve species of Bungarus were recognized at the beginning of the present study. Many of these are rare in collections, and most aspects of their biology are unknown. While some species are highly distinct, most kraits are conservative morphologically, rendering molecular methods invaluable for the study of their diversity and biogeography. This study is the first to address the relationships within Bungarus and the historical biogeography of kraits based on molecular evidence. I inferred phylogeographic relationships based on analyses of new nucleotide sequences of the entire mitochondrial cytochrome b gene of 51 kraits and partial NADH dehydrogenase subunit 4 sequences of 40 kraits which I analyzed together with a representative sample of 32 published elapid and non-elapid outgroup taxa using Bayesian, maximum-likelihood, maximum-parsimony and neighbor-joining methods. I then used the recovered phylogeny to investigate the evolution of selected morphological characters and, together with collections-based geographical distribution information, in dispersal-vicariance analyses with models of variable taxonomic and biogeographic complexity. The phylogenetic analyses demonstrate that the current taxonomy of kraits does not adequately represent either the relationships or the genetic diversity in this genus. In contrast, I identified monophyletic groups that are congruent with recognized biogeographic units as well as extensive ecomorph evolution and morphologically cryptic speciation. The following additional conclusions are collectively supported by the mitochondrial phylogeny and morphological as well as biochemical synapomorphies: (1) Kraits are monophyletic with respect to the remaining taxa of the Elapidae; (2) Bungarus flaviceps and Bungarus bungaroides form the monophyletic sister clade of a clade formed by B. fasciatus, black-and-white-banded, and uniformly black taxa; (3) the remaining taxa are divisible into two sister clades, the South Asian species (Bungarus sindanus (Bungarus caeruleus, Bungarus ceylonicus)) vs. Himalayan, Burmese, Southeast and East Asian taxa; (4) within the latter, Burmese taxa form the sister clade to Southeast and East Asian taxa; (5) the widespread and medically significant species Bungarus candidus and Bungarus multicinctus are paraphyletic. The results of this study highlight the importance of vicariant geological events and sea level fluctuations for the cladogenesis of kraits. Events of particular importance in the evolution of kraits include the uplift of the Indo-Burman ranges (Arakan-Naga Hills) which separated black-and-white banded kraits in India and Southeast Asia, and the uplift of mountain ranges in Yunnan, China (e.g., the Gaoligong Shan), which coincided with lineage separation in two distantly related clades of kraits. Alternating dispersal and vicariance events due to Pleistocene climatic and sea level changes have caused complex phylogeographic patterns in kraits in Southeast Asia. Zones of contact between closely related evolutionary lineages of the B. candidus complex are identified in Thailand, Vietnam, and southern China (Hainan). Within this complex, two main clades are revealed. One includes populations from the Southeast Asian mainland and is in contact with B. multicinctus in southern China. The other consists of populations from Thailand, southern Vietnam, Java, and Bali. The phylogeny as well as genetic distances suggest a scenario in which a Pleistocene southward dispersal of B. candidus to Sumatra, Java, and Bali during times of low sea levels was temporarily interrupted by vicariant events (rising sea levels, especially flooding of the Malacca Strait between Sumatra and the Malay Peninsula, and of the Bali Strait between Java and Bali). In this context, the close phylogenetic relationship between haplotypes from southern Vietnam and those from Java and Bali suggests that "southern" B. candidus dispersed directly via colonization of the widely receded South Chinese Sea, and not by taking a detour via the Malay Peninsula and Thailand, which were already inhabited by other populations of B. candidus. Using these phylogenetic estimates as the framework for a study on the diversity and evolution of krait venom components, I applied biochemical and molecular genetic approaches to identify and quantify polypeptide and protein toxins in krait venom, focusing on the distribution and molecular evolution of alpha-bungarotoxin, an irreversible competitive antagonist of nicotinic acetylcholine receptors with an exceptionally high applied significance as a receptor probe. I was specifically interested in the medically relevant question of intraspecific and interspecific variability in toxin diversity, and whether receptor-binding postsynaptic toxins evolve at rates different from those of presynaptic neurotoxins like beta-bungarotoxin, which act by destroying the nerve terminal and are believed to exhibit hypervariable functional diversification due to an accelerated mode of molecular evolution. In the context of this question, I isolated and purified the major lethal neurotoxins from B. candidus venoms by sequential steps of liquid chromatography for structural and functional characterization studies. Cloning and sequence analysis of toxin-coding genomic DNAs showed that the gene encoding the alpha-bungarotoxin alanine-31 variant, originally isolated from B. multicinctus venom, is widely present and highly conserved in multiple populations of B. candidus and is expressed as the principal postsynaptic neurotoxin at least in Javan B. candidus. In addition to the widespread presence of genomic DNAs encoding the alpha-bungarotoxin alanine-31 variant, the present study also revealed the partial genes of three novel alpha-bungarotoxin isoforms in addition to the previously known alanine-31 and valine-31 variants, all of which share an invariant exon 3 coding region. While alpha-bungarotoxin is the principal postsynaptic neurotoxin of Taiwanese B. multicinctus and Javan B. candidus, the main postsynaptic neurotoxin of Thai B. candidus both by quantity and lethality was a novel polypeptide of similar toxicity with a mass of 8030 Da and 73 amino acid residues, whose characterization at the genetic and protein levels revealed a novel subgroup of krait neurotoxins, here named alpha-delta-bungarotoxins and represented by four sequences from Bungarus caeruleus and B. candidus. alpha-delta-Bungarotoxins share high sequence homology with alpha-bungarotoxins but the purified, 8030 Da alpha-delta-bungarotoxin-1 exhibits only reversible, low affinity binding to nicotinic receptors and high site-selectivity for the acetylcholine binding site at the alpha-delta-subunit interface of the receptor. These properties render alpha-delta-bungarotoxin not only the first snake long-chain neurotoxin with reversible binding and binding-site selectivity, but also an exciting natural tool with which to address structure-function relationships at the subunit interfaces of the human receptor. The results of comparisons of the number of non-synonymous nucleotide substitutions per nonsynonymous site (dN) to the number of synonymous nucleotide substitutions per synonymous site (dS) strongly suggest that positive selection is acting on exon 2 of the alpha-bungarotoxin and probably also of the alpha-delta-bungarotoxin genes. In addition, the numbers of nucleotide substitutions per site of intron (dI) compared to the dS value of the toxin-coding exon regions provide strong evidence for accelerated molecular evolution in exon 2 of alpha-delta-bungarotoxins —whose value of dI is only one-eighth of the value of dS—whereas the hypothesis of accelerated evolution is rejected for 13 unique genomic DNAs encoding five alpha-bungarotoxin isoforms from B. candidus and B. multicinctus....
This paper documents the methodology underlying the construction of a global database of gross foreign asset and liability positions for 153 countries over the period 1970 to 2004 and illustrates some key data characteristics. The data cover both inflows and outflows of capital and thus allow for an assessment of the degree of international financial integration. In addition to net foreign asset stocks, we also provide details on the composition of the main asset and liability categories, namely the foreign direct investment, equity investment and debt components. Finally, we report on valuation changes as one of the main sources of discrepancy between transaction-based capital flow data and stock values of investment positions. The dataset is available for download at www.ifk-cfs.de/fileadmin/downloads/data/cfs-icfd.zip. or http://publikationen.ub.uni-frankfurt.de/volltexte/2007/4855/original/cfs-icfd.zip JEL Classification: F21; F34; F32
In this paper we revisit medium- to long-run exchange rate determination, focusing on the role of international investment positions. To do so, we develop a new econometric framework accounting for conditional long-run homogeneity in heterogeneous dynamic panel data models. In particular, in our model the long-run relationship between effective exchange rates and domestic as well as weighted foreign prices is a homogeneous function of a country’s international investment position. We find rather strong support for purchasing power parity in environments of limited negative net foreign asset to GDP positions, but not outside such environments. We thus argue that the purchasing power parity hypothesis holds conditionally, but not unconditionally, and that international investment positions are an essential component to characterizing this conditionality. Finally, we adduce evidence that whether deterioration of a country’s net foreign asset to GDP position leads to a depreciation of that country’s effective exchange rate depends on its rate of inflation relative to the rate of inflation abroad as well as its exposure to global shocks. JEL Classification: F31, F37, C23
An evaluation scheme is presented in this paper which can be used to assess groundwater vulnerability according to the requirements of the European Water Framework Directive (WFD). The evaluation scheme results in a groundwater vulnerability map identifying areas of high, medium and low vulnerability, as necessary for the measurement planning of the WFD. The evaluation scheme is based on the definition of the vulnerability of the Intergovernmental Panel on Climate Change (IPCC). It considers exposure, sensitivity and the adaptive capacity of the region. The adaptive capacity is evaluated in an actors' platform, which was constituted for the region in the PartizipA ("Participative modelling, Actor and Ecosystem Analysis in Regions with Intensive Agriculture") project. As a result of the vulnerability assessment, 21% of the catchment area was classified as being highly vulnerable, whereas 73% has medium vulnerability and 6% has low vulnerability. Thus, a groundwater vulnerability assessment approach is presented, which can be used in practice on a catchment scale for the WFD measurement planning.
Global modelling of continental water storage changes : sensitivity to different climate data sets
(2007)
Since 2002, the GRACE satellite mission provides estimates of the Earth's dynamic gravity field with unprecedented accuracy. Differences between monthly gravity fields contain a clear hydrological signal due to continental water storage changes. In order to evaluate GRACE results, the state-of-the-art WaterGAP Global Hydrological Model (WGHM) is applied to calculate terrestrial water storage changes on a global scale. WGHM is driven by different climate data sets to analyse especially the influence of different precipitation data on calculated water storage. The data sets used are the CRU TS 2.1 climate data set, the GPCC Full Data Product for precipitation and data from the ECMWF integrated forecast system. A simple approach for precipitation correction is introduced. WGHM results are then compared with GRACE data. The use of different precipitation data sets leads to considerable differences in computed water storage change for a large number of river basins. Comparing model results with GRACE observations shows a good spatial correlation and also a good agreement in phase. However, seasonal variations of water storage as derived from GRACE tend to be significantly larger than those computed by WGHM, regardless of which climate data set is used.
Metabotropic glutamate receptor subtype 7 (mGluR7) belongs to the family of G-protein coupled receptors. mGluR7 is widely distributed in the brain and primarily localized at presynaptic terminals, where it is thought to regulate neurotransmitter release and synaptic plasticity. Studies have shown that the intracellular C-terminal tail of mGluR7 binds a variety of proteins in addition to trimeric G-proteins. These newly identified protein interactions are believed to play a key role in the synaptic targeting and G-protein dependent signaling of mGluR7. Protein interacting with C kinase 1 (PICK1), a PDZ-domain protein, is a strong interaction partner of mGluR7a. In order to investigate the role of PICK1 in the synaptic trafficking and signaling of mGluR7a, a knock-in mouse line in which the interaction of mGluR7a and PICK1 is disrupted was generated. Analysis of the mutant mice by immunocytochemistry and immunoelectron microscopy showed that the synaptic targeting and clustering of mGluR7a was not altered, indicating that PICK1 is not required for mGluR7a receptor membrane trafficking and synaptic localization. However, when the spontaneous synaptic activity of cerebellar granule cell cultures prepared from both wild-type and knock-in mice was monitored, and L-AP4 (400μm) was found to decrease the frequency, but not the amplitude, of spontaneous excitatory currents in wild-type neurons, while no effect of L-AP4 on spontaneous synaptic activity was observed in knock-in neurons. This indicates that PICK1 binding to the C-terminal region of mGluR7a plays an essential role in mGluR7a mediated G-protein signaling. We examined the threshold sensitivity for the convulsant pentetrazole (PTZ) in knock-in mice. It was found that mGluR7a knock-in mice had a greater sensitivity to PTZ than wild-type mice. Moreover, the surface parietal cortex EEG recordings of the mutant mice revealed spontaneous synchronous oscillation, or "spike-and-wave discharges" (SWD), which displayed similar characteristics to absence-like seizures. It was also observed that the knock-in mice responded to pharmacology as human absence epilepsy. These data suggests that the knock-in mice displayed the phenotype of absencelike epilepsy. Furthermore, the behavioral analysis of the mGluR7a knock-in mice showed no deficits in motor coordination, pain sensation, anxiety as well as spatial learning and memory, thus the interaction of mGluR7a and PICK1 appears not to contribute to these physiological processes. Taken together, our data provides evidence for an important role of PICK1 in Gprotein dependent signaling of mGluR7a, whereas PICK1 is not required for synaptic targeting and clustering of mGluR7a. Our results also provide an animal model of absencelike epilepsy generated by disruption of a single mGluR7a-PDZ interaction, thus creating a novel therapeutic target against this neurological disease.
The main subject of the thesis is the investigation of low-temperature-grown (LTG) GaAs-based photoconductive switches used in the generation of continuous-wave (CW) and pulsed terahertz (THz) radiation. The use of photoconductive switches based on low-temperature-grown GaAs proved to be a viable option in generating electromagnetic transients on a subpicosecond time-scale, corresponding to frequencies of ~1012 Hz (between microwave and far-infrared). The most appealing property of LTG-GaAs is the ultra-short carrier lifetime obtained by incorporation of a large number of As defects when GaAs is grown at low temperatures. However, the reason for poor THz emission efficiency (low CW-THz power lrvrls) is still up to this date not fully understood. The various reasons are to be found in both, optoelectronic properties of the active layer (photoconducting material) as well as in the device characteristics. The thesis focuses primarily on the limitation imposed to the performance of the THz emitters by the material of choice for the active layer (LTG-GaAs) and secondarily, on the impact of a particular emitter design on the THz radiation efficiency. In the beginning of the thesis one finds an ample overview on the electrical and optical properties of the LTG-GaAs material. A special chapter deals with the main features of current-voltage and CW-THz emission characteristics measured from a photoconductive antenna employed as photomixer. We observed deviations from the theoretical predictions of photomixing theory which were explained by considering the high-field electrons effects (velocity overshoot and elongation of the carrier trapping time). With the scope to provide a better understanding of the correlation between device and material properties when the LTG-GaAs material is integrated with a planar antenna (photoswitch), a special THz double-pulse technique (THz-pump and -probe) was implemented. The experimental results assisted by modeling of the double-pulse THz data provide a gainful insight into the ultrafast dynamics of the electrical field and photogenerated carriers. The outcome of the double-pulse experiments is the evidence for long-living carriers in the LTG-GaAs-based photoconductive antenna under applied bias, with a deleterious impact upon the emitter performance (especially for the CW case). Additionally, by measuring the THz transients generated by a constant laser pulse with and without a CW laser background illumination, we obtained further evidence of strong field-screening effects. This phenomenon was also attributed to the existence of long-living space-charge effects. For both cases (pulsed as well as CW) we derived the de-screening time constant. The principal conclusion of the present study is that, besides shortcomings imposed by the THz-circuitry, photomixers based on materials with traps (defects) exhibit great “affinity” for space-charge screening effects with cumulative and therefore long-lived deleterious impact upon device’s performance. An alternative would be the usage of a transient-time limited device where the response time is given by the carrier collection time, possibly with only one type of carrier responsible for THz signal generation.
As if to bear out the tenet of this study, the field of black British literature has been transformed enormously over the last ten years or so, while this book was in the making. And for myself, too, this has been a formative process. During this time I’ve been supported, challenged, and encouraged by more colleagues and friends than I can acknowledge here. ...
Constructive waterfalls
(1911)
The excavation of valleys by waterfalls is one of the best known and most effective processes by which rivers cut down the surface of the earth. The influence of waterfalls is usually regarded as solely destructive, and as always helping to lower the land. They undermine and cut backward the rock faces over which they fall : by this recession they excavate deep gorges ; and the existence of these gorges enables the adjacent country to be lowered to the level of the valIey floors. The waterfalls, moreover, empty any lakes they rnay reach in their retreat, while the ravines below the falls may drain the springs and thus desiccate the neighbouring hihlands. Observations in various countries had suggested to me that waterfalls may sometimes be constructive in stead of destructive, and that they may reserse their usual procedure, advancing instead of retreating, filling valleys instead of excavating them, and forrning alluvial plains and lakes instead of destroying them. The best illustrations I have seen of such advancing, constructive waterfalls are on some rivers of Dalmatia and Bosnia, where they occur in various stages of development. ...
Safety concerns associated with the use of viral vectors in gene therapy applications have attracted considerable attention towards the development of nonviral vectors as alternatives for DNA delivery. While nonviral vectors are commonly not associated with safety problems, they are still very inefficient compared to viral vectors, and require significant improvements to approach the efficiency of their viral counterparts. Meanwhile ligands or single-chain antibody fragments that bind to cell surface receptors for increased and/or specific cellular uptake, endosome escape activities, and nuclear localization sequences (NLSs) to enhance transport of plasmid DNA into the nucleus, have become available that can be incorporated into nonviral vectors to improve their efficacy. However, as gene delivery is a multistep process, the challenge is to incorporate multiple of these functional elements into a single nonviral vector system, while retaining their specific activities. A promising method to attach such entities to plasmid DNA is the use of multifunctional fusion proteins that bind to DNA through a DNA-binding domain. In principle, two types of DNA-binding domains/proteins can be used to anchor additional functional domains or peptides to a plasmid, namely sequence-specific DNA-binding domains, described in the first part of this thesis, or those that bind DNA independent of its sequence, exemplified in the second part of this work by a derivative of the human HMGB2 protein. The first fusion protein constructed and analyzed contained the E. coli LexA repressor as a sequence-specific DNA-binding domain. In addition, this DNA-carrier protein, termed TEL, included a bacterial translocation domain as an integrated endosome escape activity, and human TGF-a for specific targeting to the EGF-receptor (EGFR). TEL was expressed in E. coli and purified under both native and denaturing conditions. Purified, denatured TEL was refolded and subsequently shown to bind specifically to EGFR-expressing cells. However, inclusion of TEL in complexes of plasmid DNA and poly-L-lysine (pL) did not lead to increased gene delivery into EGFR-expressing COS-1 cells. Most likely this was due to the absence of DNA-binding activity of the LexA moiety in TEL. In contrast, native TEL was able to interact specifically with DNA. Nevertheless, since this interaction was rather weak, and refolding of denatured TEL had not resulted in functional activity of all of its protein domains, it seemed unlikely that fusion proteins containing LexA would exhibit gene transfer capabilities superior to those of similar DNA-carrier proteins previously constructed in our group. Further work therefore focused on the use of the E2C-Sp1C protein as an alternative sequencespecific DNA-binding domain. This artificial zinc-finger protein was fused to the single-chain antibody fragment scFv(FRP5), directed against the human ErbB2 growth factor receptor. The resulting 5-E2C fusion protein was expressed in E. coli and purified under native and denaturing conditions. Refolded and native 5-E2C were found to bind specifically to ErbB2-expressing cells, indicating that scFv(FRP5) in 5-E2C was functional in both preparations. In contrast, whereas refolded 5-E2C bound DNA only weakly, significant DNA binding was observed for native 5-E2C. In addition, it could not only be shown that the interaction of native 5-E2C with DNA containing its recognition sequence was specific, but also that this protein was able to bind DNA and recombinant ErbB2 simultaneously, demonstrating the functionality of both domains in native 5-E2C. Despite these encouraging results, the inclusion of native 5-E2C in pL- or polyethyleneimine (PEI)-DNA complexes did not lead to an (5-E2C-specific) enhancement of gene transfer efficiency, irrespective of the presence of the endosome-disruptive reagent chloroquine during transfection. In the second part of this thesis an alternative approach for the development of DNA-carrier proteins for nonviral gene delivery is described, based on human HMGB2, a DNA-binding protein without sequence specificity. HMGB2 contains an acidic C-terminus that has been found to decrease the affinity of the protein for DNA. Therefore, this C-terminal tail was deleted, resulting in an HMGB2-variant consisting of amino acids 1-186. HMGB2186, purified under native conditions from E. coli lysates, was able to interact with DNA and bound to the surface of different cell lines. Importantly, after binding to plasmid DNA HMGB2186 mediated gene delivery into COS-7 cells with higher efficiency than pL. In addition, HMGB2186-mediated gene transfer was strongly enhanced in the presence of chloroquine, indicating that the endocytic pathway was involved in cellular uptake. To improve internalization and intracellular routing of HMGB2186 as a DNA-carrier, a derivative containing the TAT47-57 cell-penetrating peptide (CPP), reported to facilitate cell entry independent of endocytosis, was constructed. Since this peptide also contains an NLS, in addition an HGMB2186-variant containing the SV40-NLS was constructed to investigate the effect of a peptide that has only nuclear localizing properties. Interestingly, the resulting TAT-HMGB2186 and SV40-HMGB2186 fusion proteins displayed DNA-binding activities similar to HMGB2186, but mediated gene delivery into different cell lines clearly more efficiently than the parental molecule. Furthermore, the efficacy of both fusion proteins was enhanced markedly in the presence of chloroquine, an indication that endocytosis was involved in the transfection process mediated by these proteins. This suggests that the increased transfection efficiency observed for TAT-HMGB2186 was more likely due to the NLS function present in the TAT47-57 peptide, rather than to its ‘cell penetrating properties’. Finally, the incorporation of functional peptides derived from human proteins into HMGB2186 was investigated. An uncharged CPP originating from Kaposi-FGF, reported to facilitate efficient cellular uptake of fused protein domains in an endocytosis-independent manner, was fused to HMGB2186 together with the SV40-NLS. Interestingly, the resulting KSV40-HMGB2186 fusion protein bound DNA similarly as previously tested DNA-carrier proteins, but did not mediate enhanced transfection compared to HMGB2186. In addition, the importin-b-binding (IBB) domain derived from human importin-a2 was investigated as a component of a DNA-carrier protein. Since the IBB domain can function as an NLS, it was fused to HMGB2186 resulting in the DNA-carrier protein IBBHMGB2186. Although IBB-HMGB2186 bound DNA in a similar manner as the other HMGB2186-derivatives, gene delivery mediated by IBB-HMGB2186 was only as effective as HMGB2186 mediated transfection, suggesting no significant role of the IBB domain. However, addition of chloroquine resulted in a remarkable enhancement of IBB-HMGB2186-mediated gene transfer, which was now more efficient than with any other HMGB2186-variant tested, and not much lower than gene transfer mediated by PEI, one of the most efficient transfection reagents available to date. To enhance nonviral gene delivery even further, the HMGB2186-based DNA-carrier proteins described in this thesis might now serve as building blocks for novel fusion proteins that include additional complementing activities. In this respect it seems particularly promising that, under conditions of effective end some escape, IBB-HMGB2186, which consists entirely of protein domains of human origin, was the most efficient of all proteins tested in this work.
On seatangle tent
(1869)
RcsB is a central transcriptional regulator in enteric bacteria involved in exopolysaccharide (EPS) biosynthesis, in cell division, in the expression of osmoregulated genes, and regulates at least 20 other genes and operons. It is a member of a phosphorelay system and signal transfer is mediated by phosphorylation through the RcsC/YojN phosphorelay. RcsB proteins modified with the phosphorylation mimic BeF3- as shown by its conformational changes and DNA binding properties and resulted phosphorylated RcsB derivatives with sufficient stability. Both, the wild type RcsB protein and the mutant RcsBD11A could be modified with BeF3-. Non-phosphorylated RcsB has been shown to bind as a heterodimer with the coinducer RcsA at the conserved RcsAB box in Rcs regulated promoters. In this study, it has been shown that the modification of RcsB by BeF3 - (I) has a negative effect on its homodimerization, (II) abolishes the complex formation of RcsAB with the RcsAB box as shown by the EMSA and SPR technique. All the effects were found to be reversible by increasing the NaF concentration in the assays presumably leading to the formation of the inactive BeF4 2- salt. This hypothesis of RcsB being modified by BeF3- was also supported by other phosphodonors like ATP and acetyl phosphate, both of them showed the same negative effect on DNA binding by RcsAB heterodimer giving evidence that BeF3- could be used as a phosphorylation mimic. In addition, the phosphorylation mimic BeF3- was found to be a better phosphorylating agent than ATP and acetyl phosphate. This is the first evidence that phosphorylation of RcsB might have a negative effect on the activation of RcsAB regulated operons. Autophosphorylation of RcsB proves that it has the ability to take up phosphoryl groups and the mutant protein also become autophosphorylated with less efficiency or stability than the wild type protein. RcsB probably takes up phosphoryl groups through RcsC -> YojN -> RcsB phosphorelay pathway. To study the interaction among the proteins in this pathway, fluorescence spectroscopy, NMR spectroscopy, and an in vivo ß galactosidase assay were performed by using two domains of RcsC (T-RcsC and R-RcsC), HPt domain of the protein YojN, and RcsB. The interactions between R-RcsC/YojN-HPt and YojN-HPt/RcsB supports the proposed pathway of phosphorylating RcsB. RcsB might also be phosphorylated by YojN-HPt that is phosphorylated by other sensor kinase other than RcsC in a cross-talk mechanism. The phosphorylation of RcsB by YojN-HPt probably has the same negative effect on cps induction as obtained with BeF3 - effect on DNA binding by RcsAB heterodimer.
The biomarker record in two different lakes in central Europe, Lake Albano and Lake Constance, is used to reflect environmental changes and lake system response during the Late Glacial and Holocene. Extractable organic compounds in lake sediments, which can be assigned to their biological source (biomarkers) function as fingerprints of past aquatic or land plant organisms. Using gas chromatography coupled with mass spectrometry, 21 different biomarkers (predominantly steroids and triterpenoids) as well as a variety of n-alkanes, nalkanols, and n-alkanoic acids could be identified in the sediment records of Lake Albano and Lake Constance. In the Holocene sediments of Lake Albano, the distribution of biomarkers such as dinosterol (dinoflagellates), isoarborinol, and diplopterol (aquatic organisms) indicate three biomarker zones: The period between 0-3,800 years BP (zone 3) is characterized by high concentrations of these biomarkers and others such as tetrahymanol and diploptene. Conversely, zone 2 (3,800-6,500 years BP) shows very low concentrations of all autochthonous biomarkers. In zone 1 (6,500–11,480 years BP), dinosterol, isoarborinol, and diplopterol range on a relatively high level, whereas diploptene and tetrahymanol display comparatively low concentrations. The results suggest at least two distinct changes in the predominance of primary producers during the Holocene, which are related to changes in the lake system such as lake mixing and water column stratification. This interpretation is consistent with previous investigations of Lake Albano sediments including pigment and hydrogen index data (Ariztegui et al., 1996b; Guilizzoni et al., 2002). Allochthonous biomarkers such as long-chain n-alkanes, amyrenones and friedelin indicate a development from forest to a more open landscape from 6,000 and 5.000 years BP, respectively. After a period of high concentrations during the first half of the Holocene, all biomarkers derived from deciduous trees exhibit relatively low values until around 1,000 years BP. Again, this is consistent with results from previous pollen investigations (Ariztegui et al., 2000). The sediment core from Upper Lake Constance comprises the Late Glacial and Holocene. It was analysed for biomarkers and inorganic tracers in order to compare the biomarker results with other proxy data from the same core. Magnetic susceptibility (MS) was measured to get a high-resolution stratigraphic framework of the core and to obtain further information about changes of the proportions of allochthonous and autochthonous input. Enhanced concentrations and accumulation rates of dinosterol (biomarker for dinoflagellates) and biogenic calcite give evidence of increasing lake productivity at the beginning of the Holocene followed by a decrease in bioproductivity after around 7,000 years BP. Younger Dryas sediments are characterized by low amounts of both dinosterol and biogenic calcite indicating a low productivity. The comparison of the concentrations and accumulation rates of b-sitosterol and stigmastanol with parameters reflecting lake productivity suggests that both steroids in Lake Constance sediments are mainly derived from terrigenous sources. Biomarkers as well as concentrations and accumulation rates of allochthonous inorganic compounds such as titanium, magnesium and strontium indicate a slightly enhanced allochthonous input after 8,500 years BP. Significant increase of erosive matter input from enhanced soil erosion is not observed before 4,000 years BP. This can be attributed to the combined effects of precipitation increase as a result of climatic deterioration and anthropogenic deforestation which is consistent with observations from other lakes in Central Europe. The MS record of Lake Constance confirms these results by tracing the climatically induced shifts of more intense bioproduction (low MS caused by increased calcite deposition) during the ‘climatic optimum’. This is followed by increasing input of terrigenous sediment compounds during colder and wetter periods which lead to higher MS values in the lake sediments. The occurrence of tetrahymanol in Lake Constance sediments questions the unambiguous use of tetrahymanol as an indicator for water column stratification. Anaerobic organic macroaggregates within the oxygenated, photic zone of the water column have to be considered as a possible living space for anaerobic microorganisms containing tetrahymanol. The direct comparison of two very different lakes Albano and Constance with respect to biomarkers indicating climate or environmental change provides a contribution to the recent biomarker research for a better understanding of biomarkers in lacustrine sediments.
P2X receptors are ligand (ATP)-gated ion channels that open an intrinsic cation permeable pathway in response to extracellular ATP released from both neuronal and non-neuronal cells. P2X receptors are abundantly distributed and mediate a wide variety of physiological functions, ranging from fast synaptic transmission in the central, peripheral, and enteric nervous system, to proinflammatory cytokine release from immune cells. The primary aim of this work was to elucidate the pathway that leads to the finally assembled trimeric P2X receptors, including the assessment of a possible role of ER chaperones and folding factors in this process. Additionally, the study was conducted to investigate the various ER quality control processes involved in the selection of “properly folded and assembled” P2X receptors that are suitable for the surface expression.
The heat stress (hs) response is universal to all organisms. As the cell senses increase in temperature, heat stress transcription factors (Hsfs) are activated to upregulate the expression of a number of genes encoding heat stress proteins (Hsp) which act as molecular chaperones to protect cells against heat damages. In higher plants, the phenomenon seems to be unusually complex both at the level of Hsfs and Hsps (e.g., 21 Hsf encoding genes in Arabidopsis and at least 17 in tomato). Upon prolonged hs, another characteristic property of plant cells is the assembly of large cytosolic aggregates called heat stress granules (HSG), which are composed of Hsps, HsfA2, RNA and RNA-binding proteins. The present work was aimed to understand plant hs response using tomato as a model system. To study the function of tomato Hsfs in their native system, we generated transgenic tomato lines altered in expression of HsfA1, HsfA2, and HsfB1. Tomato plants with 10-fold overexpression of HsfA1 (OE plants) were characterised by integration of a single HsfA1 expression cassette, whereas the plants harbouring a tandem inverted repeat (IR) of the cassette showed cosuppression of HsfA1 (CS plants). The lack of HsfA1 expression in CS plants results from posttranscriptional gene silencing connected with the formation of small interfering RNA (siRNA). Under normal growth conditions, major developmental features were similar for wild-type (WT), OE and CS plants. However, in contrast to the former two, CS plants and fruits were extremely sensitive to elevated temperature because hs-induced synthesis of major chaperones and Hsfs was strongly reduced or lacking. Despite the complexity of the plant Hsf family, the function of tomato HsfA1 is unique as master regulator of induced thermotolerance. On the other hand, maintenance of essential chaperones in CS plants during seed development suggests involvement of other Hsfs and/or transcription factor(s). HsfB1 and HsfA2 transgenic tomato plants, unaffected in thermotolerance, further supported the function of HsfA1 as the major factor regulating hs-inducible genes. Hs87 independent phenotypes of plants with altered expression of HsfB1 indicates developmental role of this Hsf. Using transient reporter assays with mesophyll protoplasts from WT tomato, we demonstrated that plasmids encoding Hsfs A1, A2 and A3 were well expressed which could function as activators for reporter gene expression. However, in protoplasts derived from CS plants, plasmids encoding HsfA2 and HsfA3 were normally expressed but even higher amounts of HsfA1 expression plasmids were completely silenced. Therefore, silencing of HsfA1 in CS plants was also reproduced in its mesophyll protoplasts. Lacking thermotolerance in CS protoplasts could be restored after transformation with expression plasmids encoding functionally equivalent HsfA2 or HsfA3 resulting in (i) expression of chaperones, (ii) survival of the cells at otherwise lethal temperature, (iii) thermoprotection of firefly luciferase, and (iv) assembly of heat stress granules (HSGs). The strong silencing caused by an IR in CS plants opened the possibility of a broad use of RNAi for gene knock-down also in the transient system of mesophyll protoplasts. Using this technology, we attempted to dissect essential components of thermotolerance and HSG assembly. We demonstrated the previously reported function of chaperones such as Hsp70 and Hsp101, and could discriminate the in vivo chaperone functions of different isoforms of Hsp20 and Hsp70 proteins. Hsp17-CI, Hsp70 (hs-inducible isoforms), and Hsp101 are absolutely essential chaperones for thermotolerance in plants. Furthermore, the results also show that despite Hsp17-CI and -CII being major components of HSG complexes, they are dispensable for assembly of these complexes. Based on these results, it is proposed that in the transient protoplast system an approach with gene-specific IRs can be used to discriminate functions of closely related isoforms among protein-families and to dissect complex protein networks.
Vascular occlusive diseases are one of the leading mortality causes in westernised countries. Occlusions of one of the major arteries can be overcome without devastating consequences provided a timely induction of compensating collateral arteries occurs. Perhaps the most outstanding feature of collateral vessel growth is the proliferation of smooth muscle cells (SMCs). Understanding the molecular mechanisms and identifying key molecular players of SMC proliferation would contribute significantly to the development of efficient therapies to intervene with all processes involving neointima formation, including collateral growth. mRNA and protein coding for co-transcription factor Egr1 were found to be up-regulated in growing collateral vessels 6, 12 or 24 hours following femoral artery ligation in mice. Since Egr1 is required for SMC proliferation in vitro and in vivo and likely to be implicated in the initiation of collateral artery growth, the key signalling mediators regulating Egr1 expression specifically in proliferating vascular SMCs were investigated. Northern blot and Western blot analysis revealed a strong up-regulation of Egr1 within 2 hours of stimulation with PDGF-AB and FGF-2. These two potent SMC mitogens involved in neointima formation were used to stimulate vascular SMCs not only to delineate the regulators of Egr1 expression but also to identify additional key mediators of SMC proliferation. FGF-2 but not PDGF-AB led to a drastic reduction of desmin amount in proliferating SMCs, correlating closely with the phenotypic modulation of SMCs in vivo. Both growth factors triggered a dramatic increase in DNA-synthesis rate with a concomitant loss of p27 exp Kip1. Stimulation with PDGF-AB and FGF-2 triggered a rapid and transient activation of PDGFRβ and FGFR1 respectively, thus providing the basis for activation of down-stream targets. Analysis of an array of signalling pathways demonstrated a strong activation of the Ras-Raf-MEK-ERK cascade in response to both factors as measured by the level of phosphorylation of prominent members MEK, ERK1/2 and c-Myc. SAPK/JNK and p38, which also belong to the superfamily of MAP kinases, did not become activated following stimulation with either PDGF-AB or FGF-2. The analysis of various PKC isoforms identified PKCδ and PKCθ to be the key mediators of PDGF-AB- and FGF-2-induced mitogenesis in proliferating SMCs. Whereas PDGF-AB potently stimulated PKB/Akt with concomitant GSK3β phosphorylation, FGF-2-induced inactivation of GSK3β was independent of PKB/Akt. Specific inhibition in order to evaluate the contribution of individual pathways to Egr1 expression and vascular SMC proliferation revealed that inhibition of the Raf-MEK-ERK module by UO126 completely abolished DNA-synthesis and Egr1 expression without a compensation by alternative pathways. Surprisingly, inhibition of PI3K led to a switch to the mitogenic RafMEK-ERK signalling cascade which resulted in an augmented Egr1 expression. In conclusion, in porcine vascular SMCs, activation of the Ras-Raf-MEK-ERK signalling module appears to be the main prerequisite for Egr1 expression and DNA synthesis induction in response to PDGF-AB and FGF-2 whereas related kinases SAPK/JNK and p38 play no significant role. Inhibition of the PI3K-Akt cascade represents an alternative way to activate ERK1/2 and induce Egr1 expression. Whereas MEK is the central regulator of mitogenic effects in proliferating vascular SMCs, the PI3K-Akt pathway most likely exerts survival function. Inactivation of MEK by its specific inhibitors identified hyperphosphorylation as ayet unknown mechanism of kinase inhibition.
Summary and Outlook The aim of this work was the investigation of the Mn2+ binding sites in hammerhead and the Diels-Alder ribozymes. This project consists of three main topics. In the first part quantification and structural characterization of Mn2+ binding sites in the m- and the tsHHRz using Electron Paramagnetic Resonance (EPR) spectroscopy are described. The second part summarizes the newest results obtained for the cleavage activity of both mand tsHHRzs in the presence of different Mg2+ and Mn2+ and Na+ ion concentrations using the new method with fluorescent-labeled RNAs. Here the influence of neomycin B on the structure of Mn2+ binding pockets and on the catalytic activity of both HHRzs is discussed. In addition, a possible role of Mn2+ ions is suggested from correlation of the EPR data with the kinetic results. The last chapter is devoted to quantification and differentiation of Mn2+ binding sites of the Diels-Alder ribozyme using continuous wave (cw) EPR experiments in solution. In this work EPR spectroscopy was used to study the binding of Mn2+ ions to the cis tsHHRz and to compare it with the binding to the trans mHHRz and to the Diels-Alder ribozyme. Cw EPR measurements showed that the tsHHRz possesses a single highaffinity Mn2+ binding site with a KD of < 10 nM at a NaCl concentration of 0.1 M. This dissociation constant is three orders of magnitude smaller than the KD determined for the single high-affinity Mn2+ site in the mHHRz (KD = 4.4 μM). The measurements of catalytic activity have been performed using fluorescent-labeled RNAs. Compared to the mHHRz, the cis tsHHRz cleaves up to 20-fold faster in the presence of Mg2+/Mn2+ ions with no saturation of the cleavage rates at high metal(II) ion concentrations. This is in good agreement with the last investigations on the trans tsHHRz (Nelson et al. 2005). Thus, the much stronger Mn2+ binding and higher cleavage activity were attributed to the interaction between the two external loops of the tsHHRz which reduces the RNA dynamics and traps the Mn2+ in the tightly folded conformation. Intriguingly, according to the EPR studies the binding constants for Mn2+ ions are several orders higher than the concentration of Mn2+ ions required for the catalytic activity (mHHRz: KD = 4.4 ± 0.5 μM and the Mn2+ concentration required to achieve half of the maximum cleavage rate [Mn2+]1/2 = 4.1 ± 0.6 mM respectively). Therefore, strongly bound Mn2+ ions seem to be needed for the folding of the HHRz, whereas weakly bound metal(II) ions are required to achieve full catalytic activity, and may be directly involved in catalysis. A comparison between the Electron Spin Echo Envelope Modulation (ESEEM) and Hyperfine Sublevel Correlation (HYSCORE) spectra of m- and tsHHRz demonstrates that both binding sites in HHRzs are structurally very similar. This suggests that the Mn2+ is located in both ribozymes between the bases A9 and G10.1 of the sheared G•A tandem basepair, as shown previously and in detail for the mHHRz (Vogt and DeRose 1998, Schiemann et al. 2003). However, the hyperfine spectra of the tsHHRz with 15N labeled G10.1 revealed no difference in comparison with the ones with 14N. This leads to an interpretation that the Mn2+ binding sites in both ribozymes are not identical. In addition, aminoglycoside antibiotic neomycin B inhibits the cleavage activity of both despite of the fact that it displaces the high-affinity Mn2+ ion only from the mHHRz. Hence, binding of neomycin B to the m- and the tsHHRzs probably occurs at different sites and neomycin B displaces only loosely bound Me2+ ions from the tsHHRs, whereas in the mHHRz both the high-affinity ion and the weakly bound ions are replaced. Therefore, it cannot be excluded that weakly bound Mg2+/Mn2+ ions, together with looploop interactions, induce a structural rearrangement which brings the high-affinity ion closer to the cleavage site. In the case of the Diels-Alder ribozyme it possesses five Mn2+ binding sites with KD = 0.6 ± 0.2 μM in solution under conditions where it is catalytically active. The competition experiment with Cd2+ allows to distinguish three different types of Mn2+ binding sites in the Diels-Alder ribozyme including inner-sphere monomeric Mn2+, monomeric Mn2+ bound through water-mediated contacts and electronically coupled dimeric Mn2+. Three Mn2+ ions are more strongly bound to the ribozyme via inner-sphere contacts, whereas two other Mn2+ ions form water-mediated outer-sphere contacts with the nucleotides of the ribozyme. The inner-sphere Mn2+ with the highest affinity and the fourth Mn2+ ions added to the ribozyme form a dimer with a Mn2+-Mn2+ distance of ~6 Å (as arises from simulations). Moreover, an addition of the product analog inhibitor (AMDA) to the [Diels-Alder ribozymes/ Mn2+] complex shows no conformational changes in the Mn2+ binding pockets. This is in good agreement with the recent studies which suggest that the Diels-Alder ribozyme is preorganized (Keiper et al. 2004). Some considerations on the evolution of the project (Outlook) There may be several venues of continuation of this project, which exploit on unique combination of EPR experiments and biochemical studies on RNA. This combination may allow us to significantly contribute to understanding of metal role in HHRz catalysis. Since the tsHHRz possesses the high affinity Mn2+ binding site (Kd < 10 nM) it creates a possibility to find conditions where the structural site is occupied by Mn2+, while catalytic sites are occupied by Mg2+ ions. If these conditions will be established by EPR titration, a set of standard biochemical experiments may be designed to look at the kinetic of cleavage and differentiate the “structural” and catalytic effects. The other experiment would be to look at the Mn2+ binding site in the tsHHRz in comparison with P1 and P1/P2 complexes and compare the results with the ones for the mHHRz. No matter the answer, P1 can be used as a simpler model to study the effect of tertiary structure on Mn2+ binding. A set of the tsHHRz mutants can be created to observe the mutations affect on Mn2+ binding sites, Mn2+ affinity and correlate the data with the kinetic analysis. FRET-based kinetic assay with fluorophore pairs on P1 and P2 can be designed for the kinetic experiments. Having this system one will be able to perform kinetic measurements 100-fold faster comparing to standard gel procedures (everything will be done in 96-wells). By manipulating the lengths and the sequence of P2 we most likely will be able to use FRET assay for the chemical step analysis (provided Kd > k2), and measure it using stop-flow system with time resolution of microseconds. And finally, one will be able to quantitatively measure the effect of neomycin B on the tsHHRz. Another interesting possibility would be to look at the state of metal(II) in the tsHHRz – enzyme alone (dissociated product) and in the enzyme-product complex and compare with the full-length tsHHRz. It will provide the information about the local rearrangements upon catalysis and the role of metal(II) ions. Furthermore, additional pulse-EPR experiments using 15N labeling have to be performed in order to reveal the location of the high-affinity Mn2+ binding site in the tsHHRz. Additionally, paramagnetic Mn2+ ions can be localized within the global fold of HHRzs using PELDOR and site-directed spin labeling. Further characterization of the high-affinity binding site in the tsHHRz can be performed using high-field ENDOR measurements in order to obtain the 14N and 31P tensors.
Unlimited self-renewal is an absolute prerequisite for any malignancy, and is the ultimate arbiter of the continuous growth and metastasis of tumors. It has been suggested that the self-renewal properties of a tumor are exclusively contained within a small population, i.e., the so-called cancer stem cells. Enhanced self-renewal potential plays a pivotal role in the development of leukemia. My data have shown that APL associated translocation products PML/RARalpha and PLZF/RARalpha increased the replating efficiency of mouse lin-/Sca1+ hematopoietic stem cells (HSCs). This effect is partly mediated by induction of gamma–catenin which is an important mediator of the Wnt signaling pathway and has been shown to be up regulated by the AML associated translocation products(AATPs). Suppression of gamma–catenin by siRNA can abrogate the increased replating efficiency induced by AATPs. Transduction of gamma–catenin in lin-/Sca1+ HSCs led to increased replating efficiency and the expression of stem cell markers Sca1 and c-kit. Additionally it induced accelerated cell cycle progression of mouse bone marrow HSCs. Transduction/transplantation mouse models have shown that ectopic expression of gamma–catenin in HSCs led to acute myeloid leukemia without maturation. These data suggest important roles of Wnt signaling pathway in the leukemogenesis induced by PML/RARalpha, PLZF/RARalpha and AML1/ETO. In contrast to AATPs, CML and Ph+-ALL associated translocation products p185(BCR-ABL) and p210(BCR-ABL) did not affect the self-renewal potential of hematopoietic stem/progenitor cells. However my studies indicated that their reciprocal translocation products p40(ABL/BCR) and p96(ABL/BCR) actually increased the replating efficiency of hematopoietic stem/progenitor cells. The effect is stronger when induced by p96(ABL/BCR) than by p40(ABL/BCR). It is very intriguing that p96(ABL/BCR) can activate Wnt signaling and up regulate the expression of HoxB4. Transduction/transplantation mouse model has shown that p40(ABL/BCR) and p96(ABL/BCR) both have their own leukemogenic potential. Given the fact that leukemic stem cells maintain the growth of tumor and are the origin of relapse, the cure of leukemia is dependent on the eradication of the leukemic stem cell and abrogation of aberrantly regulated self-renewal capability. Both t-RA and As2O3 have been shown to induce complete remission in APL patients with PML/RARalpha translocation product. However, t-RA as a single agent achieves completeremission (CR) but not complete molecular remissions (CMR). Therefore, virtually all patients will experience a relapse within a few months. In contrast to t-RA, As2O3 as a single agent is able to induce CR as well as CMR followed by long-term relapse-free survival in about 50% of APL patients even if relapsed after treatment with t-RA-containing chemotherapy regimens. Nothing is known about the mechanisms leading to the complete different clinical outcomes by the two compounds although both have been shown to induce differentiation of blast cells, proliferation arrest, induction of apoptosis and degradation of PML/RARalpha. We investigated the effect of t-RA and arsenic on PML/RARalpha-expressing cell population with stem cell capacity derived from the APL cell line NB4 as well as Sca1+/lin- murine bone marrow cells. We found that t-RA did not reduce the replating efficiency in PML/RARalpha- and PLZF/RARalpha-infected Sca1+/lincells whereas it selected small compact colonies representing very early progenitor cells. T-RA was unable to reduce the capacity to form colony forming units-spleen (CFU-S) of Sca1+/lin-cells expressing PML/RARalpha, additionally t-RA did not impair the capability of engraftment of NB4 cells in NOD/SCID mouse. On the contrary to t-RA, As2O3 abolished the aberrant self-renewal potential of Sca1+/lin- cells expressing PML/RARalpha. As2O3 not only abolished the replating efficiency of PML/RARalpha positive cells but also completely abrogated the ability of PML/RARalpha-positive HSC to produce CFU-S in vivo. On the contrary to As2O3, t-RA increased the absolute cell number and the percentage of cells in the side population with respect to the whole cell population in NB4 cells. Taken together these data suggest that arsenic but not all-trans retinoic acid overcomes the aberrant stem cell capacity of PML/RARalpha positive leukemic stem cells. My data prove for the first time that there is a direct relationship between the capacity of compounds to effectively target the LSC and their capacity to eradicate the leukemia, and, thereby, to induce complete molecular remission and long-term relapse-free survival. Thus, in order to increase the curative potential of leukemia therapies, future studies need to include the effect of given compounds on the stem cell compartment to determine their ability to eradicate the LSC.
The experience of pain is mediated by a specialized sensory system, the nociceptive system. There is considerable evidence that the cGMP/cGMP kinase I (cGKI) signaling pathway modulates the nociceptive processing within the spinal cord. However, downstream targets of cGKI in this context have not been identified to date. In this study we investigated whether cysteine-rich protein 2 (CRP2) is a downstream effector of cGKI in the spinal cord and is involved in nociceptive processing. Immunohistochemistry of the mouse spinal cord revealed that CRP2 is expressed in superficial laminae of the dorsal horn. CRP2 is colocalized with cGKI and with markers of primary afferent C fibers. Importantly, the majority of CRP2 mRNA-positive dorsal root ganglion (DRG) neurons express cGKI and CRP2 is phosphorylated in a cGMP-dependent manner. To elucidate the functional role of CRP2 in nociception, we investigated the nociceptive behavior of CRP2-deficient (CRP2-/-) mice. Touch perception and acute thermal nociception were unaltered in CRP2-/- mice. However, CRP2-/- mice showed an increased nociceptive behavior in models of persistent pain as compared to wild type mice. Intrathecal administration of cGKI activating cGMP analogs increased the nociceptive behavior in wild type but not in CRP2-/- mice, indicating that the presence of CRP2 was essential for cGMP/cGKI-mediated nociception. These data indicate that CRP2 is a new downstream effector of cGKI-mediated spinal nociceptive processing and point to an inhibitory role of CRP2 in the generation of inflammatory pain.
cGMP- and cAMP-dependent protein kinases (cGK and cAK) mediate the inhibitory effects of endothelium-derived messenger molecules nitric oxide and prostacyclin on platelets. To understand the mechanisms involved in platelet inhibition we searched for new substrates of cGK and cAK. We identified Rap1GAP2, the only GTPase-activating protein of Rap1 in platelets. Rap1 is a guanine-nucleotide binding protein that controls integrin activity, platelet adhesion and aggregation. Rap1GAP2 is required to turn over Rap1-GTP to Rap1-GDP resulting in the inactivation of integrins and reduced cellular adhesion. Using phospho-specific antibodies we demonstrate phosphorylation of endogenous Rap1GAP2 on serine 7 by cGK and cAK in intact platelets. Yeast-two-hybrid screening revealed an interaction of the phosphoserine/-threonine binding adapter protein 14-3-3 with Rap1GAP2, and we mapped the 14-3-3 binding site to the N-terminus of Rap1GAP2 close to the cGK/cAK phosphorylation site. We could show that 14-3-3 binding to Rap1GAP2 requires phosphorylation of serine 9. Platelet activation by ADP and thrombin treatment induces Rap1GAP2 serine 9 phosphorylation and enhances the attachment of 14-3-3 to Rap1GAP2. In contrast, phosphorylation of serine 7 by cGK/cAK leads to the detachment of 14-3-3. Furthermore, Rap1GAP2 serine 7 phosphorylation correlates with the inhibition of Rap1-GTP formation by cGMP and cAMP in platelets. Cell adhesion experiments provide additional evidence that Rap1GAP2 is activated by the detachment of 14-3-3. Point mutants of Rap1GAP2 deficient in 14-3-3 binding inhibit Rap1-mediated cell adhesion significantly stronger than a Rap1GAP2 mutant that binds 14-3-3 constitutively. Our findings define a novel regulatory mechanism that might contribute to both platelet activation and endothelial inhibition of platelet adhesion and aggregation.
Oxidative stress attenuates the NO-cGMP pathway, e.g. in the vascular system, through scavenging of free NO radicals by superoxide O2•-, by inactivation of soluble guanylyl cyclase (sGC) via oxidation of its central Fe2+ ion, and by down-regulation of sGC protein levels. While the former pathways are well established, the molecular mechanisms underlying the latter are still obscure. Using oxidative sGC inhibitor ODQ we demonstrate rapid down-regulation of sGC protein in mammalian cells. Co-incubation with proteasomal inhibitor MG132 results in accumulation of ubiquitinated sGC whereas sGC activator BAY 58–2667 prevents ubiquitination. ODQ-induced down-regulation of sGC is mediated through selective ubiquitination of its b subunit, and BAY 58–2667 abrogates this effect. Ubiquitination of sGC-b is dramatically enhanced by E3 ligase CHIP. Our data indicate that oxidative stress promotes ubiquitination of sGC b subunit through E3 ligase CHIP, and that sGC activator 58–2667 reverts this effect, most likely through stabilization of the heme-free b subunit. Thus the deleterious effects of oxidative stress can be counter-balanced by an activator of a key enzyme of vascular homeostasis.
Much has been written on the success of the Indian software industry, enumerating systemic factors like first-class higher education and research institutions, both public and private; low labour costs, stimulating (state) policies etc. However, although most studies analyzing the 'Indian' software industry cover essentially the South (and West) Indian clusters, this issue has not been tackled explicitly. This paper supplements the economic geography explanations mentioned above with the additional factor social capital, which is not only important within the region, but also in transnational (ethnic) networks linking Indian software clusters with the Silicon Valley. In other words, spatial proximity is complemented with cultural proximity, thereby, extending the system of innovation. The main hypothesis is that some Indian regions are more apt to economic development and innovation due to their higher affinity to education and learning, as well as, their more general openness, which has been a main finding of my interviews. In addition, the transnational networks of Silicon Valley Indians seem to be dominated by South Indians, thus, corroborating the regional clustering of the Indian software industry. JEL Classifications: O30, R12, Z13, L86
Bypassing of DNA lesions by damage-tolerant DNA polymerases depends on the interaction of these enzymes with the monoubiquitylated form of the replicative clamp protein, PCNA. We have analyzed the contributions of ubiquitin and PCNA binding to damage bypass and damage-induced mutagenesis in Polymerase {eta} (encoded by RAD30) from the budding yeast Saccharomyces cerevisiae. We report here that a ubiquitin-binding domain provides enhanced affinity for the ubiquitylated form of PCNA and is essential for in vivo function of the polymerase, but only in conjunction with a basal affinity for the unmodified clamp, mediated by a conserved PCNA interaction motif. We show that enhancement of the interaction and function in damage tolerance does not depend on the ubiquitin attachment site within PCNA. Like its mammalian homolog, budding yeast Polymerase {eta} itself is ubiquitylated in a manner dependent on its ubiquitin-binding domain.
To facilitate the measurement of intramolecular distances in solvated RNA systems, a combination of spin-labeling, electron paramagnetic resonance (EPR), and molecular dynamics (MD) simulation is presented. The fairly rigid spin label 2,2,5,5-tetramethyl-pyrrolin-1-yloxyl-3-acetylene (TPA) was base and site specifically introduced into RNA through a Sonogashira palladium catalyzed crosscoupling on column. For this purpose 5-iodouridine, 5-iodo-cytidine and 2-iodo-adenosine phosphoramidites were synthesized and incorporated into RNA-sequences. Application of the recently developed ACE (R) chemistry presented the main advantage to limit the reduction of the nitroxide to an amine during the oligonucleotide automated synthesis and thus to increase substantially the reliability of the synthesis and the yield of labeled oligonucleotides. 4-Pulse Electron Double Resonance (PELDOR) was then successfully used to measure the intramolecular spin–spin distances in six doubly labeled RNA-duplexes. Comparison of these results with our previous work on DNA showed that A- and B-Form can be differentiated. Using an all-atom force field with explicit solvent, MD simulations gave results in good agreement with the measured distances and indicated that the RNA A-Form was conserved despite a local destabilization effect of the nitroxide label. The applicability of the method to more complex biological systems is discussed.
Riboswitches are highly structured elements in the 50-untranslated regions (50-UTRs) of messenger RNA that control gene expression by specifically binding to small metabolite molecules. They consist of an aptamer domain responsible for ligand binding and an expression platform. Ligand binding in the aptamer domain leads to conformational changes in the expression platform that result in transcription termination or abolish ribosome binding. The guanine riboswitch binds with high-specificity to guanine and hypoxanthine and is among the smallest riboswitches described so far. The X-ray-structure of its aptamer domain in complex with guanine/ hypoxanthine reveals an intricate RNA-fold consisting of a three-helix junction stabilized by longrange base pairing interactions. We analyzed the conformational transitions of the aptamer domain induced by binding of hypoxanthine using highresolution NMR-spectroscopy in solution. We found that the long-range base pairing interactions are already present in the free RNA and preorganize its global fold. The ligand binding core region is lacking hydrogen bonding interactions and therefore likely to be unstructured in the absence of ligand. Mg2+-ions are not essential for ligand binding and do not change the structure of the RNA-ligand complex but stabilize the structure at elevated temperatures. We identified a mutant RNA where the long-range base pairing interactions are disrupted in the free form of the RNA but form upon ligand binding in an Mg2+-dependent fashion. The tertiary interaction motif is stable outside the riboswitch context.
Background Cryptic species are two or more distinct but morphologically similar species that were classified as a single species. During the past two decades we observed an exponential growth of publications on cryptic species. Recently published reviews have demonstrated cryptic species have profound consequences on many biological disciplines. It has been proposed that their distribution is non-random across taxa and biomes. Results We analysed a literature database for the taxonomic and biogeographical distribution of cryptic animal species reports. Results from regression analysis indicate that cryptic species are almost evenly distributed among major metazoan taxa and biogeographical regions when corrected for species richness and study intensity. Conclusion This indicates that morphological stasis represents an evolutionary constant and that cryptic metazoan diversity does predictably affect estimates of earth´s animal diversity. Our findings have direct theoretical and practical consequences for a number of prevailing biological questions with regard to global biodiversity estimates, conservation efforts and global taxonomic initiatives.
Membranes are essential for life, because a cell must separate itself from the environment to keep its molecules from dissipating away and also must keep out foreign molecules that disturb them or their cell components. However, the cell must communicate with the environment and adapt to the external conditions, needs to pump in nutrients and release toxic products of its metabolism. Membrane proteins present in the membranes of the cell and cell organelles, help the cell to gather information about the environment and perform various biological processes. Membrane proteins perform a wide range of biological functions including respiration, signal transduction and transport. Despite their high importance in biological function, only few structures have been determined because of the difficulties in producing high amounts of membrane proteins and obtaining good quality crystals. This Ph. D. thesis involves the study of different kinds of cytochrome oxidases and a membrane anchored cytochrome oxidase electron donor. Though structures of many cytochrome oxidases are known to date, there exist many different types of oxidases in different organisms, which help the organism to survive under unfavorable environmental conditions. The structural differences between these terminal oxidases which make the organism to survive in extreme environments are unclear. To investigate these, structures of different types of oxidases are necessary. Therefore, we are interested in revealing the structural details of different types of oxidases. The different types of oxidase I worked with were the caa3 HiPIP:oxygen oxidoreductase from Rhodothermus marinus, the aa3-type quinol oxidase from Acidianus ambivalens and bd-type quinol oxidase from three different organisms (Escherichia coli, Bacillus thermodenitrificans and Aquifex aeolicus). Besides the protein from E. coli all other proteins are from thermophilic organisms from which the proteins obtained are generally believed to be highly stable. The presence of a high content of charged amino acids that enhances the occurrence of salt bridges contributes to the stability of thermophilic proteins. ....
In this thesis the three dimensional solution strucutre of the RbfA protein from Thermotoga maritima was solved using multidimensional heteronuclear NMR spectroscopy. The RbfA protein binds to the helix I region of the 16S rRNA. To gain insights into the binding mode of RbfA to its target, a second RbfA construct from Helicobacter pylori was used. Comparison of the RbfA proteins with the published structure of RbfA from Escherichia coli, led to studies concerning the differences between proteins from thermophile and mesophile systems. In the second part of this thesis the native binding motive of the RbfA protein was identified. The RbfA protein binds to an alternate helix fold within the pre-sequence of the immature 16S rRNA.
Membrane proteins play vital role in a variety of cellular processes, such as signal transduction, transport and recognition. In turn they are involved in numerous human diseases and currently represent one of the most prevalent drug targets. A comprehensive understanding of the mechanisms mediated by membrane proteins requires information about their structures at near-atomic resolution, although structural studies of membrane proteins remain behind those of soluble proteins. A bottleneck in the study of membrane proteins resides in the difficulties that are encountered during their high-level production in cell based systems. However, many toxic effects attributed to the over production of membrane proteins are eliminated by cell-free expression, as viable host cells are no longer required. Therefore, the objective of this study was to obtain adequate amounts of selected membrane transport proteins for their structural studies using a cell-free expression system. For the establishment of the cell-free system for membrane proteins, the transporters YbgR and YiiP from Salmonella typhimurium LT2, PF0558 and PF1373 from Pyrococcus furiosus, from the cation diffusion family (CDF), BetP from Corynebacterium glutamicum from the betaine/carnitine/choline transporter (BCCT) family and Aq-2030 from Aquifex aeolicus VF5 from the monovalent cation/proton antiporter-2 (CPA2) family were selected. An Escherichia coli S-30 extract based cellfree system was established by generating the best expression constructs of the target proteins, preparing T7 RNA polymerase and an S-30 extract with high translation efficiency. The functionality of the S-30 extract was shown by the cell-free expression of correctly folded Green Fluorescent Protein (GFP). Essential factors of the cell-free system such as the Mg2+ concentration, the bacterial S-30 extract proportion in the reaction mixture and the time-course of cell-free reactions have been optimized. For the cell-free production of membrane proteins in soluble form, the possibility to supplement cell-free reactions with detergents was explored. A wide range of non-ionic or zwitterionic detergents, were found to be compatible with cell-free synthesis, while ionic detergents and non-ionic detergents at high concentrations had an inhibitory effect. Moreover, high concentrations of polyoxyethylene-alkyl-ethers (Brij) detergents were found to have enhancing effect on the production levels as well as on the solubility of cell-free produced proteins. As membrane proteins tend to misfold and aggregate in a membrane-free translation system, the possibility to supplement the cell-free reactions with inner membrane vesicles (IMVs) to obtain correctly folded target transport proteins was explored. All the target proteins were successfully produced in the batch cell-free reactions and were found to be incorporated in the IMVs. A continuous exchange cell-free (CECF) system was established, where consumable substrates (amino acids, nucleotides and energy regenerating compounds) were supplied to the cell-free reaction mixture through a dialysis membrane, which in consequence resulted in high-level production of target proteins compared to the batch system. The osmosensing and osmoregulated sodium-coupled symporter BetP from C. glutamicum was chosen for the large scale production in CECF set-up. The protein is easily produced in E. coli and is functional as assayed by its transport activity, after purification and reconstitution in liposomes. It is therefore possible to compare in-vivo and cell-free production. High-level cell-free production of BetP was achieved in CECF mode in different forms: (i) as precipitate, (ii) as soluble form in detergent, and (iii) incorporated in IMVs. Cell-free production of BetP resulted in the yield of about 0.5 mg of purified BetP from 1 ml of CECF reaction. The yield of purified BetP was increased to 1.6 fold by addition of 1% polyoxyethylene-(20)-cetyl-ether (Brij58) detergent in the reaction mixture. Moreover, the high level cell-free production of BetP (0.5 mg purified BetP/ml reaction mixture) incorporated in IMVs was shown for the first time in this work.However, it was observed that oligomerization of BetP was not efficient in the cell-free system. Factors that can promote the folding of membrane proteins such as lipids and chaperones were investigated. Addition of lipids and molecular chaperone GroE facilitated correct folding of BetP resulting in increased yield and stability of cell-free produced BetP. The results obtained indicate that most of the cell-free produced BetP exists in functional oligomeric form. The possibility of obtaining milligram amounts of BetP, a 12 trans-membrane protein from the cell-free reactions holds promise for structural and functional studies of other membrane proteins. In any case, the strategies adapted in this study should prove extremely valuable for the production of membrane proteins in the E. coli cell-free expression system.
First milestone of this Ph.D. thesis was the successful extension of conventional NTA/His-tag technique to self-assembling, multivalent chelator thiols for high-affinity recognition as well as stable and uniform immobilization of His-tagged proteins on chip surfaces. Bis-NTA was linked via an oligoethylene glycol to alkyl thiols by an efficient modular synthesis strategy yielding a novel, multivalent compound for formation of mixed SAMs with anti-adsorptive matrix thiols on gold. Multivalent chelator chips allow a specific, high-affinity, reversible, long-term immobilization of His-tagged proteins. In AFM studies reversibility of the specific protein immobilization process was visualized at single molecule level. The entire control over the orientation of the immobilized protein promotes this chip surface to an optimal platform for studies focusing on research targets at single molecule level and nanobiotechnology. Based on the constructed protein chip platform above and a novel AFM mode (contact oscillation mode, COM) – developed during the current Ph.D. work – protein nanolithography under physiological conditions enabling fabrication of active biomolecular patterns in countless variety has been established. Reversible COM-mediated nanostructuring is exceptionally suitable for multiplexed patterning of protein assemblies in situ. The first selfassembled protein layer acts as a biocompatible and ductile patterning material. Immobilized proteins can be replaced by the AFM tip applying COM, and the generated structures can be erased and refilled with different proteins, which are immobilized in a uniform and functional manner. Multi-protein arrays can be systematically fabricated by iterative erase-and-write processes, and employed for protein-protein interaction analysis. Fabrication of two-dimensionally arranged nanocatalytic centres with biological activity will establish a versatile tool for nanobiotechnology. As an alternative chip fabrication approach, the combined application of methodologies from surface chemistry, semiconductor technology, and chemical biology demonstrated successfully how pre-patterned templates for micro- and nanoarrays for protein chips are fabricated. The surface physical, as well the biophysical experiments, proved the functionality of this technology. The promises of such process technology are fast and economic fabrication of ready-to-use nanostructured biochips at industrial scale. Membrane proteins are complicated in handling and hence require sophisticated solutions for chip technological application. A silicon-on-insulator (SOI) chip substrate with microcavities and nanopores was employed for first technological investigation to construct a protein chip suitable for membrane proteins. The formation of an artificial lipid bilayer using vesicle fusion on oxidized SOI cavity substrates was verified by CLSM. Future AFM experiments will give further insights into the chip architecture and topography. This will provide last evidence of the sealing of the cavity by the lipid bilayer. Transmembrane proteins will be employed for reconstitution experiments on this membrane protein chip platform. Highly integrated microdevices will find application in basic biomedical and pharmaceutical research, whereas robust and portable point-of-care devices will be used in clinical settings.
Background Synchronous neuronal firing has been discussed as a potential neuronal code. For testing first, if synchronous firing exists, second if it is modulated by the behaviour, and third if it is not by chance, a large set of tools has been developed. However, to test whether synchronous neuronal firing is really involved in information processing one needs a direct comparison of the amount of synchronous firing for different factors like experimental or behavioural conditions. To this end we present an extended version of a previously published method NeuroXidence [1], which tests, based on a bi- and multivariate test design, whether the amount of synchronous firing above the chance level is different for different factors.
Background The synchrony hypothesis postulates that precise temporal synchronization of different pools of neurons conveys information that is not contained in their firing rates. The synchrony hypothesis had been supported by experimental findings demonstrating that millisecond precise synchrony of neuronal oscillations across well separated brain regions plays an essential role in visual perception and other higher cognitive tasks [1]. Albeit, more evidence is being accumulated in favour of its role as a binding mechanism of distributed neural responses, the physical and anatomical substrate for such a dynamic and precise synchrony, especially zero-lag even in the presence of non-negligible delays, remains unclear. Here we propose a simple network motif that naturally accounts for zero-lag synchronization for a wide range of temporal delays [3]. We demonstrate that zero-lag synchronization between two distant neurons or neural populations can be achieved by relaying the dynamics via a third mediating single neuron or population. Methods We simulated the dynamics of two Hodgkin-Huxley neurons that interact with each other via an intermediate third neuron. The synaptic coupling was mediated through alpha-functions. Individual temporal delays of the arrival of pre-synaptic potentials were modelled by a gamma distribution. The strength of the synchronization and the phase-difference between each individual pairs were derived by cross-correlation of the membrane potentials. Results In the regular spiking regime the two outer neurons consistently synchronize with zero phase lag irrespective of the initial conditions. This robust zero-lag synchronization naturally arises as a consequence of the relay and redistribution of the dynamics performed by the central neuron. This result is independent on whether the coupling is excitatory or inhibitory and can be maintained for arbitrarily long time delays (see Fig. 1). Conclusion We have presented a simple and extremely robust network motif able to account for the isochronous synchronization of distant neural elements in a natural way. As opposed to other possible mechanisms of neural synchronization, neither inhibitory coupling, gap junctions nor precise tuning of morphological parameters are required to obtain zero-lag synchronized neuronal oscillation.
Die Verarbeitung von Informationen im zentralen Nervensystem beruht auf dem Zusammenspiel von erregender und hemmender Neurotransmission. Die Übertragung von Signalen zwischen Neuronen erfolgt chemisch über die Ausschüttung von Neurotransmittern an spezialisierten Kontaktstellen, den Synapsen. Glyzin und gamma-Aminobuttersäure (GABA) sind die bedeutendsten inhibitorischen Neurotransmitter im zentralen Nervensystem von Säugern, welche Rezeptoren vom Glyzin- (GlyR) und GABAA-Typ (GABAAR) aktivieren. Diese ligandengesteuerten Ionenkanäle sind in postsynaptischen Membranen angereichert und mit intrazellulären Proteinen assoziiert. Die Rekrutierung der Rezeptoren in postsynaptischen Domänen ist ein an das zytoplasmatisch lokalisierte Protein Gephyrin gekoppelter Prozess. So bindet Gephyrin spezifisch an die intrazelluläre Domäne der beta-Untereinheit des GlyR (GlyR beta) und bildet für die Verankerung des Rezeptors ein gerüstartiges Netzwerk unterhalb der synaptischen Membran. Die gezielte Inaktivierung des Gephyrin-Gens führt in Mäusen zu einem postnatal letalen Phänotyp und zu dem Verlust der synaptischen Anreicherung des GlyR und bestimmter GABAA-Rezeptoren auf zellulärer Ebene. Gephyrin ist ein 93 kDa großes Protein, das nicht nur im zentralen Nervensystem (ZNS), sondern auch in anderen Organen wie Leber und Niere exprimiert wird, in denen es an der Synthese des Molybdän-Kofaktors von Oxido-Reduktasen beteiligt ist. Das Gephyrin-Protein wird durch 30 Exons codiert, von denen zehn als sogenannte Kassetten alternativ gespleißt werden können. Die bestuntersuchte Spleißvariante besitzt 736 Aminosäuren und ist in eine N- und eine C-terminale Domäne (Aminosäuren 1-181 bzw. 318-736) sowie eine zentrale Linker-Domäne unterteilt. Die N- und die C-terminalen Bereiche von Gephyrin sind den Proteinen MogA und MoeA aus E. coli homolog und werden daher auch als G-Domäne (N-terminal) bzw. E-Domäne (C-terminal) bezeichnet. In kristallographischen Untersuchungen wurde gezeigt, dass die G- und E-Domänen zur Tri- bzw. Dimerisierung befähigt sind. Diese speziellen Oligomerisierungseigenschaften der beiden Gephyrindomänen bilden wahrscheinlich die Grundlage für die Entstehung von Gephyrin-Clustern sowie eines hexagonalen Gephyrin-Gerüstes. Dieses Gerüst stellt den Verknüpfungspunkt zwischen Rezeptoren und dem Zytoskelett dar und ermöglicht somit die effiziente Clusterbildung und die zielgerichtete Anordnung einer großen Anzahl inhibitorischer Rezeptoren. In der vorliegenden Arbeit sollten die Rolle dieser beiden Domänen bei der Bildung membranassoziierter Gephyrinaggregate und die molekularen Mechanismen der Clusterbildung des Gephyrinmoleküls untersucht werden. Zu diesem Zweck wurden durch zielgerichtete Mutagenese unterschiedliche Gephyrin-Mutanten hergestellt, um die Fähigkeit der Oligomerisierung der G- und E-Domäne gezielt zu modifizieren. Dadurch sollte die Bedeutung der Oligomerisierung hinsichtlich der Aggregat- bzw. Clusterbildung untersucht werden. Außerdem sollten die Wechselwirkungen zwischen Gephyrin und anderen Proteinen und deren Einfluss auf die synaptische Lokalisation analysiert werden. Für diese Untersuchungen wurden auf der Basis von Röntgenstruktur-Daten spezifische Aminosäurereste an den bei der Oligomerisierung beteiligten Kontaktstellen ausgetauscht. In der G-Domäne wurden zu diesem Zweck vier separate Aminosäuren des Trimer-Interface durch Arginin ersetzt (GephRRRR). Analog hierzu wurden in der EDomäne einzelne Aminosäuren durch Arginin bzw. Glutamat substituiert (GephRER), um dadurch eine Dimersierung zu verhindern. Für die Kassette C5’ wird angenommen, dass deren Vorhandensein die Interaktion zwischen Gephyrin und GlyR beeinträchtigt, wodurch GlyR aus GABAergenen Synapsen ausgeschlossen wird. Daher wurde der Einfluss dieser Gephyrin-Spleißvariante (GephC5’), die zu einer Peptidinsertion innerhalb der G-Domäne führt, und einer Gephyrin-Mutante (Gephmut), die den Verlust der Wechselwirkung mit dem GlyR bedingt, auf die Aggregatbildung von Gephyrinoligomeren untersucht. Bei dem Konstrukt Gephmut wurden, basierend auf Daten von Röntgenstrukturuntersuchungen, neun Aminosäuren (713-721) am Cterminalen Ende der E-Domäne durch den homologen Bereich des bakteriellen MoeA Proteins aus E. coli ersetzt. Zunächst wurden die einzelnen isolierten Domänen mittels Gelfiltration hinsichtlich ihres Oligomerisierungsverhaltens untersucht. Die Mutationen wurden hierzu in verkürzte Proteine eingeführt, bei denen nur die G- bzw. die E-Domäne exprimiert wurden. Diese Konstrukte wurden daher als GRRRR, GC5’ bzw. ERER und Emut bezeichnet. Bei diesen zeigte sich, dass die G-Domäne des Gephyrin-Wildtyps zu trimeren Proteinkomplexen oligomerisiert. Im Gegensatz hierzu war die Mutante GRRRR nicht in der Lage, Trimere zu bilden. Das Einfügen der C5’-Kassette führte ebenfalls zu einer Störung der Trimerisierung. Gelfiltrationsexperimente mit der E-Domäne ergaben, dass die mutierte Domäne ERER, im Gegensatz zum Wildtyp-Konstrukt, keine Dimere ausbildet. Bisherige Studien haben jedoch gezeigt, dass das Emut Polypeptid zur Dimerisierung befähigt ist. Das Oligomerisierungsverhalten des kompletten Gephyrin-Proteins wurde mittels blauer nativer Gelelektrophorese (BN-PAGE) analysiert. Für die hier beschriebenen Untersuchungen mit BN-PAGE wurde rekombinantes Gephyrin in Xenopus laevis Oozyten heterolog exprimiert. Die Analyse ergab, dass Wildtyp Gephyrin nativ als Hexamer vorliegt, welches durch ansteigende Konzentrationen des Detergenzes Natriumdodecylsulfat (SDS) in Trimere, Dimere und Monomere zerfällt. Sowohl GephRRRR und GephC5’ liegen nativ fast ausschließlich als Dimere vor, während GephRER nur trimere Aggregate formt. Die entsprechende Doppelmutante mit Mutationen in Gund E-Domäne war wie erwartet nur noch als Monomer existent. Die als Kontrolle eingesetzte Glyzinrezeptor-Bindungsmutante Gephmut bildete, ebenso wie der Wildtyp, Hexamere aus. Daraus folgt, dass die Oligomere der G- bzw E-Domäne Zwischenprodukte der Hexamerbildung darstellen. Die Analyse der Oligomerisierungseigenschaften der Mutanten wurde nachfolgend in humanen embryonalen Nierenzellen (HEK 293T) untersucht. Nach heterologer Expression von Wildtyp Gephyrin in HEK 293T-Zellen formen sich große, charakteristische Gephyrinaggregate. Die Oligomerisierungs-Mutanten GephRRRR, GephRER und GephC5’ aggregierten jedoch nicht, sondern waren diffus im Zytoplasma verteilt. Die wiederum als Kontrolle eingesetzte Bindungsmutante Gephmut hingegen wies eine normale Aggregation auf. Diese Ergebnisse bestätigen die grundlegende Rolle der Oligomerisierung von G- und E- Domänen für die Aggregatbildung von Gephyrin. Mittels GST-Pulldown und Kolokalisationsanalysen in HEK Zellen wurde die Wechselwirkung der Gephyrinmutanten mit der GlyR beta, dem Motorkomplexprotein Dynein light chain-1 (Dlc-1) und dem Guanin-Nukleotid-Austauschfaktor Collybistin (Cb) untersucht. Beide Ansätze weisen darauf hin, dass die Trimerisierung der G-Domäne an der Interaktion von Gephyrin mit Dlc-1 und die Dimerisierung der E-Domäne bei der Bindung an GlyR beta und Cb beteiligt ist. Die Mutante Gephmut zeigte in beiden Fällen einen totalen Verlust der Bindungsfähigkeit sowohl an das GlyR beta Bindungsmotiv als auch an Cb. Der Einbau der C5’ Kassette in Gephyrin scheint jedoch nicht dessen Bindung an den GlyR zu beeinflussen. Für die Analyse der Clusterbildung und des zielgerichteten Transports in Neuronen wurden Wildtyp und mutiertes Gephyrin in hippocampalen und spinalen Primärkulturen der Ratte exprimiert. Zur Überprüfung einer synaptischen Lokalisation wurde Gephyrin gemeinsam mit dem vesikulären inhibitorischen Aminosäure-Transporter (VIAAT), einem präsynaptischen Marker-Protein, detektiert. In beiden Kulturen wies Gephyrin eine punktartige Verteilung in den Neuriten auf und wurde gezielt an Synapsen angereichert. Im Kontrast dazu zeigten alle Oligomerisierungsmutanten, GephRRRR, GephC5’ und GephRER keine Ausbildung von Clustern sondern eine diffuse Verteilung im Zellkörper und in Dendriten. Das Konstrukt Gephmut wies jedoch Clusterbildung und eine punktförmige Verteilung auf. Diese Daten belegen, dass die Oligomerisierung der G- wie auch der E-Domänen für die Clusterbildung und synaptische Lokalisation von Gephyrin unerlässlich ist. Die Wechselwirkung mit dem GlyR und/oder Collybistin ist ebenfalls für die Anreicherung in der Synapse erforderlich, nicht jedoch für die Bildung der Gephyrin-Cluster. Die dargestellten Ergebnisse belegen die Rolle der spezifischen Oligomerisierungseigenschaften der G- und E-Domäne für die Ausbildung des hexagonalen Gephyringerüstes und dessen grundlegende Bedeutung für die spezifische Anreicherung von Gephyrin an inhibitorischen Synapsen in Neuronen.
The Indian IT industry has received great attention. Although most studies cover South Indian locations, clustering has rarely been a topic. This study focuses on Bangalore addressing questions related to Bangalore’s successful development and lessons thereof for other regions in and outside India. The approach pertains to economic geography and international business; hypotheses have been developed from a multi-disciplinary literature survey and interview fieldwork in Bangalore. I emphasize human and social capital and networks. While the first chapter delineates cultural foundations of human capital formation, the second and third deal with bonding and bridging social capital (or dense and loose networks), respectively; the fourth is an outlook on future opportunities through intersectoral upgrading. The main hypothesis is that a combination of both forms of social networks - contingent upon sub-sectors – has helped Bangalore developing a successful IT industry. Positive attitudes towards education led to relatively more human capital spawning two positive feedbacks: 1) establishment of national research and educational institutes resulting in large inflows of a diversity of people providing the required setting for creativity and innovation; 2) transnational networks linking to Silicon Valley are dominated by people from South India, allowing for additional knowledge spillovers corroborating the regional clustering.
The goal of this thesis was to gain further insight into the binding behavior of ligands in the heptahelical domain (HD) of group I metabotropic glutamate receptors (mGluRs). This was realized by the establishment of strategies for the detection and optimization of molecules acting as non-competitive antagonists of group I mGluRs (mGluR1/5). These strategies should guarantee high diversity in the retrieved chemotypes of the detected compounds not resembling original reference molecules (“scaffold-hopping”). The detection of new scaffolds, in turn, was divided into two approaches: First the development of pharmacological assays to screen compounds at a certain target for bioactivity (here: affinity towards the allosteric recognition site of mGluR1 and mGluR5), and second the evaluation of computer assisted methods for the identification of virtual hits to be screened afterwards on the pharmacological assays established before. Promising molecules should be optimized with respect to activity/affinity and selectivity, their binding mode investigated and, finally, compared to existing lead compounds. Initially, membrane based binding assays for the HD of mGlu1 and mGlu5 receptors with enhanced throughput (shifting from 24-well plates to 96-well plates) were set up. For the mGluR1 assay the potent antagonist EMQMCM exhibited high affinity towards the binding site (Ki ~3nM), which is in accordance with published data from Mabire et al. (functional IC50 3nM). For mGluR5 the reference antagonist MPEP binds with high affinity to the receptor (binding IC50 13.8nM), which confirmed earlier findings from Anderson et al. (binding IC50 15nM). In another series of experiments the properties of rat cerebellar (mGluR1) and corticalmembranes (mGluR5) as well as of radiotracers were investigated by means of binding saturation studies and kinetic experiments. Furthermore, the influence of the solvent DMSO, necessary for compound screening of lipophilic substances, on positive and negative controls was evaluated. As the precise architecture of the HD of mGluR1 is still not known our efforts in identifying new ligands for this receptor focused on the ligand-based approach. All computer assisted methods that were applied to virtually screen large compound collections and to retrieve potential hits (“activity-enriched subsets”) acting at the heptahelical domain of mGluR1 relied on the existence of a valid dataset of reference molecules. This was realized by an initial compilation of a mGluR reference data collection comprising in total 357 entries predominantly negative but also some positive allosteric modulators for mGluR1 and mGluR5. In the next step a pharmacophore model for non-competitive mGluR1 antagonists was constructed. It was based upon six selective, potent and structurally diverse ligands. Prospective virtual screening was performed using the CATS atom-pair descriptor. The Asinex Gold-Collection was screened for each seed compound and some of the most similar compounds (according to the CATS descriptor) were ordered and tested forbinding affinity and functional activity at mGluR1. A high hit rate of approximately 26% (IC50 < 15 micro M) was yielded confirming the applicability of this method. One compound exerted functional activity below one micro molar (IC50-value of C-07:362nM ± 0.03). Moreover, non-linear principal component analysis was employed. Again the Asinex vendor database served as test database and was filtered by the pharmacophore model for mGluR1 established before. Test molecules that were adjacently located with mGluR1 antagonist references were selected. 15 compounds were tested on mGluR1 in binding and functional assays and three of them exhibited functional activity (IC50) below 15 micro M. The most potent molecule P-06 revealed an IC50-value of 1.11 micro M (± 0.41). The COBRA database comprising 5,376 structurally diverse bioactive molecules affecting various targets was encoded with the CATS descriptor and used for training two selforganizing maps (SOM). The encoded mGluR reference data collection was projected onto this map according to the SOM algorithm. This projection allowed to clearly distinguish between antagonists of mGluR1 and mGluR5 subtype. 28 compounds were ordered and tested on activity and affinity for mGluR1. They exhibited functional activity down to the sub-micro molar range (IC50-value of S-08: 744nM ± 0.29) yielding a final hit rate of 46% (<15 micro M). Then, the Asinex collection was screened using the SOM approach. For a predicted target panel including the muscarinic mACh (M1) receptor, the histamine H1-receptor and the dopamine D2/D3 receptors, the tested mGluR ligands exhibited the calculated binding pattern. This virtual screening concept might provide a basis for early recognition of potential sideeffects in lead discovery. We superimposed a set of 39 quinoline derivatives as non-competitive mGluR1 antagonists that were recently published by Mabire and co-workers. A CoMFA model (QSAR) was established and the influence of several side chains on functional activity was investigated. The coumarine derivative C-07 was obtained as a result of similarity searching. Starting from this compound a series of chemical derivatives was synthesized. This led to the discovery of potent (B-28, IC50: 58nM ± 0.008; Ki: 293nM ± 0.022) and selective (rmGluR5 IC50: 28.6 micro M) mGluR1 antagonists. From a homology model of mGluR1 we derived a potential binding mode for coumarines within the allosteric transmembrane region. Potential interacting patterns with amino acids were proposed considering the difference of the binding pockets between rat and human receptors. The proposed binding modes for quinolines (here:EMQMCM) and coumarines (here:B-04) were compared and discussed considering in particular the influence on activity of several side chains of quinolines obtained from the QSAR studies. The present studies demonstrated the applicability of ligand-based virtual screening for non-competitive antagonists of a G-protein coupled receptor, resulting in novel, potent and selective agents.