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Wie herzig!
(2019)
Doch Vorsicht – dies ist kein Einblick in die Hirnwindungen eines verliebten Teenagers. Vielmehr handelt es sich hier um einen wissenschaftlichen Blick in die Großhirnrinde einer Maus. Die Forscherinnen und Forscher um Prof. Amparo Acker-Palmer vom Buchmann Institut für Molekulare Lebenswissenschaften und dem Institut für Zellbiologie und Neurowissenschaften der Goethe-Universität haben 2018 in der Zeitschrift "Science" darüber berichtet, dass Blutgefäße bei der Entwicklung neuronaler Zellnetzwerke im Gehirn eine bislang unbekannte Rolle spielen ...
The trade in bear parts for medicine and for status is a conservation challenge throughout Asia. The Asiatic black bear (Ursus thibetanus) and the sun bear (Helarctos malayanus) are endemic to this region, and populations are estimated to have declined throughout their ranges due to widespread illegal killing of bears and trade in parts, combined with loss of habitat. Previous studies have indicated that legislation alone is insufficient to prevent illegal hunting and trade, indicating instead a need to address demand for bear parts and products. We conducted mixed-method surveys in Cambodia to understand the key motivators for individuals to consume bear parts, and to understand whether specialised questioning techniques are applicable in this context. Bear part use is illegal in Cambodia and may therefore be considered a sensitive behaviour, in that individuals may be reluctant to admit to it. To counteract possible biases, four specialised questioning techniques were used in this study: randomised response technique (RRT), unmatched count technique (UCT), nominative technique (NT), and false consensus bias (FCB). All four methods serve to shield a respondent’s admittance of a sensitive behaviour from the interviewer. The results presented here show that great variability exists in anonymous methods’ efficacy in certain contexts. However, the results overall indicate that individuals in Cambodia are under-reporting their consumption of bear parts when directly asked, and that the prevalence of bear part use in Cambodia may be as high as 15% of the population, representing a significant conservation challenge.
In three-dimensional light microscopy, the heterogeneity of the optical density in a specimen ultimately limits the achievable penetration depth and hence the three-dimensional resolution. The most direct approach to reduce aberrations, improve the contrast and achieve an optimal resolution is to minimise the impact of changes of the refractive index along an optical path. Many implementations of light sheet fluorescence microscopy operate with a large chamber filled with an aqueous immersion medium and a further inner container with the specimen embedded in a possibly entirely different non-aqueous medium. In order to minimise the impact of the latter on the optical quality of the images, we use multi-facetted cuvettes fabricated from vacuum-formed ultra-thin fluorocarbon (FEP) foils. The ultra-thin FEP-foil cuvettes have a wall thickness of about 10–12 µm. They are impermeable to liquids, but not to gases, inert, durable, mechanically stable and flexible. Importantly, the usually fragile specimen can remain in the same cuvette from seeding to fixation, clearing and observation, without the need to remove or remount it during any of these steps. We confirm the improved imaging performance of ultra-thin FEP-foil cuvettes with excellent quality images of whole organs such us mouse oocytes, of thick tissue sections from mouse brain and kidney as well as of dense pancreas and liver organoid clusters. Our ultra-thin FEP-foil cuvettes outperform many other sample-mounting techniques in terms of a full separation of the specimen from the immersion medium, compatibility with aqueous and organic clearing media, quick specimen mounting without hydrogel embedding and their applicability for multiple-view imaging and automated image segmentation. Additionally, we show that ultra-thin FEP foil cuvettes are suitable for seeding and growing organoids over a time period of at least ten days. The new cuvettes allow the fixation and staining of specimens inside the holder, preserving the delicate morphology of e.g. fragile, mono-layered three-dimensional organoids.
Aufgrund des großen Potenzials der Nanotechnologie ist in Zukunft eine Zunahme der Produktion und Verwendung von Nanomaterialien zu erwarten, wodurch mit einer steigenden Freisetzung in der Umwelt zu rechnen ist. In der vorliegenden Dissertation werden daher Methoden zur Untersuchung von Nanomaterialien betrachtet und Effekte von NP auf Algen untersucht.
In Teil I wurden Silber-, Titandioxid- und Polystyrol-Nanopartikel sowie Kohlenstoffnano-röhrchen untersucht. Von jedem Nanomaterial standen eine unmodifizierte Form sowie zwei modifizierte Partikeltypen mit geladener Oberfläche und zusätzlich Polystyrol-Mikropartikel zur Verfügung. Zunächst erfolgte eine Charakterisierung der Materialien mittels Transmissions-elektronenmikroskopie, wobei die Größe der Objekte gemessen und das Verhalten beschrieben wurde. Zudem wurde im Fall der Polystyrol-Nanopartikel der Einfluss mehrerer Chemikalien getestet, welche im Zusammenhang mit der Probenvorbereitung für das Elektronen¬mikroskop zum Einsatz kamen. In einem nächsten Schritt erfolgte die Untersuchung von Nanomaterialien in umweltrelevanten Matrices. Hierbei wurden Boden- und Wasserproben sowie humane Körperflüssigkeiten und Fischgewebe elektronenmikroskopisch auf die Anwesenheit von synthetischen Nanomaterialien untersucht und Proben mit Nanomaterialien versetzte, um die Nachweisbarkeit mit dem Elektronenmikroskop bewerten zu können. Zusätzlich wurden verschiedene Zellkulturen und Gewebe auf morphologische Auffälligkeiten im Zusammenhang mit einer Exposition gegenüber Nanomaterialien untersucht.
Die durchgeführten Versuche zeigen, dass die Transmissionselektronenmikroskopie für viele Nanomaterialien ein sinnvolles Charakterisierungswerkzeug darstellt. Die Untersuchung besonders kleiner Partikel mit einem Durchmesser im einstelligen Nanobereich gestaltet sich jedoch schwierig bis unmöglich. Für den Nachweis von Nanomaterialien in Umweltmatrices und Zellen ist die Methode nur bedingt geeignet, wobei insbesondere niedrige Partikelkonzentrationen problematisch sind. Die Methode ist somit lediglich als Ergänzung zu anderen Nachweismethoden zu betrachten, kann jedoch hilfreiche Informationen zur Lokalisation von Nanoobjekten in Zellen und zu ihrem Verhalten in Umweltproben liefern.
In Teil II wurden die beiden Grünalgen Raphidocelis subcapitata und Chlamydomonas reinhardtii sowie die Diatomee Cyclotella meneghiniana gegenüber unterschiedlich modifizierten Silber-, Titandioxid- und Polystyrol-Nanopartikeln exponiert. Die Beurteilung der Toxizität wurde anhand der über die Absorption gemessenen Zellzahl, des Chlorophyll a Gehalts, der über die Chlorophyllfluoreszenz gemessenen Parameter Fv/Fm und NPQ sowie der transmissions¬elektronenmikroskopischen Untersuchung der Algenzellen vorgenommen. Zudem wurde der Einfluss der Beschattung von Algenzellen durch die Nanopartikel experimentell untersucht.
Die Untersuchungen zeigen, dass Nanomaterialien bei Absorptionsmessungen in Abhängigkeit von ihrem Grundmaterial, ihrer Oberflächenmodifikation und dem umgebenden Medium ein mehr oder weniger starkes Streuungsverhalten zeigen. Auch die Anwesenheit von Algen kann einen deutlichen Einfluss haben. Trotz der Beeinflussung der Lichtstreuung hat die Beschattung von Algen durch die Trübung des Mediums durch Nanomaterialien keinen Einfluss auf das Wachstum der Testorganismen. Die direkte Exposition der Algen gegenüber den Nanomaterialien zeigt, dass Silber-Nanopartikel die toxischste Wirkung haben. Die Abgabe von Silberionen durch die Partikel kann hierbei die auftretenden Effekte erklären. Auch Titandioxid-Nanopartikel führen zu negativen Effekten, wobei mögliche Gründe die Toxizität des Materials und die physikalische Isolierung der Zellen sind. Die Polystyrol-Nanopartikel haben eine stimulierende Wirkung auf die Algenzellen, welche auf einer Präferenz von adhäsivem Wachsen und dem Hormesis-Effekt beruhen kann. Die Oberflächenmodifikation der Nanomaterialien hat zwar einen Effekt auf die Toxizität, ihr Einfluss wird jedoch durch andere Faktoren überlagert. In Bezug auf die unterschiedlichen Methoden zum Nachweis der Toxizität, ist die Bestimmung des Chlorophyll a-Gehalts als besonders sensitiv zu bewerten und kann zudem auf alle Partikel angewandt werden. Hinsichtlich der Absorptionsmessung besteht teilweise ein Einfluss durch die Partikelstreuung. Die Messung der Chlorophyllfluoreszenz scheint einer starken Beeinflussung durch externe Faktoren und ggf. die Nanomaterialien selbst zu unterliegen. Die elektronenmikroskopische Untersuchung ist vergleichsweise wenig sensitiv, kann jedoch ergänzende Informationen bezüglich der Wirkweise von Nanomaterialien liefern. Der Vergleich der Testorganismen zeigt, dass Raphidocelis subcapitata empfindlicher reagiert als Chlamydomonas reinhardtii. Eine allgemeingültige Sensitivitätsabstufung zwischen den Grünalgen und der Diatomee ist nicht möglich, da die Reaktionen in Abhängigkeit von Medium bzw. Partikelgrundmaterial unterschiedlich ausfallen.
The genomes of many prokaryotes contain substantial fractions of gene pairs with overlapping stop and start codons (ATGA or TGATG). A potential benefit of overlapping gene pairs is translational coupling. In 720 genomes of archaea and bacteria representing all major phyla, we identify substantial, albeit highly variable, fractions of co-directed overlapping gene pairs. Various patterns are observed for the utilization of the SD motif for de novo initiation at upstream genes versus reinitiation at overlapping gene pairs. We experimentally test the predicted coupling in 9 gene pairs from the archaeon Haloferax volcanii and 5 gene pairs from the bacterium Escherichia coli. In 13 of 14 cases, translation of both genes is strictly coupled. Mutational analysis of SD motifs located upstream of the downstream genes indicate that the contribution of the SD to translational coupling widely varies from gene to gene. The nearly universal, abundant occurrence of overlapping gene pairs suggests that tight translational coupling is widespread in archaea and bacteria.
Die Rheumatoide Arthritis (RA) ist die häufigste chronisch-entzündliche Gelenkerkrankung, die inadäquat therapiert zu Gelenkzerstörung und resultierender Invalidität führen kann. Genetische Risikofaktoren sowie Lebensstileinflüsse führen in präklinischen Erkrankungsstadien zu posttranslationalen Modifikationen körpereigener Strukturen, die die immunologische Selbst-Toleranz brechen und zur immunologischen Fehlerkennung von Gelenkstrukturen durch B- und T-Lymphozyten führen.
Das Ziel der hier vorliegenden Arbeit war die Aufklärung von Wirkmechanismen eines für die immunmodulatorische Therapie der RA entwickelten innovativen Ansatzes zur Rekonstitution der immunologischen Autotoleranz mittels rekombinant hergestellter MHC-Klasse-II/Peptidkomplexe durch Induktion regulatorischer T-Zellen. Im Mittelpunkt der in vitro Studien steht hierbei eine über Speziesbarrieren hinweg evolutionär konservierte, von T-Lymphozyten auf dem Kollagen Typ-II (CII) erkannte, durch Glykosylierung posttranslational modifizierte, autoantigene Strukturdeterminante. Dieses T-Zellepitop (CII-Peptid) stellt sowohl in der humanen RA als auch in der murinen Experimentalerkrankung der CIA (Collagen induced arthritis) eine immunodominante Struktur der arthritogenen Autoimmunität dar. Für die modellhaften in vitro Studien zur Aufklärung der Wirkweise rekombinanter MHC-II/Peptidkomplexe auf humane T-Zellen, standen über eine Kooperation mit Prof. Rikard Holmdahl (Karolinska Institut, Stockholm) T-Zell-Hydridome mit transgener Expression des humanen MHC-II/Moleküls DR4 (DRA1/DRB1*04:01) mit unterschiedlicher Epitopspezifität (T-Zell-Hybridom 3H8, Spezifität: unmodifiziertes CII-Peptid und mDR1.1, Spezifität: galaktosyliertes CII-Peptid an Position K264) zur Verfügung. Das aus einer α- und β-Kette bestehende MHC-II/Molekül DR4 ist durch das DRA1-Gen und allelische Varianten des DRB1-Locus (stärkste RA-Assoziation: DRB1*04:01) kodiert und bildet die Form seiner Bindungstasche für die Präsentation antigener Peptide an den T-Zell-Rezeptor (TCR) auf der Oberfläche antigenpräsentierender Zellen (APC). In den Studien zur Stimulation der Hybridomzellen konnte gezeigt werden, dass die T-Zellstimulation und die daraus resultierende Zytokinausschüttung (IL-2 und IL-10) kontextabhängig ist. Je nach Stimulationsart, ob festphasengebunden- oder löslich, erfolgt die Stimulusperzeption über differente TCR-Anordnungen in Mikrodomänen der Zelloberfläche und resultiert in entsprechend modulierten Signalstärken. So führt die Zellaktivierung über die festphasengebundene Stimulation mittels MHC-II/Peptidkomplexen zur Ausbildung einer hohen TCR-Dichte, die über hohe Signalstärken zu einer spezifischen IL-2 Sekretion als Antwort führen. Die Stimulation mit monomeren DR4/CII-Peptidkomplexen in gelöster Form adressiert dagegen die auf der gesamten Zelloberfläche verteilten T-Zell-Rezeptoren, was in einer geringeren Aktivierungsdichte und einer attenuierten Gesamtsignalstärke sowie der Sekretion des immunsupressiv wirkenden IL-10 resultiert. Für den angestrebten pharmakologischen Einsatz der DR4/CII-Peptidkomplexe ist bedeutsam, dass die aktivierende TCR-Bindung der gelösten monomeren Komplexe nur partiell agonistisch wirkt und die Induktion immunregulatorischer IL-10 Zytokinantworten begünstigt. Neben der direkten T-Zellinteraktion konnte auch die Möglichkeit einer indirekten Aktivierung unter Vermittlung von APCs nach Endozytose der DR4/CII-Peptidkomplexe, ihrer lysosomalen Prozessierung und Präsentation auf endogenen neusynthetisierten DR4/Molekülen experimentell u.a. unter Verwendung der HLA-DR4- exprimierenden murinen Makrophagenlinie BL25 als APC-Modell belegt werden. Im Hinblick auf die intendierte Weiterentwicklung zu therapeutischen Anwendungen der MHC-II/CII-Peptidkomplexe unter Gesichtspunkten der Arzneimittelsicherheit ist wichtig, dass der aufgezeigte indirekte Weg der T-Zellaktivierung nach vorausgehender Prozessierung durch APCs ineffizient ist. Dieser Weg erfordert nämlich sehr hohe Konzentrationen an MHC-II/Peptidkomplexen, welche weit oberhalb der in tierexperimentellen Studien unter therapeutisch wirksamen Dosierungen erreichten Gewebespiegel liegen.
Darüber hinaus ist es uns gelungen, methodisch den Nachweis CII-spezifischer T-Zellen, die im Gesamtrepertoire der CD4+ T-Zellen im peripheren Blut von RA-Patienten (HLA-DRB1*04:01) nur in sehr niedriger Frequenz vorkommen, mittels T-Zellaktivierung und spezifischer Tetramerbindung als phänotypischen Marker zu verbessern. Für die Tetramerbindung wurden Monomere mit dem galaktosylierten CII-Peptid (CIIgal259-273) beladenen DR4/Moleküle über einen aminoterminal konjugierten Biotinrest mittels eines Fluorochromgekoppelten Streptavidins tetramerisiert. Unter Einsatz dieser Methoden ist es gelungen, aus den durchflusszytometrisch sortierten CII-spezifischen Zellen, mittels Nukleotidsequenzierung, ihr TCR-Repertoire zu analysieren und hinsichtlich präferentieller V-Genverwendung zu charakterisieren. Für zwei humane DR4-restringiert gal264CII-spezifische T-Zell-Rezeptoren aus RA-Patienten konnte die Funktionalität und Epitopspezifität durch rekombinante Expression demonstriert werden. Auf Basis der gemeinsamen Vorarbeiten mit Prof. Rikard Holmdahl im murinen CIA-Modell und den bekannten Daten zur Induktion regulatorischer T-Zellen (Tr1-Zellen) durch MHC-II/CII-Peptidkomplexe, wurden in vitro Differenzierungsexperimente an humanen PBMCs DR4-positiver RA-Patienten unter dem Einfluss von DR4/gal264CII-Peptidkomplexen durchgeführt. Die Studien belegen, dass die Komplexe mit den antigenspezifischen T-Zellen interagieren und zur Induktion von Markern eines Tr1-Phänotyps, darunter PD-1 und IL-10 führen. Zukünftige Kristallstrukturanalysen eines TCR/DR4/gal264CII-Komplexes sollen dem verbesserten molekularen Verständnis der TCR-Erkennung von CII als Autoantigen insbesondere bzgl. des flexibleren Galaktoserestes für Arthritogenität und Tolerogenität dienen. Fernziel ist die Entwicklung einer wirksamen und sicheren immunmodulatorischen Therapie der RA durch Induktion regulatorischer T-Zellen.
Atelopus is a species-rich group of Neotropical bufonids. Present knowledge on bioacoustics in this genus is relatively poor, as vocalisations have been described in only about one fifth of the ca. 100 species known. All studied members of the genus produce vocalisations although, with a few exceptions, most species lack a middle ear. Nonetheless, hearing has been demonstrated even in earless Atelopus making bioacoustics in these toads an inspiring research field. So far, three structural call types have been identified in the genus. As sympatry is uncommon in Atelopus, calls of the same type often vary little between species. Based on recordings from the 1980s, we describe vocalisations of three Venezuelan species (A. carbonerensis, A. mucubajiensis, A. tamaense) from the Cordillera de Mérida, commonly known as the Andes of Venezuela and the Tamá Massif, a Venezuelan spur of the Colombian Cordillera Oriental. Vocalisations correspond, in part, to the previously identified call types in Atelopus. Evaluation of the vocalisations of the three species presented in this study leads us to recognise a fourth structural call type for the genus. With this new addition, the Atelopus acoustic repertoire now includes (1) pulsed calls, (2) pure tone calls, (3) pulsed short calls and (4) pure tone short calls. The call descriptions provided here are valuable contributions to the bioacoustics of these Venezuelan Atelopus species, since all of them have experienced dramatic population declines that limit possibilities of further studies.
The balance between peripheral T-cell reactivity and self-tolerance is achieved during T-cell development in the thymus. During thymic development T-cell sensitivity to self-antigens drives their selection and is dynamically regulated via multiple mechanisms. The microRNA miR-181 has been implicated as a post-transcriptional modulator of T-cell sensitivity due to its suppression of several negative regulators of T-cell receptor (TCR) signalling. By tuning developing thymocytes to be exquisitely sensitive to signals transduced through their TCR, miR-181 has previously been shown to be essential for the agonist selection of invariant natural killer T (iNKT) cells. In this thesis, we extend the knowledge on the developmental control elicited by miR-181 in the thymus to cover mucosal-associated invariant T (MAIT), regulatory T (Treg) and conventional T cells. Using a germline knock-out of mature miR-181a/b-1, we could show that all agonist-selected T cell populations are critically dependant on miR-181a/b-1, noting an absence of MAIT and a reduction of thymic-derived Tregs in miR-181a/b-1-deficient mice. Furthermore, we provided evidence that miR-181 is also required for the negative selection of conventional T cells, with miR-181a/b-1-deficient mice presenting with a near absence of apoptotic markers. Therefore, by heightening the TCR sensitivity to self-antigens, miR-181a/b-1 aids in the detection and subsequent elimination of autoreactive thymocytes. In addition, we characterised the murine primary miR-181a/b-1 transcript, which surprisingly has a transcription start site (TSS) more than 70kB upstream of the mature miRNA sequences. This shall hopefully lead to future research aimed at deciphering the upstream regulatory networks that promote dynamic miR-181a/b-1 expression in developing thymocytes. In summary, we present here a single miRNA subset with broad implications in T-cell development. In disagreement with central dogma that individual miRNAs generally provide weak to moderate modulation over cellular pathways, we showcase the miR-181 family subset, miR-181a/b-1, as an efficient regulator of TCR signalling pathways. Due to the sensitive nature of TCR signalling during thymocyte selection, miR-181a/b-1 elicits gross effects, which are essential for agonist selection, central tolerance and generating a functional self-tolerant peripheral T cell repertoire. We therefore conclude that miR-181a/b-1 is fundamental in T-cell development as a whole.
The nuclear exosome and its essential co-factor, the RNA helicase MTR4, play crucial roles in several RNA degradation pathways. Besides unwinding RNA substrates for exosome-mediated degradation, MTR4 associates with RNA-binding proteins that function as adaptors in different RNA processing and decay pathways. Here, we identify and characterize the interactions of human MTR4 with a ribosome processing adaptor, NVL, and with ZCCHC8, an adaptor involved in the decay of small nuclear RNAs. We show that the unstructured regions of NVL and ZCCHC8 contain short linear motifs that bind the MTR4 arch domain in a mutually exclusive manner. These short sequences diverged from the arch-interacting motif (AIM) of yeast rRNA processing factors. Our results suggest that nuclear exosome adaptors have evolved canonical and non-canonical AIM sequences to target human MTR4 and demonstrate the versatility and specificity with which the MTR4 arch domain can recruit a repertoire of different RNA-binding proteins.
Orthologs document the evolution of genes and metabolic capacities encoded in extant and ancient genomes. However, the similarity between orthologs decays with time, and ultimately it becomes insufficient to infer common ancestry. This leaves ancient gene set reconstructions incomplete and distorted to an unknown extent. Here we introduce the "evolutionary traceability" as a measure that quantifies, for each protein, the evolutionary distance beyond which the sensitivity of the ortholog search becomes limiting. Using yeast, we show that genes that were thought to date back to the last universal common ancestor are of high traceability. Their functions mostly involve catalysis, ion transport, and ribonucleoprotein complex assembly. In turn, the fraction of yeast genes whose traceability is not sufficient to infer their presence in last universal common ancestor is enriched for regulatory functions. Computing the traceabilities of genes that have been experimentally characterized as being essential for a self-replicating cell reveals that many of the genes that lack orthologs outside bacteria have low traceability. This leaves open whether their orthologs in the eukaryotic and archaeal domains have been overlooked. Looking at the example of REC8, a protein essential for chromosome cohesion, we demonstrate how a traceability-informed adjustment of the search sensitivity identifies hitherto missed orthologs in the fast-evolving microsporidia. Taken together, the evolutionary traceability helps to differentiate between true absence and nondetection of orthologs, and thus improves our understanding about the evolutionary conservation of functional protein networks. "protTrace," a software tool for computing evolutionary traceability, is freely available at https://github.com/BIONF/protTrace.git; last accessed February 10, 2019.
Acinetobacter baumannii is a Gram-negative pathogen that causes a multitude of nosocomial infections. The Acinetobacter trimeric autotransporter adhesin (Ata) belongs to the superfamily of trimeric autotransporter adhesins which are important virulence factors in many Gram-negative species. Phylogenetic profiling revealed that ata is present in 78% of all sequenced A. baumannii isolates but only in 2% of the closely related species A. calcoaceticus and A. pittii. Employing a markerless ata deletion mutant of A. baumannii ATCC 19606 we show that adhesion to and invasion into human endothelial and epithelial cells depend on Ata. Infection of primary human umbilical cord vein endothelial cells (HUVECs) with A. baumannii led to the secretion of interleukin (IL)-6 and IL-8 in a time- and Ata-dependent manner. Furthermore, infection of HUVECs by WT A. baumannii was associated with higher rates of apoptosis via activation of caspases-3 and caspase-7, but not necrosis, in comparison to ∆ata. Ata deletion mutants were furthermore attenuated in their ability to kill larvae of Galleria mellonella and to survive in larvae when injected at sublethal doses. This indicates that Ata is an important multifunctional virulence factor in A. baumannii that mediates adhesion and invasion, induces apoptosis and contributes to pathogenicity in vivo.
The division Ascomycota(Fungi) contains a large number of taxa known to reproduce only asexually by the formation of conidia or other non-motile propagules produced by mitotic cellular devisions. They are called anamorphic, mitosporic, asexual or conidial fungi and ecologically, they are often found associated with plant debris in different stages of decay. In general, saprobic anamorphs of ascomycetous affinities are poorly studied and their outstanding diversity is currently underexplored. Phylogenetic relationships are unknown for many of them and they are still largely underrepresented in the current phylogenetic classification system of Fungi, with many morphologically defined anamorphic taxa still awaiting taxonomic reassessment in the light of molecular approaches. The increasing usage of molecular markers combined with robust statistical methods has allowed their phylogenetic affinities to be revealed and to gradually incorporate many of them into the different taxonomic groups of the division Ascomycota. However, the phylogenetic placement and taxonomic status of a large number of saprobic taxa remain unresolved due to the lack of DNA sequence data.
The present dissertation aims to explore the rich but understudied diversity of those anamorphic fungi traditionally known as hyphomycetes that inhabit dead plant debris. It consists of five publications in which a polyphasic approach integrating morphological, developmental, cultural and molecular data was used to incorporate novel or incertae sedis taxa within Ascomycota and to make more sound decisions regarding their taxonomic status. Specific objectives include: 1. the collection, isolation and morphological characterization of selected anamorphic fungi representing putative new or interesting taxa of uncertain phylogenetic placement; 2. the generation of novel DNA sequence data to infer their phylogenetic relationships and to resolve their taxonomic affinities within Ascomycota; 3. the testing of any previously available morphologically based hypotheses on their putative position, generic placement or relationships with teleomorphic, pleomorphic or other anamorphic taxa; and 4. the determination of their generic validity, monophyly and taxonomic boundaries using molecular data and phylogenetic analyses methods.
Materials studied in these five projects consisted of specimens collected during field work carried out by the author or collaborators in different countries including USA, the Czech Republic and Panama between the years 2014 and 2017. The target substrates were dead leaves of different palm trees, dead wood and bark of pines and twigs or stems of unknown shrubs and woody vines that are all known to harbor a rich saprobic mycobiota. Putative novelties or anamorphic taxa with unknown or poorly studied phylogenetic affinities were selected for further morphological and molecular investigation. Micromorphological studies were based on fungal structures observed on natural substrate, herbarium specimens and in culture. DNA was extracted from cultures and PCR amplification followed by Sanger sequencing was carried out using relevant molecular markers employed in fungal phylogenetic studies. Newly obtained DNA sequence data were analyzed following a standard phylogenetic analysis pipeline and phylogenetic relationships were reconstructed using character-based methods such as Maximum Likelihood and Bayesian inference.
Conclusion is that anamorphic Ascomycota inhabiting dead plant debris represents a largely untapped source of biodiversity and information still in need of further exploration. A new capnodiaceous genus Castanedospora, seven new species named Taeniolella sabalicola, Hermatomyces bifurcatus, H. constrictus, H. megasporus, H. sphaericoides, H. verrucosus and Septonema lohmanii, and two new combinations, Castanedospora pachyanthicola and H. reticulatus, are proposed based on morphological and DNA sequence data. Molecular phylogenetics was confirmed as the tool of choice for the inference of relationships in novel or incertae sedis anamorphic fungi that are otherwise difficult to assess in the absence of a teleomorphic state. They were first resolved or revisited for several saprobic species such as Ernakulamia cochinensis, H. sphaericus, H. tucumanensis or Septonema fasciculare in a suitable framework for phylogenetic hypothesis testing. Molecular data allowed to fully incorporate all these taxa in Ascomycota, particularly within the classes Dothideomycetes and Sordariomycetes, and to provide a foundation for better taxonomic decisions on their classification. Large and polyphyletic genera such as Taeniolella, Sporidesmium and Septonema, partially treated in this work and containing mostly saprobic species of obscure affinities, remained in need of further investigation.
Synthesis and SAR of the antistaphylococcal natural product nematophin from Xenorhabdus nematophila
(2019)
The repeated and improper use of antibiotics had led to an increased number of multiresistant bacteria. Therefore, new lead structures are needed. Here, the synthesis and an expanded structure–activity relationship of the simple and antistaphylococcal amide nematophin from Xenorhabdus nematophila and synthetic derivatives are described. Moreover, the synthesis of intrinsic fluorescent derivatives, incorporating azaindole moieties was achieved for the first time.
Communication sounds are ubiquitous in the animal kingdom, where they play a role in advertising physiological states and/or socio-contextual scenarios. Distress sounds, for example, are typically uttered in distressful scenarios such as agonistic interactions. Here, we report on the occurrence of superfast temporal periodicities in distress calls emitted by bats (species Carollia perspicillata). Distress vocalizations uttered by this bat species are temporally modulated at frequencies close to 1.7 kHz, that is, ∼17 times faster than modulation rates observed in human screams. Fast temporal periodicities are represented in the bats’ brain by means of frequency following responses, and temporally periodic sounds are more effective in boosting the heart rate of awake bats than their demodulated versions. Altogether, our data suggest that bats, an animal group classically regarded as ultrasonic, can exploit the low frequency portion of the soundscape during distress calling to create spectro-temporally complex, arousing sounds.
Background: Developmental biology relies to a large extent on the observation and comparison of phenotypic traits through time using high resolution microscopes. In this context, transparent model organisms such as the zebrafish Danio rerio in which developing tissues and organs can be easily observed and imaged using fluorescent proteins have become very popular. One limiting factor however is the acquisition of a sufficient amount of data, in standardized and reproducible conditions, to allow robust quantitative analysis. One way to improve this is by developing mounting methods to increase the number of embryos that can be imaged simultaneously in near-to-identical orientation.
Results: Here we present an improved mounting method allowing semi-automated and high-content imaging of zebrafish embryos. It is based on a 3D-printed stamp which is used to create a 2D coordinate system of multiple μ-wells in an agarose cast. Each μ-well models a negative of the average zebrafish embryo morphology between 22 and 96 h-post-fertilization. Due to this standardized and reproducible arrangement, it is possible to define a custom well plate in the respective imaging software that allows for a semi-automated imaging process. Furthermore, the improvement in Z-orientation significantly reduces post-processing and improves comparability of volumetric data while reducing light exposure and thus photo-bleaching and photo-toxicity, and improving signal-to-noise ratio (SNR).
Conclusions: We present here a new method that allows to standardize and improve mounting and imaging of embryos. The 3D-printed stamp creates a 2D coordinate system of μ-wells in an agarose cast thus standardizing specimen mounting and allowing high-content imaging of up to 44 live or mounted zebrafish embryos simultaneously in a semi-automated, well-plate like manner on inverted confocal microscopes. In summary, image data quality and acquisition efficiency (amount of data per time) are significantly improved. The latter might also be crucial when using the services of a microscopy facility.
Understanding global biodiversity patterns is one of the main objectives of ecology. Spatial variation in species richness can be explained by several environmental factors. The relationships between species richness and environmental factors have been associated with latitudinal, longitudinal and elevational gradients. The number of species is determined by birth, death and migration rates of species in a given area. These rates are affected by abiotic and biotic factors acting at local and regional scales. Climatic seasonal variation may also influence biodiversity, directly through physiological limitations and indirectly through biotic interactions, vegetation structure and food availability. Climate and land use change are the main factors for landscape simplification and biotic homogenization. Thus, the study of community patterns across environmental gradients may help to predict the effect of projected environmental change.
I investigated how abiotic and biotic factors influence different facets of bird diversity across an elevational gradient. My study was conducted along an elevational gradient spanning 2000 m within and around Podocarpus National Park and San Francisco reserve on the southeastern slope of the Andes in Ecuador. The climate is humid tropical montane with a bimodal rain regime. The region is characterized by evergreen premontane forest at low elevations, evergreen lower montane forest at mid elevations and upper montane forest at high elevations. The elevational gradient has natural continuous forests within the protected reserves and fragmented forests surrounding the reserves in a matrix of cattle pastures. To monitor bird diversity, I placed nine 20-m radius point counts within 18 one-hectare plots, in continuous and fragmented forest at 1000, 2000 and 3000 m a.s.l. I recorded and identified all birds for 10 minutes within each point count. Bird communities were sampled eight times per plot, in the most humid season and in the least humid season of 2014 and 2015. To estimate flower and fruit availability, I recorded all plants with open flowers and ripe fruits within each point count. To obtain the relative invertebrate availability, I assessed understory invertebrate fresh biomass using a standardized sweep-netting design along 100-metre borders of each plot. Vertical vegetation heterogeneity was estimated at eight layers above the ground within each point count. Temperature for each plot was obtained using an air temperature regionalization tool and precipitation through remote sensing techniques and meteorological data.
In the first chapter of this thesis, I explored the effects of elevation, climate and vegetation structure on overall bird communities as well as on frugivorous and insectivorous birds. I found that elevation was mostly indirectly associated with bird diversity, jointly mediated via temperature, precipitation and vegetation structure. Additionally, elevation was directly and positively associated with both the overall bird community and with insectivores, but not with frugivores. My findings indicate a reduction of bird diversity due to climatic factors and vegetation structure with increasing elevation. However, the direct, positive effect of elevation suggests that bird diversity was higher than expected towards high elevations, probably due to spatial, biotic and evolutionary settings.
In the second chapter, I analysed the influence of climate and resource availability on temporal variation of bird communities. I found a higher bird diversity in the least humid season than in the most humid season. The seasonality of the bird communities was mainly driven by temperature and precipitation. While temperature had a significant positive effect at high elevations, precipitation had a significant negative effect at low elevations. Resource availability had no significant effect. My findings suggest that the temporal fluctuations in bird communities likely occur due to climate
constraints rather than due to resource limitations.
In the third chapter, I studied the effect of forest fragmentation on taxonomic and functional bird diversity. I found that taxonomic diversity was higher in fragmented compared to continuous forests, while functional diversity was negatively affected by fragmentation, but only at low elevations. The increase of taxonomic diversity in disturbed habitats suggests an increase of habitat generalists, which may compensate the loss of forest specialists. My findings suggest that taxonomic diversity can be uncoupled from functional diversity in diverse communities at low elevations.
My results show the effects of environmental factors on the spatio-temporal patterns of bird communities and the potentially uncoupled responses of taxonomic and functional diversity to forest fragmentation. My findings highlight that bird communities respond differently to abiotic and biotic factors across elevational gradients. Overall, my study helps to better understand the mechanisms that drive species communities in response to complex environmental conditions, which could be an essential contribution for the conservation of bird communities in the tropical Andes.
The neocortical microcircuit, a local network of excitatory and inhibitory neurons, is a highly complex information processing unit, which can flexibly be modulated to adapt to external context and internal state such as motivation or attention. The mechanisms underlying these adaptations for flexible processing are not sufficiently understood yet. The aim of this study is to further elucidate the role of inhibitory and excitatory components of the local neocortical microcircuit for the processing of sensory information in an awake, behaving animal.
Layer 1 of the neocortex is of particular importance because it contains afferents from the thalamus and more distant cortical regions, which relay top-down information that is important for processes such as learning and attention. The dendrites of the excitatory pyramidal neurons located in deeper layers extend into layer 1, and in addition to that layer 1 contains inhibitory neurons, as well as axons from inhibitory somatostatin expressing (SOM) neurons located in lower layers. These layer 1 inhibitory neurons and SOM axons are therefore well positioned to control top-down information transfer at the pyramidal dendrites, and thus to flexibly regulate information processing in the local circuit. To further investigate this, the stimulus responses in inhibitory (SOM axons) and excitatory (layer 2/3 pyramidal neurons) components of the neocortical microcircuit were measured in primary auditory cortex during learning, when auditory stimuli gain relevance.
For this purpose, I first established a suitable learning behaviour, an auditory GO-NOGO discrimination task, which can be performed by head-fixed mice under the microscope. The task also contains a visual start cue, which signals the start of every trial, as a multimodal element. Mice learn to distinguish two auditory stimuli by being rewarded with water after the GO stimulus and receiving no reward after the NOGO stimulus. They indicate that they have identified the stimuli accordingly by licking at a water dispenser during the GO stimulus and not during the NOGO stimulus. Licking during the NOGO stimulus is punished by an aversive air puff. As the mice learn this behaviour, the stimuli gain relevance. The activity in the same neuronal structures was observed over the course of all training sessions via 2-photon imaging in awake, behaving mice, and their stimulus responses were measured throughout the learning process, acquiring a comprehensive dataset. In these data, short-term and long-term plasticity of the stimulus responses can be detected and these changes in the stimulus responses differ for SOM axons and pyramidal neurons. Already from the first training day, stimulus responses change in the course of a single session, both in SOM axons and in pyramidal cells. With time over the course of task acquisition, the stimulus representation in a group of pyramidal neurons in layer 2/3 is enhanced and distal dendrites are less inhibited over training through reduced activation of the SOM axons, so that the integration of information along the somatodendritic axis shifts, increasing the relative impact of top-down information. This shift is even stronger for the NOGO stimulus in correct trials compared to the GO stimulus. This is the first study to show that this somato-dendritic shift by SOM-axon responses occurs at different strengths for the GO and NOGO stimulus, probably due to the different learned responses (action or refraining), which require different forms of circuit control. After learning, the neuronal responses to GO and NOGO stimuli also differ in pyramidal neurons, with the GO stimulus evoking stronger responses than the NOGO stimulus. This learned distinction is reversed in passive trials during which the mice have no possibility to respond to the stimuli, in both SOM axons and pyramidal neurons, resulting in similar response sizes for both stimuli. This indicates that not only learning over the long term, but also short-term changes regarding the state (active execution of the discrimination task or no active participation during the stimulus presentations) affect the processing of the stimuli in the local circuit. In addition, on an even shorter time scale pyramidal neurons show a modulation of responses from trial to trial, probably due to anticipation of reward, which is absent from SOM axon responses. Thus, there are various levels of plasticity that develop over the course of training: long-term changes in the response size of both the excitatory and inhibitory components that facilitate stimulus recognition when engaged, and short-term modulation (possibly in anticipation of reward) in excitatory neurons that could underlie sensorimotor transformation. Both pyramidal neurons and SOM axons in the primary auditory cortex respond to multimodal and reinforcement-related stimuli, likely contributing to the optimisation of circuit dynamics for goal-directed information processing. This shows that the circuit flexibly adjusts information processing under different circumstances, depending on the relevance the stimuli carry and whether the mouse is active or inactive and can use the presented information to achieve a goal.
Zinc finger domains are highly structured and can mediate interactions to DNA, RNA, proteins, lipids, and small molecules. Accordingly, zinc finger proteins are very versatile and involved in many biological functions. Eukaryotes contain a wealth of zinc finger proteins, but zinc finger proteins have also been found in archaea and bacteria. Large zinc finger proteins have been well studied, however, in stark contrast, single domain zinc finger µ-proteins of less than 70 amino acids have not been studied at all, with one single exception. Therefore, 16 zinc finger µ-proteins of the haloarchaeon Haloferax volcanii were chosen and in frame deletion mutants of the cognate genes were generated. The phenotypes of mutants and wild-type were compared under eight different conditions, which were chosen to represent various pathways and involve many genes. None of the mutants differed from the wild-type under optimal or near-optimal conditions. However, 12 of the 16 mutants exhibited a phenotypic difference under at least one of the four following conditions: Growth in synthetic medium with glycerol, growth in the presence of bile acids, biofilm formation, and swarming. In total, 16 loss of function and 11 gain of function phenotypes were observed. Five mutants indicated counter-regulation of a sessile versus a motile life style in H. volcanii. In conclusion, the generation and analysis of a set of deletion mutants demonstrated the high importance of zinc finger µ-proteins for various biological functions, and it will be the basis for future mechanistic insight.
Hereditary Parkinson’s disease (PD) can be triggered by an autosomal dominant overdose of alpha-Synuclein (SNCA) as stressor or the autosomal recessive deficiency of PINK1 Serine/Threonine-phosphorylation activity as stress-response. We demonstrated the combination of PINK1-knockout with overexpression of SNCAA53T in double mutant (DM) mice to exacerbate locomotor deficits and to reduce lifespan. To survey posttranslational modifications of proteins underlying the pathology, brain hemispheres of old DM mice underwent quantitative label-free global proteomic mass spectrometry, focused on Ser/Thr-phosphorylations. As an exceptionally strong effect, we detected >300-fold reductions of phosphoThr1928 in MAP1B, a microtubule-associated protein, and a similar reduction of phosphoSer3781 in ANK2, an interactor of microtubules. MAP1B depletion is known to trigger perturbations of microtubular mitochondria trafficking, neurite extension, and synaptic function, so it was noteworthy that relevantly decreased phosphorylation was also detected for other microtubule and microfilament factors, namely MAP2S1801, MARK1S394, MAP1AT1794, KIF1AS1537, 4.1NS541, 4.1GS86, and ADD2S528. While the MAP1B heavy chain supports regeneration and growth cones, its light chain assists DAPK1-mediated autophagy. Interestingly, relevant phosphorylation decreases of DAPK2S299, VPS13DS2429, and VPS13CS2480 in the DM brain affected regulators of autophagy, which are implicated in PD. Overall, significant downregulations were enriched for PFAM C2 domains, other kinases, and synaptic transmission factors upon automated bioinformatics, while upregulations were not enriched for selective motifs or pathways. Validation experiments confirmed the change of LC3 processing as reflection of excessive autophagy in DM brain, and dependence of ANK2/MAP1B expression on PINK1 levels. Our new data provide independent confirmation in a mouse model with combined PARK1/PARK4/PARK6 pathology that MAP1B/ANK2 phosphorylation events are implicated in Parkinsonian neurodegeneration. These findings expand on previous observations in Drosophila melanogaster that the MAP1B ortholog futsch in the presynapse is a primary target of the PARK8 protein LRRK2, and on a report that MAP1B is a component of the pathological Lewy body aggregates in PD patient brains. Similarly, ANK2 gene locus variants are associated with the risk of PD, ANK2 interacts with PINK1/Parkin-target proteins such as MIRO1 or ATP1A2, and ANK2-derived peptides are potent inhibitors of autophagy.
The website Sci-Hub enables users to download PDF versions of scholarly articles, including many articles that are paywalled at their journal’s site. Sci-Hub has grown rapidly since its creation in 2011, but the extent of its coverage has been unclear. Here we report that, as of March 2017, Sci-Hub’s database contains 68.9% of the 81.6 million scholarly articles registered with Crossref and 85.1% of articles published in toll access journals. We find that coverage varies by discipline and publisher, and that Sci-Hub preferentially covers popular, paywalled content. For toll access articles, we find that Sci-Hub provides greater coverage than the University of Pennsylvania, a major research university in the United States. Green open access to toll access articles via licit services, on the other hand, remains quite limited. Our interactive browser at https://greenelab.github.io/scihub allows users to explore these findings in more detail. For the first time, nearly all scholarly literature is available gratis to anyone with an Internet connection, suggesting the toll access business model may become unsustainable.
Die Neurowissenschaften sind in Forschungsarbeiten für Schüler und Studierende immer wieder als eines der schwierigsten Teilgebiete der Biologie angeführt. Die Inhalte werden überwiegend nicht verstanden. Als mögliche Ursache gelten die seltenen praktischen Zugänge für die Lernenden aufgrund limitierter Ressourcen. Diese Ursache konnte in der vorliegenden Arbeit durch eine Befragung der Lehrkräfte zu ihren Praxisumsetzungen bestätigt werden. 70 % der Lehrkräfte gaben an, dass sie keine Experimente in der Schule zum Thema Nervenzellen anbieten. Experimente zur Verhaltensbiologie führen 65 % der Lehrkräfte nicht durch.
Um Schülern die Möglichkeit zu geben, sich experimentell mit den Themenfeldern der Neuro- und Verhaltensbiologie auseinanderzusetzen, wurden im Rahmen der vorliegenden Arbeit Schülerlabortage auf dem Feld der Neurowissenschaften konzipiert. Die Konzepte wurden schülerorientiert umgesetzt und neurowissenschaftliche Forschung durch den eigenen Umgang mit modernen Forschungsapparaturen erfahrbar gemacht. Die drei Labortage für die Sekundarstufe II wurden wissenschaftlich begleitet: 1) Verhaltensbiologie, 2) systemische Ebene der Elektrophysiologie, 3) elektrophysiologische Forschungsmethoden. Um die Qualität und Wirksamkeit der Labortage beurteilen zu können, wurden sie mit Feedbackerhebungen begleitet. Die drei Labortage wurden sowohl von den Lehrkräften als auch von den Schülern bezüglich ihrer Qualität positiv bewertet. Für die Schüler konnte gezeigt werden, dass die Beurteilung weitgehend unabhängig von einem zugrunde liegenden Interesse an Biologie und Forschung ausfällt. Anhand einer retrospektiven Erhebung wird außerdem gezeigt, dass alle drei Labortage eine höchst signifikante, selbsteingeschätzte Steigerung des „Wissens“, der „Anwendungszuversicht“ und des „Interesses“ bewirken. Schüler mit niedrigen Ausgangswerten zeigen einen besonders hohen Anstieg. Für das Interesse kann weiter gezeigt werden, dass auch Schüler mit hohem Ausgangswert eine große Interessenssteigerung durch den Labortag aufweisen. Das Interesse für den verhaltensbiologischen Labortag liegt etwas niedriger – die Labortage mit elektrophysiologischen Inhalten zeigen dagegen für die Anwendungszuversicht etwas niedrigere Werte.
Der Fokus der fachdidaktischen Forschung lag auf der Betrachtung des experimentellen Zugangs zur Elektrophysiologie über ein entwickeltes „EPhys-Setup“. Dabei handelt es sich um einen quasi-realen Messaufbau. Die Umsetzung kombiniert dazu Komponenten eines realen Elektrophysiologie-Setups (Hands-on Komponenten) mit einer speziell entwickelten schülerfreundlichen Software (Neurosimulation) und einem virtuellen Nervensystem in Form einer Platine. Als Modellnervensystem werden für diese Umsetzung Ganglien von Hirudo medicinalis verwendet – der Neurosimulation liegen originale elektrophysiologische Messspuren des Ganglions zugrunde. Experimentelle Vermittlungsansätze für die Elektrophysiologie finden sich kaum für den Schulbereich. Dem Bedarf einer entsprechenden Beforschung wurde mit verschiedenen Testinstrumenten nachgegangen, um den Vermittlungsansatz mit dem EPhys-Setup bewerten zu können. Dafür fand eine Wirksamkeitsanalyse über die Erhebung der Motivation der Schüler statt (Lab Motivation Scale; Dohn et al. 2016). Von Bedeutung war auch, inwiefern gegenüber der Umsetzung eine Technologieakzeptanz vorliegt (Technology Acceptance Model; Davis 1989), die im Schulkontext ausgehend von der steigenden Einbindung von Technologien einen entsprechenden Forschungsbedarf aufweist. Weiter wurde untersucht, ob sich die Bewertung des EPhys-Setups von der Bewertung einer Kontrollgruppe unterscheidet. Für die Kontrollgruppe wurde die Neurosimulation von den Hands-on Komponenten gelöst und die Schüler arbeiteten ausschließlich PC-basiert. Die Ergebnisse zeigen, dass beide Umsetzungen die Motivation förderten und eine Technologieakzeptanz bei den Schülern aufwiesen. Der Unterschied der Untersuchungsgruppen fällt gering aus. Die Abhängigkeiten, die für die verwendete Simulationsumsetzung gefunden wurden, beziehen sich ausschließlich auf Komponenten der „Freude“. Somit wird der intrinsische Bereich von den Schülern die am EPhys-Setup gearbeitet haben höher bewertet. Zur weiteren Analyse der Testinstrumente wurde auch eine Abhängigkeit der Bewertung vom zugrunde liegenden Biologieinteresse sowie von den Computerfähigkeiten vergleichend betrachtet. Der Einfluss auf die Bewertungen der drei Testskalen ist in vielen Fällen höher als der Einfluss der verwendeten Simulation. Vom individuellen Biologieinteresse der Schüler zeigen alle untersuchten Komponenten eine Abhängigkeit. Die größeren Effekte beziehen sich auf die Komponenten der „Lernwirksamkeit“ oder der „Freude“. Von den individuellen Computerfähigkeiten der Schüler zeigen Komponenten zur „Zuversicht bezüglich der Methoden und der Inhalte“ eine Abhängigkeit.
Proteins encoded by small open reading frames (sORFs) have a widespread occurrence in diverse microorganisms and can be of high functional importance. However, due to annotation biases and their technically challenging direct detection, these small proteins have been overlooked for a long time and were only recently rediscovered. The currently rapidly growing number of such proteins requires efficient methods to investigate their structure–function relationship. Herein, a method is presented for fast determination of the conformational properties of small proteins. Their small size makes them perfectly amenable for solution-state NMR spectroscopy. NMR spectroscopy can provide detailed information about their conformational states (folded, partially folded, and unstructured). In the context of the priority program on small proteins funded by the German research foundation (SPP2002), 27 small proteins from 9 different bacterial and archaeal organisms have been investigated. It is found that most of these small proteins are unstructured or partially folded. Bioinformatics tools predict that some of these unstructured proteins can potentially fold upon complex formation. A protocol for fast NMR spectroscopy structure elucidation is described for the small proteins that adopt a persistently folded structure by implementation of new NMR technologies, including automated resonance assignment and nonuniform sampling in combination with targeted acquisition.
Natural products (NPs) from microorganisms have been important sources for discovering new therapeutic and chemical entities. While their corresponding biosynthetic gene clusters (BGCs) can be easily identified by gene-sequence-similarity-based bioinformatics strategies, the actual access to these NPs for structure elucidation and bioactivity testing remains difficult. Deletion of the gene encoding the RNA chaperone, Hfq, results in strains losing the production of most NPs. By exchanging the native promoter of a desired BGC against an inducible promoter in Δhfq mutants, almost exclusive production of the corresponding NP from the targeted BGC in Photorhabdus, Xenorhabdus and Pseudomonas was observed including the production of several new NPs derived from previously uncharacterized non-ribosomal peptide synthetases (NRPS). This easyPACId approach (easy Promoter Activated Compound Identification) facilitates NP identification due to low interference from other NPs. Moreover, it allows direct bioactivity testing of supernatants containing secreted NPs, without laborious purification.
Climate change forces many species to move their ranges to higher latitudes or elevations. Resulting immigration or emigration of species might lead to functional changes, e.g., in the trait distribution and composition of ecological assemblages. Here, we combined approaches from biogeography (species distribution models; SDMs) and community ecology (functional diversity) to investigate potential effects of climate-driven range changes on frugivorous bird assemblages along a 3000 m elevational gradient in the tropical Andes. We used SDMs to model current and projected future occurrence probabilities of frugivorous bird species from the lowlands to the tree line. SDM-derived probabilities of occurrence were combined with traits relevant for seed dispersal of fleshy-fruited plants to calculate functional dispersion (FDis; a measure of functional diversity) for current and future bird assemblages. Comparisons of FDis between current and projected future assemblages showed consistent results across four dispersal scenarios, five climate models and two representative concentration pathways. Projections indicated a decrease of FDis in the lowlands, an increase of FDis at lower mid-elevations and little changes at high elevations. This suggests that functional dispersion responds differently to global warming at different elevational levels, likely modifying avian seed dispersal functions and plant regeneration in forest ecosystems along tropical mountains.
Frontal areas of the mammalian cortex are thought to be important for cognitive control and complex behaviour. These areas have been studied mostly in humans, non-human primates and rodents. In this article, we present a quantitative characterization of response properties of a frontal auditory area responsive to sound in the bat brain, the frontal auditory field (FAF). Bats are highly vocal animals and they constitute an important experimental model for studying the auditory system. At present, little is known about neuronal sound processing in the bat FAF. We combined electrophysiology experiments and computational simulations to compare the response properties of auditory neurons found in the bat FAF and auditory cortex (AC) to simple sounds (pure tones). Anatomical studies have shown that the latter provide feedforward inputs to the former. Our results show that bat FAF neurons are responsive to sounds, however, when compared to AC neurons, they presented sparser, less precise spiking and longer-lasting responses. Based on the results of an integrate-and-fire neuronal model, we speculate that slow, low-threshold, synaptic dynamics could contribute to the changes in activity pattern that occur as information travels through cortico-cortical projections from the AC to the FAF.
A new cyclic lipopeptide, phototemtide A (1), was isolated from Escherichia coli expressing the biosynthetic gene cluster pttABC from Photorhabdus temperata Meg1. The structure of 1 was elucidated by HR‐ESI‐MS and NMR experiments. The absolute configurations of amino acids and 3‐hydroxyoctanoic acid in 1 were determined by using the advanced Marfey's method and comparison after total synthesis of 1, respectively. Additionally, three new minor derivatives, phototemtides B–D (2–4), were identified by detailed HPLC–MS analysis. Phototemtide A (1) showed weak antiprotozoal activity against Plasmodium falciparum, with an IC50 value of 9.8 μm. The biosynthesis of phototemtides A–D (1–4) was also proposed.
Truffle fungi are well known for their enticing aromas partially emitted by microbes colonizing truffle fruiting bodies. The identity and diversity of these microbes remain poorly investigated, because few studies have determined truffle-associated bacterial communities while considering only a small number of fruiting bodies. Hence, the factors driving the assembly of truffle microbiomes are yet to be elucidated. Here we investigated the bacterial community structure of more than 50 fruiting bodies of the black truffle Tuber aestivum in one French and one Swiss orchard using 16S rRNA gene amplicon high-throughput sequencing. Bacterial communities from truffles collected in both orchards shared their main dominant taxa: while 60% of fruiting bodies were dominated by α-Proteobacteria, in some cases the β-Proteobacteria or the Sphingobacteriia classes were the most abundant, suggesting that specific factors (i.e., truffle maturation and soil properties) shape differently truffle-associated microbiomes. We further attempted to assess the influence in truffle microbiome variation of factors related to collection season, truffle mating type, degree of maturation, and location within the truffle orchards. These factors had differential effects between the two truffle orchards, with season being the strongest predictor of community variation in the French orchard, and spatial location in the Swiss one. Surprisingly, genotype and fruiting body maturation did not have a significant effect on microbial community composition. In summary, our results show, regardless of the geographical location considered, the existence of heterogeneous bacterial communities within T. aestivum fruiting bodies that are dominated by three bacterial classes. They also indicate that factors shaping microbial communities within truffle fruiting bodies differ across local conditions.
Numerous cell–cell and cell–matrix interactions within the bone marrow microenvironment enable the controlled lifelong self-renewal and progeny of hematopoietic stem and progenitor cells (HSPCs). On the cellular level, this highly mutual interaction is granted by cell adhesion molecules (CAMs) integrating differentiation, proliferation, and pro-survival signals from the surrounding microenvironment to the inner cell. However, cell–cell and cell–matrix interactions are also critically involved during malignant transformation of hematopoietic stem/progenitor cells. It has become increasingly apparent that leukemia-associated gene products, such as activated tyrosine kinases and fusion proteins resulting from chromosomal translocations, directly regulate the activation status of adhesion molecules, thereby directing the leukemic phenotype. These observations imply that interference with adhesion molecule function represents a promising treatment strategy to target pre-leukemic and leukemic lesions within the bone marrow niche. Focusing on myeloid leukemia, we provide a current overview of the mechanisms by which leukemogenic gene products hijack control of cellular adhesion to subsequently disturb normal hematopoiesis and promote leukemia development.
The overarching aim of this doctoral research was to examine and quantify the spatiotemporal variability in the movements of nomadic ungulates to better understand the possible drivers and characteristics of such movements as well as to examine the particular conservation challenges associated with nomadic movements.
Durch natürliche Selektion werden Funktionen, die dem Überleben und dem Fortpflanzungserfolg eines Organismus dienen, optimiert. Da die Struktur eines Organs dessen Funktion und umgekehrt die Funktion eines Organs dessen Struktur bestimmt, kann durch das Studium der Morphologie die Funktionsweise von Organen verstanden werden. Trotz des umfangreichen Wissens über die Struktur von Nervensystemen sowohl auf mikro- als auch auf makroskopischer Ebene, ist es weiterhin unklar, wie Bewusstsein und ein kohärentes Abbild der Umwelt im Gehirn erzeugt werden. Der Grund hierfür ist vor allem die gewaltige Komplexität neuronaler Netzwerke, die unmöglich geistig erfasst werden können. Eine Möglichkeit, das Gehirn ohne das detaillierte Wissen über all seine Bestandteile zu verstehen, bietet das Studium von Optimierungsprinzipien und deren Anwendung in theoretischen Modellen. So wie eingangs erwähnt die Funktion von Organen durch natürliche Selektion optimiert wird, sollte auch die Funktion neuronaler Netzwerke optimiert werden und neuronale Netzwerke sollten entsprechend solcher Optimierungsprinzipien aufgebaut sein. Ein wichtiges Prinzip, das essenziell für die Effizienz neuronaler Netzwerke ist, ist die Minimierung der Verbindungslänge zwischen Neuronen. Basierend auf diesem Prinzip wurde im Rahmen dieser Dissertation eine algorithmische Methode etabliert, die es ermöglicht Vorhersagen der relativen Position von Neuronen anhand ihrer Verbindungen zu treffen. Diese neuronale Platzierungsmethode beruht darauf, dass Neuronen mit ähnlicher Verbindungsnachbarschaft näher zueinander platziert werden als zu Neuronen mit weniger ähnlichen Verbindungsnachbarn, wodurch die durchschnittliche Verbindungslänge minimiert wird. Nach der Etablierung dieser Methode, wurde diese benutzt um Modelle zu erstellen, die es ermöglichen die Entstehung neuronaler Karten und kortikaler Faltungen im Zusammenhang mit der Konnektivität und der Anzahl der Neuronen zu untersuchen.
Neuronale Karten sind geordnete Muster auf der Oberfläche des Kortex, die durch die präferierte Aktivität einzelner Neuronen in Antwort auf Stimuli einer Modalität beobachtet werden können. Im visuellen Kortex existieren sogar mehrere Karten, je nachdem welche Qualität visueller Stimuli man betrachtet. Abhängig von der Präferenz für einen Sehwinkel, ein stimuliertes Auge oder der Orientierung eines Balken-Stimulus, können retinotopische Karten, Karten mit streifenartigen Mustern oder Karten mit sogenannten „Pinwheel“-Strukturen beobachtet werden. Pinwheels sind periodische Strukturen, die sichtbar werden indem man die Orientierungspräferenz von Neuronen für die spezifische Orientierung eines Balken-Stimulus mit der entsprechenden Farbe des Farbkreises visualisiert. Da diese Strukturen eine Ähnlichkeit mit bunten Windrädern haben, werde sie als Pinwheels bezeichnet. Die in dieser Dissertation erstellten Modelle sagen vorher, dass die Entstehung strukturierter neuronaler Karten im Allgemeinen von der Anzahl der Neuronen abhängt. In der Tat könnte diese Abhängigkeit auch für neuronale Karten im Kortex gelten. Während strukturierte Karten im visuellen Kortex in verschiedenen Säugerordnungen wie Primaten, Karnivoren und Huftieren existieren, sind sie in kleinen Nagern mit weniger Neuronen nicht vorhanden, trotz ähnlicher Verbindungsspezifizität. Folglich müssen Unterschiede in der Struktur neuronaler Karten im Kortex nicht zwangsläufig mit einer unterschiedlichen Funktionsweise zusammenhängen, sondern könnten auch durch allgemeine Optimierungsprinzipien beim Aufbau neuronaler Netzwerke bedingt werden. Eine weitere Gemeinsamkeit zwischen verschiedenen Säugetierordnungen ist, dass die relative Dichte der Pinwheels ziemlich genau bei der Zahl Pi liegt. Entsprechend der Ergebnisse dieser Dissertation könnte dies dadurch erklärt werden, dass für neuronale Karten ähnlicher Struktur die Anzahl der Neuronen pro Pinwheel relativ konstant ist. Unterschiede in der räumlichen Dichte der Pinwheels könnten dann einfach durch Unterschiede in der Dichte der Neuronen erklärt werden.
Neben den Modellen für neuronale Karten wurde im Rahmen dieser Dissertation auch ein Modell kortikaler Faltungen mit derselben neuronalen Platzierungsmethode erstellt. Die Existenz kortikaler Faltungen wird gemeinhin damit erklärt, dass der Kortex ohne Faltungen wegen seiner verhältnismäßig großen Oberfläche nicht in den Schädel gepackt werden könnte. Allerdings haben Experimente gezeigt, dass die Faltungen nicht durch eine Restriktion des wachsenden Kortex an der Schädeloberfläche entstehen, da auch mit mehr Platz für die Expansion des Kortex die gleichen Faltungsmuster exprimiert werden. Interessanterweise entstehen die kortikalen Faltungen erst, wenn die Proliferation der Neuronen während der Entwicklung größtenteils abgeschlossen ist und die Neuronen anfangen ihre Verbindungen auszubilden. Um kortikale Faltungen basierend auf der Konnektivität zwischen Neuronen im Modell vorherzusagen, genügt es das allgemeine Muster einer starken lokalen, aber schwachen globalen Konnektivität zwischen Neuronen nachzubilden. Abhängig von Variationen dieser Konnektivität, der Anzahl der kortikalen Kolumnen und der Neuronenanzahl innerhalb dieser Kolumnen, können im Modell viele Eigenschaften kortikaler Faltungsmuster in Säugetieren vorhergesagt werden. Ähnlich wie in Säugetieren ist der Faltungsgrad der vom Modell vorhergesagt wird von dem Verhältnis zwischen Parametern, die die Größe und Dicke des Kortex beschreiben, abhängig. Dementsprechend werden mehr und mehr Faltungen mit steigender Anzahl der Kolumnen, aber gleicher Anzahl von Neuronen pro Kolumne vorhergesagt. Wie in Säugetieren entstehen dabei auch die größeren primären Faltungen zuerst bevor es innerhalb der größeren Faltungen zu kleineren Faltungen höherer Ordnung kommt. Neben der Abhängigkeit des Faltungsgrads von der Größe des Kortex können Variationen in der Konnektivität erklären, wie es einerseits zu stereotypischen Faltungsmustern kommen kann, aber andererseits auch warum der Faltungsgrad zwischen verschiedenen Säugerordnungen unterschiedlich mit der Größe des Kortex skaliert. Letztlich könnten pathologische Veränderungen der Konnektivität zu den entsprechenden Änderungen im Faltungsmuster führen.
Insgesamt wurde in dieser Arbeit gezeigt, dass mittels einfacher Prinzipien, die die Verbindung zwischen Neuronen und deren relative Position zueinander beschreiben, komplexe neuroanatomische Strukturen vorhergesagt werden können. Da mit derselben Methode zur neuronalen Platzierung sowohl neuronale Karten als auch kortikalen Faltungen, also sehr unterschiedliche Strukturen vorhergesagt werden konnten, stellt sich die Frage, ob diese Strukturen durch einen gemeinsamen biologischen Mechanismus entstehen. Neuronale Zugkräfte sind ein möglicher Mechanismus, der die Entstehung kortikaler Faltungen erklären könnte. Auch wenn es eher unwahrscheinlich ist, dass die Entstehung neuronaler Karten von Zugkräften zwischen Neuronen abhängt, kann es nicht vollständig ausgeschlossen werden. Ob solche Kräfte an der Selbstorganisation neuronaler Netzwerke beteiligt sein könnten, ist eine interessante Fragestellung für zukünftige empirische Studien.
Summary
Wild relatives of crops thrive in habitats where environmental conditions can be restrictive for productivity and survival of cultivated species. The genetic basis of this variability, particularly for tolerance to high temperatures, is not well understood. We examined the capacity of wild and cultivated accessions to acclimate to rapid temperature elevations that cause heat stress (HS).
We investigated genotypic variation in thermotolerance of seedlings of wild and cultivated accessions. The contribution of polymorphisms associated with thermotolerance variation was examined regarding alterations in function of the identified gene.
We show that tomato germplasm underwent a progressive loss of acclimation to strong temperature elevations. Sensitivity is associated with intronic polymorphisms in the HS transcription factor HsfA2 which affect the splicing efficiency of its pre‐mRNA. Intron splicing in wild species results in increased synthesis of isoform HsfA2‐II, implicated in the early stress response, at the expense of HsfA2‐I which is involved in establishing short‐term acclimation and thermotolerance.
We propose that the selection for modern HsfA2 haplotypes reduced the ability of cultivated tomatoes to rapidly acclimate to temperature elevations, but enhanced their short‐term acclimation capacity. Hence, we provide evidence that alternative splicing has a central role in the definition of plant fitness plasticity to stressful conditions.
Mapping biodiversity is the marathon of the 21st Century as an answer to the present extinction crisis. A century in which science is also characterised by large scientific datasets collected through new technologies aiming to fill gaps in our knowledge of species distributions. However, most species records rely on observations that are not linked to specimens, which does not allow verification of species hypotheses by other scientists. Natural history museums form a verifiable source of biodiversity records which were made by taxonomists. Nonetheless, these museums seem to be forgotten by biologists in scientific fields other than taxonomy or systematics. Naturalis Biodiversity Center (NBC) in Leiden is care keeper of large collections of marine organisms, which were sampled in the Northeast Atlantic during the CANCAP and Tyro Mauritania II expeditions (1976–1988). Many octocorals were sampled and deposited in the NBC collection, where they became available for study and were partially identified by the senior author (M.G.) in the 1980s. Nonetheless, no checklist or taxonomic revision was published so far with the complete results. In 2016 the first author visited NBC to examine NE Atlantic Plexauridae octocorals. Plexauridae octocoral-vouchered records were listed and mapped to reveal high standard primary biodiversity records unreported so far for the NE Atlantic Ocean. Twenty-four Plexauridae species with ~ six putative new species to science were discovered and eleven new biogeographical records were made from distinct Macaronesian archipelagos. Finally, new depth range records were found for three species at sea basin level and for eight species at a regional scale.
Nanoplastics (NP) and microplastics (MP) accumulate in our environment as a consequence of the massive consumption of plastics. Huge knowledge-gaps exist regarding uptake and fate of plastic particles in micro- and nano-dimensions in humans as well as on their impact on human health.
This study investigated the transport and effects of 50 nm and 0.5 μm COOH-modified polystyrene (PS) particles, as representatives for NP and MP, in different biological models in vitro. Acute toxicity and potential translocation of the particles were studied at the human intestinal and placental barrier using advanced in vitro co-culture models. Furthermore, embryotoxicity and genotoxicity were investigated as highly sensitive endpoints.
Polystyrene was not acutely toxic in both sizes (nano- and microparticles). No transport across the intestinal and placental barrier but a cellular uptake and intracellular accumulation of PS nano- and microparticles were determined. The particles were identified as weak embryotoxic and non-genotoxic.
In contrast to single-organ studies, this multi-endpoint study is providing a data-set with the exact same type of particles to compare organ-specific outcomes. Our study clearly shows the need to investigate other types of plastics as well as towards long-term or chronic effects of plastic particles in different biological models in vitro.
Autophagy, meaning “self-eating”, is an important cellular waste disposal mechanism. Thereby, damaged proteins, lipids and organelles are enclosed by autophagosomes and subsequently transported to the lysosomes for degradation into basic, cellular building blocks. Under basal conditions autophagy prevents the accumulation of defective and harmful material and generally promotes cell survival. However, several studies reported that hyperactivated autophagy, e.g. during developmental processes in lower eukaryotes, or during chemotherapeutic treatment of cancer cells, can also trigger cell death.
In recent years, autophagic cell death (ACD) has been considered as an alternative cell death pathway for tumor therapy, especially for solid tumors with high apoptosis resistance such as glioblastoma. Glioblastoma (GBM) is a very aggressive, malignant primary brain tumor with a median survival of ~ 15 months despite surgery and chemoradiotherapy. Accordingly, there is a great interest in improving GBM therapy through alternative cell death mechanisms. Interestingly, it has been shown that various substances, e.g. AT 101, cannabinoids and the combination of imipramine and ticlopidine (IM+TIC), induce ACD in GBM cells.
The aim of this project was to identify the underlying mechanisms of stress- and drug-induced ACD and its therapeutic potential for glioblastoma treatment. For detailed investigation of ACD, a CRISPR/Cas9-based approach was used to generate ATG5 and ATG7 knockouts as genetic models of autophagy deficiency. In a previous study of our lab it was demonstrated that administration of AT 101 triggers ACD in glioblastoma cells, which was associated with early mitochondrial fragmentation but no signs of apoptosis. Since mitochondrial fragmentation often precedes mitophagy, the first part of this thesis explored the potential role of mitophagy in AT 101-induced cell death.
ATG5-depleted cells confirmed that AT 101 induces ACD. In addition, treatment with AT 101 resulted in a pronounced mitochondrial depolarization, which was at least partly caused by the opening of the mitochondrial permeability pore. Global proteome analysis of AT 101-treated GBM cells revealed a robust decrease in mitochondrial protein clusters as well as a strong increase in the enzyme heme oxygenase-1 (HMOX1). Subsequent experiments for detailed investigation of mitophagy following AT 101 treatment (western blot, flow cytometric MTG and mt-mKeima, qRT-PCR of mitochondrial vs nuclear DNA) consistently indicated strong mitophagy induction by AT 101, which could be reduced by genetic or pharmacological inhibition of autophagy. Furthermore, siRNA-mediated knockdown experiments revealed that the selective mitophagy receptors BNIP3 and BNIP3L and the HMOX1 enzyme play an essential role in AT 101-induced mitophagy and subsequent cell death. Taken together, these data demonstrate that AT 101-induced mitochondrial dysfunction and HMOX1 induction synergize to promote excessive mitophagy with a lethal outcome in glioma cells.
The second part of this thesis focused on the identification of new substances that cause ACD and the investigation of the underlying cell death pathways. Using a cell death screen of the ENZO Screen-Well™ autophagy library in MZ-54 wild-type vs ATG5 and ATG7-depleted cells, loperamide, pimozide, and STF-62247 were identified as ACD-inducing agents. The increase of the autophagic flux and the induction of ACD by these substances was confirmed by using different ATG5 and ATG7 knockout cell lines and the already established positive control IM+TIC.
In contrast to AT 101, IM+TIC, STF-62247, loperamide and pimozide produced neither mitochondrial dysfunction nor mitophagy. Interestingly, it has been described that imipramine, loperamide and pimozide inhibit the lysosomal enzyme acid sphingomyelinase, which is associated with impaired lipid transport. Global proteome analysis and cholesterol staining confirmed that all four substances, but especially loperamide and pimozide, inhibit cellular lipid transport, leading to massive lipid accumulation in the lysosomes. In the further course of the experiments, the connection between defective lipid transport and autophagy was investigated in more detail. On the one hand, the defective lipid transport contributed to the induction of autophagy, on the other hand the massive accumulation of lipids led to lysosomal membrane damage, inhibition of lysosomal degradation at later time points and finally to a lysosomal cell death. Remarkably, it has been shown that hyperactivated autophagy by IM+TIC, loperamide and pimozide massively promotes lysosomal membrane damage. This result highlights the difficulties of a clear distinction between autophagic and lysosomal cell death.
In summary, two new signaling pathways that induce autophagic cell death in GBM cells and may be relevant for glioblastoma therapy were investigated in this study.
Frontal areas of the mammalian cortex are thought to be important for cognitive control and complex behaviour. These areas have been studied mostly in humans, non-human primates and rodents. In this article, we present a quantitative characterization of response properties of a frontal auditory area responsive to sound in the brain of Carollia perspicillata, the frontal auditory field (FAF). Bats are highly vocal animals, and they constitute an important experimental model for studying the auditory system. We combined electrophysiology experiments and computational simulations to compare the response properties of auditory neurons found in the bat FAF and auditory cortex (AC) to simple sounds (pure tones). Anatomical studies have shown that the latter provides feedforward inputs to the former. Our results show that bat FAF neurons are responsive to sounds, and however, when compared to AC neurons, they presented sparser, less precise spiking and longer-lasting responses. Based on the results of an integrate-and-fire neuronal model, we suggest that slow, subthreshold, synaptic dynamics can account for the activity pattern of neurons in the FAF. These properties reflect the general function of the frontal cortex and likely result from its connections with multiple brain regions, including cortico-cortical projections from the AC to the FAF.
Holocarpic oomycetes are poorly known but widespread parasites in freshwater and marine ecosystems. Most of the holocarpic species seem to belong to clades that diverge before the two crown lineages of the oomycetes, the Saprolegniomycetes and the Peronosporomycetes. Recently, the genus Miracula was described to accommodate Miracula helgolandica, a holocarpic parasitoid of Pseudo-nitzschia diatoms, which received varying support for its placement as the earliest-diverging oomycete lineage. In the same phylogenetic reconstruction, Miracula helgolandica was grouped with some somewhat divergent sequences derived from environmental sequencing, indicating that Miracula would not remain monotypic. Here, a second species of Miracula is reported, which was found as a parasitoid in the limnic centric diatom Pleurosira leavis. Its life-cycle stages are described and depicted in this study and its phylogenetic placement in the genus Miracula revealed. As a consequence, the newly discovered species is introduced as Miracula moenusica.
Wolves (Canis lupus) are currently showing a remarkable comeback in the highly frag-mented cultural landscapes of Germany. We here show that wolf numbers increasedexponentially between 2000 and 2015 with an annual increase of about 36%. Wedemonstrate that the first territories in each newly colonized region were establishedover long distances from the nearest known reproducing pack on active militarytraining areas (MTAs). We show that MTAs, rather than protected areas, served asstepping-stones for the recolonization of Germany facilitating subsequent spreadingof wolf territories in the surrounding landscape. We did not find any significant differ-ence between MTAs and protected areas with regard to habitat. One possible reasonfor the importance of MTAs may be their lower anthropogenic mortality rates com-pared to protected and other areas. To our knowledge, this is the first documented casewhere MTAs facilitate the recolonization of an endangered species across large areas.
Microenvironmental regulation of tumor progression and therapeutic response in brain metastasis
(2019)
Cellular and non-cellular components of the tumor microenvironment (TME) are emerging as key regulators of primary tumor progression, organ-specific metastasis, and therapeutic response. In the era of TME-targeted- and immunotherapies, cancer-associated inflammation has gained increasing attention. In this regard, the brain represents a unique and highly specialized organ. It has long been regarded as an immunological sanctuary site where the presence of the blood brain barrier (BBB) and blood cerebrospinal fluid barrier (BCB) restricts the entry of immune cells from the periphery. Consequently, tumor cells that metastasize to the brain were thought to be shielded from systemic immune surveillance and destruction. However, the detailed characterization of the immune landscape within border-associated areas of the central nervous system (CNS), such as the meninges and the choroid plexus, as well as the discovery of lymphatics and channels that connect the CNS with the periphery, have recently challenged the dogma of the immune privileged status of the brain. Moreover, the presence of brain metastases (BrM) disrupts the integrity of the BBB and BCB. Indeed, BrM induce the recruitment of different immune cells from the myeloid and lymphoid lineage to the CNS. Blood-borne immune cells together with brain-resident cell-types, such as astrocytes, microglia, and neurons, form a highly complex and dynamic TME that affects tumor cell survival and modulates the mode of immune responses that are elicited by brain metastatic tumor cells. In this review, we will summarize recent findings on heterotypic interactions within the brain metastatic TME and highlight specific functions of brain-resident and recruited cells at different rate-limiting steps of the metastatic cascade. Based on the insight from recent studies, we will discuss new opportunities and challenges for TME-targeted and immunotherapies for BrM.
Cyanobacteria are photoautotrophic microorganisms present in almost all ecologically niches on Earth. They exist as single-cell or filamentous forms and the latter often contain specialized cells for N2 fixation known as heterocysts. Heterocysts arise from photosynthetic active vegetative cells by multiple morphological and physiological rearrangements including the absence of O2 evolution and CO2 fixation. The key function of this cell type is carried out by the metalloprotein complex known as nitrogenase. Additionally, many other important processes in heterocysts also depend on metalloproteins. This leads to a high metal demand exceeding the one of other bacteria in content and concentration during heterocyst development and in mature heterocysts. This review provides an overview on the current knowledge of the transition metals and metalloproteins required by heterocysts in heterocyst-forming cyanobacteria. It discusses the molecular, physiological, and physicochemical properties of metalloproteins involved in N2 fixation, H2 metabolism, electron transport chains, oxidative stress management, storage, energy metabolism, and metabolic networks in the diazotrophic filament. This provides a detailed and comprehensive picture on the heterocyst demands for Fe, Cu, Mo, Ni, Mn, V, and Zn as cofactors for metalloproteins and highlights the importance of such metalloproteins for the biology of cyanobacterial heterocysts.
Die Differenzierung zwischen Teilpopulationen hin zu unterschiedlichen Arten kann nur erfolgen, wenn zwischen diesen Teilpopulationen reproduktive Isolation besteht. Wie die unterschiedlichen Arten von reproduktiver Isolation zusammenwirken und welche Voraussetzungen bestehen müssen, um neue Arten zu bilden, muss in jedem Studiensystem untersucht werden. Ein idealer Ansatzpunkt sind Arten, die sich mehrfach an anspruchsvolle Habitate angepasst haben, deren Artbildung also von ökologischen Habitatparametern bestimmt wird. Dieser Vorgang wird als Ökologische Artbildung bezeichnet. Im Artkomplex Poecilia spec., der im Süden Mexikos mehrere schwefelangepasste Ökotypen ausgebildet hat, wurden erste Hinweise auf eine Korrelation zwischen der Selektionsstärke von natürlicher und sexueller Selektion gefunden, deren Einfluss zusammen die bestehenden reproduktiven Barrieren zwischen Klarwasser- und Schwefelökotyp formen. Wie diese Reproduktionsbarrieren beschaffen sind und wie die Umweltvariable Schwefel auf die Morphologie und das Verhalten der Poeciliiden Einfluss nimmt, wurde in der vorliegenden Arbeit anhand von fünf Fragestellungen untersucht. (1) Die Körperfärbung kann ein aussagekräftiges Signal für die Qualität des potentiellen Partners bei der Fortpflanzung sein. Wie beeinflusst die extreme Umweltvariable Schwefel die Ausbildung von Färbung? (2) Sind die gefundenen Anpassungen der Färbung erblich oder werden sie plastisch entsprechend des Nahrungsangebots ausgebildet? (3) In einem der untersuchten Flusssysteme konnte unvollständige reproduktive Isolation zwischen der Klarwasser- und Schwefelpopulation nachgewiesen werden. Sind in den Mischzonen zwischen diesen beiden Habitaten Hybriden genetisch nachweisbar und bilden diese die Färbungsanpassungen der Klarwasser-, der Schwefelpopulation oder eine intermediäre Form aus? (4) Die Gelbfärbung der Flossen bei Männchen scheint ein geeignetes Merkmal für die Anzeige der Qualität zu sein, da es möglicherweise unabhängig vom Nahrungsangebot ausgebildet wird. Besteht eine weibliche Präferenz für dieses Merkmal? (5) Auch die weibliche Partnerwahlpräferenz wird vom Habitat und dem eigenen Zustand beeinflusst. Wie verändert sich die Präferenz für Männchen mit gutem Ernährungszustand bei Weibchen, die hungrig sind?
Um diese Fragen zu beantworten, wurden in mehreren Jahren Männchen und Weibchen der Arten Poecilia mexicana und Poecilia sulphuraria aus sieben Populationen im Studiengebiet in Südmexiko gefangen und auf ihre Färbung untersucht sowie Laborpopulationen getestet. Es konnten generelle Anpassungen der Färbung an die Umweltvariable Schwefel nachgewiesen werden. Dazu gehören die Aufhellung der Körperregionen, die durch Tarnung (konkret: countershading und background matching) vor Entdeckung durch Prädatoren schützen, und die Reduktion von Gelb- und Rottönen. Diese Anpassung ist vermutlich auf das geringe Angebot an Karotinoiden in den schwefelbelasteten Extremhabitaten zurückzuführen. Außerdem konnten zahlreiche flusssystem¬spezifische Anpassungen beschrieben werden, deren Ursachen in den Unterschieden zwischen den Schwefelhabitaten untereinander begründet sind. Das Flusssystem des Río Tacotalpa stellt hier eine Besonderheit dar, da Männchen eine besonders starke Gelbfärbung der Flossen aufweisen. Wildgefangene und laborgeborene Männchen dieses Flusssystems wurden verglichen, um einen Hinweis auf den Einfluss des Nahrungsangebots auf dieses Merkmal zu untersuchen. Tatsächlich ist die Ausprägung dieses Merkmals, die Gelbfärbung der Flossen, unabhängig vom Angebot an Karotinoiden. Während die hier verwendeten genetischen Analysen nicht geeignet waren, Hybriden aus den Mischzonen zwischen Schwefel- und Klarwasserhabitat nachzuweisen, ergaben die Untersuchungen von Individuen aus den Mischzonen keine eindeutigen Ergebnisse über eine etwaige intermediäre Ausbildung der Färbung. Die Präsentation von Männchen, deren Gelbintensität an den Flossenspitzen künstlich verändert wurde, konnte bei Weibchen keine eindeutige Präferenz für stärker gefärbte Männchen aufzeigen. Vielmehr weist dieses Ergebnis auf eine starke Korrelation zwischen mehreren Merkmalen (z. B. weitere morphologische Merkmale, Verhalten) hin, die für die Beurteilung der männlichen Qualität herangezogen werden. Die weibliche Präferenz für konditionsabhängige Merkmale wird bei schwefelangepassten Weibchen leicht verstärkt, wenn diese hungrig sind. Eine solche flexible Präferenz sollte gerade in Habitaten mit starken Fluktuationen im Nährstoffangebot existieren. Dabei waren Weibchen, denen Videoaufnahmen präsentiert wurden, eher in der Lage, das qualitativ hochwertigere Männchen zu identifizieren, als Weibchen, denen animierte Bilder präsentiert wurden. Auch hier wird davon ausgegangen, dass die Reduktion auf eines oder wenige Merkmale, die für die Partnerwahl zur Verfügung stehen, keine ausreichend starke Reaktion auslösen können. Vielmehr ist der Zugriff auf alle Aspekte der männlichen Erscheinung wichtig, um die Qualität des potentiellen Partners zu beurteilen.
Färbung ist also generell geeignet, den Ökotyp eines Individuums zu bestimmen und ein solches Merkmal kann der Artbestimmung im ersten Schritt der Partnerwahl dienen. Dasjenige männliche Färbungsmerkmal, das über mehrere Generationen gleichbleibend ausgeprägt wurde – die Gelbfärbung der Flossen – reicht jedoch nicht aus, um bei der weiblichen Partnerwahl eine Reaktion auszulösen. Vielmehr deuten die Ergebnisse auf eine enge Korrelation der Färbung mit weiteren Merkmalen in Morphologie und Verhalten eines Individuums hin, die vom wählenden Weibchen stets gemeinsam entsprechend der Multiple-message-Theorie betrachtet werden. Auch der Vergleich zwischen Videoaufnahmen und animierten Fotografien als Stimuli bei der Partnerwahl ergab, dass der Aspekt Verhalten (nur verfügbar mit Videoaufnahmen) für eine Partnerwahlentscheidung von Bedeutung ist.
Meine Arbeit konnte den bestehenden Wissensschatz um die bestehenden reproduktiven Barrieren im Studiensystem um den Aspekt der Färbung erweitern. Meine Ergebnisse zeigen weitere spannende Fragestellungen auf. Je größer das Verständnis der vorliegenden Selektionskräfte und Mechanismen reproduktiver Isolation ist, desto besser kann die Wissenschaft verstehen, welche Umgebungsvariablen welchen Einfluss auf den Prozess der Artbildung haben.
Cardiovascular diseases are a leading cause of morbidity and mortality worldwide. Aging inflicts structural and molecular changes on the heart that oftentimes involve ischemic events, cardiomyocyte apoptosis and cardiac stiffening, which makes it a major risk factor for cardiovascular disease. After being disregarded as transcriptional noise for a long time, long non-coding RNAs have lately emerged as key regulators of many cellular processes in physiology and disease of virtually all tissues and organs, with some of them being differentially regulated during aging.
This study identified a long non-coding transcript antisense to the OXCT1 gene locus, Sarrah, to be downregulated in the heart during aging, after acute myocardial infarction and upon heart failure with preserved ejection fraction. Sarrah is expressed in several cardiac cell types with highest levels in cardiomyocytes, where it is predominantly localized in the nucleus. In mouse and human cardiomyocytes, Sarrah levels are reduced upon exposure to hypoxia or treatment with hypoxiamimetic agents in vitro.
Sarrah exerts an anti-apoptotic function in mouse and human cardiomyocytes as assessed from caspase activity and annexin V staining. Histological stainings of Sarrah-depleted human engineered heart tissue organoids and Sarrah overexpressing infarcted mouse hearts confirmed its anti-apoptotic function. Sarrah also plays a role in cardiomyocyte contractility, which is substantially impaired upon Sarrah silencing in human engineered heart tissue and neonatal rat cardiomyocytes. Additionally, cardiomyocytal Sarrah stimulates endothelial cell proliferation via paracrine effects as observed after Sarrah overexpression in mouse hearts as well as in co-culture settings with human endothelial cells and Sarrah-depleted or Sarrah overexpressing human cardiomyocytes. A microarray analysis revealed that silencing Sarrah in human cardiomyocytes induced apoptosisrelated gene expression. Mechanistically, Sarrah was predicted to form triplexes in human and mouse with promoters of genes downregulated, but not upregulated after Sarrah knockdown, suggesting that Sarrah interacts with target genes to activate their transcription. This interaction was confirmed in vitro using nucleic acid oligonucleotides containing the sequences of the Sarrah triplex motif and the Sarrah binding site of the exemplary target gene GPC6 of both human and mouse. RNA immunoprecipitation experiments in human cells demonstrated that Sarrah is associated with open chromatin, transcription factor CRIP2, transcriptional co-activator p300 and DNA-RNA hybrid structures that also occur in Sarrah target gene promoters, which indicated that Sarrah activates gene expression by triplex formation and recruitment of protein interaction partners. Deleting the triplex motif of endogenous Sarrah in mouse cardiomyocytes augmented apoptosis, showing that triplex formation is of functional relevance for Sarrah action.
Finally, overexpressing Sarrah in an acute myocardial infarction mouse model improved recovery of cardiac contractile function as assessed from ejection fraction, stroke volume, wall motion and wall thickness measured by echocardiography and magnetic resonance imaging. Infarct size was substantially reduced in Sarrah overexpressing mice compared with controls. This in vivo study implies that restoring Sarrah levels in the aged or infarcted heart bears significant therapeutic potential, which can be attributed to the combination of three Sarrah effects: increased cardiomyocytes survival, enhanced contractility of individual cardiomyocytes and paracrine stimulation of endothelial cell proliferation likely contributing to increased angiogenesis and tissue perfusion.
In summary, cardiac lncRNA Sarrah is evolutionary conserved with regard to its genomic locus, function and molecular mechanism. Via triplex formation with gene promoters, it is capable to activate a set of target genes that together mediate the anti-apoptotic and pro-contractile function of Sarrah in cardiomyocytes and that confer angiogenic effects to endothelial cells. A therapeutic utilization of Sarrah in the context of myocardial ischemia is conceivable in the future if Sarrah upregulation proves to be beneficial in further studies.