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Analysis of photosystem I (PSI) complexes from Cyclotella meneghiniana cultured under different growth conditions led to the identification of three groups of antenna proteins, having molecular weights of around 19, 18, and 17 kDa. The 19-kDa proteins have earlier been demonstrated to be more peripherally bound to PSI, and their amount in the PSI complexes was significantly reduced when the iron supply in the growth medium was lowered. This polypeptide was almost missing, and thus the total amount of fucoxanthin-chlorophyll proteins (Fcps) bound to PSI was reduced as well. When treating cells with high light in addition, no further changes in antenna polypeptide composition were detected. Xanthophyll cycle pigments were found to be bound to all Fcps of PSI. However, PSI of high light cultures had a significantly higher diatoxanthin to diadinoxanthin ratio, which is assumed to protect against a surplus of excitation energy. PSI complexes from the double-stressed cultures (high light plus reduced iron supply) were slightly more sensitive against destruction by the detergent treatment. This could be seen as a higher 674-nm emission at 77 K in comparison to the PSI complexes isolated from other growth conditions. Two major emission bands of the Fcps bound to PSI at 77 K could be identified, whereby chlorophyll a fluorescing at 697 nm was more strongly coupled to the PSI core than those fluorescing at 685 nm. Thus, the build up of the PSI antenna of several Fcp components enables variable reactions to several stress factors commonly experienced by the diatoms in vivo, in particular diatoxanthin enrichment under high light and reduction of antenna size under reduced iron conditions.
Xenorhabdus and Photorhabdus spp. are bacterial symbionts of entomopathogenic nematodes (EPNs). In this study, we isolated and characterized Xenorhabdus and Photorhabdus spp. from across Thailand together with their associated nematode symbionts, and characterized their phylogenetic diversity. EPNs were isolated from soil samples using a Galleria-baiting technique. Bacteria from EPNs were cultured and genotyped based on recA sequence. The nematodes were identified based on sequences of 28S rDNA and internal transcribed spacer regions. A total of 795 soil samples were collected from 159 sites in 13 provinces across Thailand. A total of 126 EPNs isolated from samples taken from 10 provinces were positive for Xenorhabdus (n = 69) or Photorhabdus spp. (n = 57). Phylogenetic analysis separated the 69 Xenorhabdus isolates into 4 groups. Groups 1, 2 and 3 consisting of 52, 13 and 1 isolates related to X. stockiae, and group 4 consisting of 3 isolates related to X. miraniensis. The EPN host for isolates related to X. stockiae was S. websteri, and for X. miraniensis was S. khoisanae. The Photorhabdus species were identified as P. luminescens (n = 56) and P. asymbiotica (n = 1). Phylogenenic analysis divided P. luminescens into five groups. Groups 1 and 2 consisted of 45 and 8 isolates defined as subspecies hainanensis and akhurstii, respectively. One isolate was related to hainanensis and akhurstii, two isolates were related to laumondii, and one isolate was the pathogenic species P. asymbiotica subsp. australis. H. indica was the major EPN host for Photorhabdus. This study reveals the genetic diversity of Xenorhabdus and Photorhabdus spp. and describes new associations between EPNs and their bacterial symbionts in Thailand.
EGFL7 regulates adult neural stem cell maintenance and differentiation by inhibition of Notch1
(2010)
In neurobiology the preexisting dogma on the unchangeability of the adult mammalian brain and its inability to give rise to new neurons has been challenged since the early nineties. Generally, it is now accepted that neurogenesis persists in adults. Progress in developmental and stem cell biology in recent years led to an increasing interest in regeneration-based treatment strategies for damaged tissue of the central nervous system. Thus, the enhancement of the endogenous potential of the brain to repair itself is potentially a feasible therapeutic strategy to treat various types of brain damage. Therefore, it is of great interest to understand the molecular mechanism that regulate adult neurogenesis. One of the prominent pathways suggested to be involved here is the Notch signaling cascade. Previously, it has been shown that various components of Notch signaling are expressed in the stem cell niche of the adult subventricular zone (SVZ) in vivo. Interestingly, a recent study demonstrated that the self-renewal potential of adult neural stem cells (NSCs) isolated from the SVZ depend on Notch signaling in vitro.
Recently, we identified a novel non-canonical Notch ligand termed epidermal growth factor-like domain 7 (EGFL7), which was originally described as a protein secreted by endothelial cells and functionally implicated in cellular responses of the vascular system such as cell migration and blood vessel formation. We were able to show that secreted EGFL7 binds to a region in Notch that is involved in ligand-mediated receptor activation, thus acting as an antagonist of Notch signaling.
The present study identifies neurons of the human and murine brain as a novel source of EGFL7, which suggests functions of EGFL7 in the neural system. Expression analyses by quantitative RT-PCR (qRT-PCR) revealed EGFL7 is down regulated in the adult SVZ, which suggests that endogenous EGFL7 may act as a Notch modulator of NSCs. We assessed the expression of Notch pathway components in adult NSCs isolated from the SVZ of adult mice and demonstrated that inhibition of Notch activity by the γ-secretase inhibitor DAPT reduced the self-renewal potential of NSCs. Accordingly, adenoviral-mediated expression of EGFL7 in vitro decreased Notch-specific signaling and reduced proliferation and self-renewal of NSCs. Conversely, activation of Notch by a constitutive active form of Notch (NICD) rescued the EGFL7-mediated reduction of NSC self-renewal verifying that this effect was directly linked to Notch signaling. Congruent to the reduced proliferation rate measured in vitro, induced expression of EGFL7 in vivo significantly reduced the number of Ki-67 positive cells within the SVZ upon cerebroventricular injection of EGFL7 adenovirus.
Expression analyses in the developing brain showed single EGFL7-positive cells within the marginal zone of the neocortex as measured by in situ hybridization. These cells might be Cajal-Retzius cells, specialized neurons, which specifically express Reelin, which is a protein of the extracellular matrix known to control neuronal migration and differentiation. Interstingly, we could show that Reelin and EGFL7 are expressed in a subtype of neurons of the adult mouse cortex. This implied an interaction of both proteins and was verified by co-immunoprecipitation assays, suggesting an additional role for EGFL7 in neuronal maintenance. QRT-PCR based expression analyses in vitro comparing differentiated and non-differentiated NSCs displayed an increase in EGFL7 expression during the differentiation process, which was paralled by reduced Notch signaling. NSCs differentiated on coverslips coated with EGFL7 differentiated into all three cell types - neurons, oligodendrocytes and astrocytes. EGFL7 favored the formation of neurons as compared to control comparable to the effect of the Notch-inhibitor DAPT. Furthermore, additional oligodendrocytes were formed. These cells displayed a mature morphology with distinct sprouts and branches in contrast to the small and round oligodendrocytes that formed on control coverslips, which resembled us of precursor cells. Neurons and oligodendrocytes were formed at the expense of astrocytes. Congruently to the effect observed in vitro, adenoviral-based expression of EGFL7 in the SVZ yielded a slight induction of neuronal differentiation in vivo. Taken together, these results show for the first time a previously unrecognized role for EGFL7 in the brain by modulation of the Notch pathway in adult NSCs, which changes the proliferation and differentiation potential of adult NSCs in vitro and in vivo.
Protein translocation across the chloroplast membrane is mediated by molecular machinery composed of protein complexes termed the TOC/TIC (the outer/inner envelope chloroplasts translocases). This translocation process is regulated by metabolic energy in form of GTP and ATP and is influenced by the lipid composition of the membrane. The ability to study the function of a single complex “TOC” in vitro using purified protein or purified chloroplast outer envelope vesicles has been instrumental for our understanding of the mechanism underlying this process.
Indeed, the TOC complex has been purified by previously established procedures. However its functional and structural analyses are impaired by the limited yield of purified protein. Therefore, protocols for native TOC complex purification are described here. The complex isolation is achieved by direct biochemical treatment of biological membrane hosting this complex or by tandem affinity purification of modified protein complex components from generated transgenic plants.
Furthermore, in this thesis, radioactive based in vitro import assays are described, namely those that allow monitoring translocation activity across the outer envelope of chloroplast. Based on the analysis of knock-out plants and isolated complexes it was previously suggested that lipid dependence of protein translocation might exist. Thus, the question was raised whether the lipid composition of the membrane has a direct influence on the behavior and functionality of the TOC translocon, or whether additional components of the chloroplast membrane account for the observed effect in vivo. To answer this question, a technique for vesicle fusion was developed. The principal aim was to explore the effect of an exchange of the lipid environment surrounding the complex translocon. This method helped to demonstrate that the SQDG and PI act stimulatory on the translocation across the outer envelope of chloroplast, whereas DGDG exhibits an inhibitory effect on TOC complex functionality.
Sponges are one of the major components of benthic communities and are considered to be a
key role organism in marine ecosystems. In addition to their importance in terms of
biodiversity, sponges are becoming increasingly attractive to the industry, as they themselves
or associated symbionts, produce various kinds of secondary metabolites of pharmaceutical
properties. Some of them have already been clinically applied.
The taxonomic characters of Porifera are limited to only a few morphological and
histological characters. In addition, sponges of the same species often show a wide
morphological variability, whereas the latter depends on different ecological parameters such
as water depth and current conditions. Thus, the taxonomic classification of sponges often
becomes a scientific challenge.
The fauna of the Yellow Sea rates among the least studied worldwide. At the same time,
according to the UN Atlas of the Ocean, the Yellow Sea is one of the most intensively
exploited marine areas in the world. This is not least due to the dense human population living
in the entire catchment area of the Yellow Sea region. In order to compile medium- and longterm
conclusions about the anthropogenic impact on biota of the Yellow Sea, the knowledge
of species and their distribution is of crucial importance, as these data form the baseline for all
future conservation efforts.
Until now the sponge fauna of the Chinese Yellow Sea is insufficiently investigated.
Thus, there is only one publication on sponges from this region that has been released
hitherto. This paper is dealing with only a view species. However, there is no reference
concerning the present location of the voucher material, on which this publication is based on.
Consequently, no scientific collection on Porifera from the Chinese part of the Yellow Sea
exists to date.
In order to compile a documentation of the recent sponge community of the Chinese
Yellow Sea, 12 study sites along the coast of the Liaoning Peninsula, China, Northeast
Yellow Sea, were investigated with focus on sponge distribution. The corresponding habitats
were characterized in regard to their topographical features, abiotic parameters, and common
composition of benthic megafaunal and macroalgal assemblages.
Due to the lack of comparable studies, a comprehensive literature research on sponges of the
shallow Northwest Pacific Ocean was required. As a result the first compilation of
publications is presented, dealing with sponges from shallow depths of the northwestern
Pacific Ocean.
Abstract
2
In the course of this study, 31 sponge species in total were recorded, which are scientifically
processed. With the exception of four all specimens were determined to species- level.
Twelve out of the total number of species are new to science and are described and classified
according to the recent taxonomic system of the phylum Porifera.
The results of this study indicate considerable differences in species composition between
investigated sites. It is shown that physical factors (particularly current regime, sedimentation,
seasonally related variations in temperatures), as well the availability of suitable substrates are
directly related to the diversity and abundance of investigated sponge communities. In this
context possible adaptation strategies of the corresponding sponges were discussed in detail.
Two sponge species, Clathria (Clathria) asodes and Antho (Acarnia) lithophoenix, formerly
known exclusively from the northeastern Pacific Ocean, are now recorded from the Northwest
Pacific Ocean for the first time. Furthermore, Penares hongdoensis, Clathria (Clathria)
hongdoensis and Celtodoryx girardae were synonymized with Penares cortius, Clathria
(Clathria) acanthostyli, and Celtodoryx ciocalyptoides respectively. Moreover, the occurrence
of eight sponge species, which were known from previous records from the Yellow Sea, could
be confirmed.
As a result of this study the Asian origin of a sponge species that is invasive to the French and
Dutch coasts of the Northeast Atlantic Ocean since the 1990s could be established. Moreover,
it is demonstrated that Celtodoryx girardae from the northeastern Atlantic is in fact
conspecific with Cornulum ciocalyptoides described by Burton (1935) from the Posiet Bay,
Sea of Japan. Apart from taxonomic remarks, variations between populations from both
oceans are examined and discussed thoroughly in regard to possible ecological implications.
The community of documented sponges shows overlapping with the one from the Sea of
Japan. According to the results it is assumed that the endemic degree of the sponges from the
Chinese Yellow Sea is rather low to moderate.
The material obtained in the course of this study was integrated in the collection of the
Senckenbergischen Naturforschenden Sammlungen. Therefore, it is the first scientific
collection of sponges from the Chinese Yellow Sea that can be consulted as a basis for all
further studies on sponges of this region.
The present study is the only investigation of sponges from Dalian and adjacent waters before
the spill occurred in the Dalian harbour in July 2010. Therefore, it provides an essential
baseline needed to assess the impact of the oil spill on benthic communities.
Strukturelle Organisation und Mobilisierung des Primaten-spezifischen Non-LTR-Retrotransposons SVA
(2011)
SVA-Elemente repraesentieren die juengste Familie der Non-LTR-Retrotransposons,
welche das humane Genom fortwaehrend modifizieren. SVA-Elemente zeichnen sich
durch ihre Organisation aus zusammengesetzten repetitiven Elementen aus. Um
Rueckschluesse auf den Assemblierungsprozess, der zur gegenwaertigen Organisation der
SVA-Elemente fuehrte, und ueber transkriptionelle Regulation dieser Elemente zu ziehen,
wurden Unterschiede in der Struktur der 116 SVA-Elemente, die auf humanem
Chromosom 19 lokalisiert sind, detailliert untersucht.
SVA-Elemente konnten in sieben unterschiedliche Strukturvarianten eingeteilt werden,
einschliesslich neuer Varianten wie SVA2, 3`-verkuerzte Elemente und Elemente mit 5`-
flankierenden Transduktionen. Ich habe auch eine extrem erfolgreiche human-spezifische
5`-Transduktionsgruppe identifiziert, SVA_F1, die trotz ihres jungen evolutionaeren Alters
ca. 32% aller Mitglieder der SVA-Subfamilie SVA_F umfasst. Die transkriptionelle
Kontrolle einer retrotransponierten und 5`-verkuerzten SVA_F-Kopie durch den Promotor
des MAST2-Gens diente als urspruengliches Source-Element dieser umfangreichen 5`-
Transduktionsgruppe, die mindestens 84 Elemente einschliesst. Die zusaetzlichen 5`-
sowie 3`-Transduktionsereignisse der vollstaendigen Alu-Sequenzen bei Mitgliedern der
SVA_F1-Transduktionsgruppe 4 weisen auf ihre wichtige Rolle in der erfolgreichen
Expansion im humanen Genom hin. Diese nachtraeglich erworbenen Alu-Sequenzen
machen SVA_F1-Familienmitglieder offensichtlich zum besseren Substrat fuer die Trans-
Mobilisierung durch die L1-Proteinmaschinerie. Die unterschiedlichen konsekutiven 5`-
Tansduktionsereignisse der SVA_F1-Familienmitglieder deuten auf transkriptionelle
Kontrolle ihrer Source-Elemente durch eine Vielzahl externer zellulaerer Promotoren hin,
die im Laufe der Evolution in Keimzellen aktiv waren. Ausserdem zeigt die Existenz von
5`-Transduktionen, dass SVA-Elemente sich die 5`-flankierenden Sequenzen aneignen
koennen. Die Daten zeigen auch, dass SVA-vermittelte 5-Tansduktionsereignisse
alternatives RNA-Spleissen an putativen Spleissstellen involvieren. Aus der EST-
Datenbankanalyse ist ersichtlich, dass Mitglieder der SVA_F1-Subfamilie auch
gegenwaertig transkribiert werden.
SVA-Elemente sind hoch aktiv im humanen Genom, aber der Mechanismus ihrer
Retrotransposition wurde bislang nicht aufgeklaert. Vorangehende Analysen genomischer
SVA-Kopien liessen auf eine L1-vermittelte Mobilisierung schliessen; allerdings wurde
der experimentelle Beweis dieser Hypothese bislang nicht geliefert. Mit Hilfe der
Zellkultur-basierten Trans-Mobilisierungsassays wurde in dieser Arbeit zum ersten Mal
experimentell bewiesen, dass SVA-Elemente tatsaechlich durch die L1-kodierten Proteine
in trans mobilisiert werden. Zu diesem Zweck wurden HeLa-Zellen mit einem
vollstaendigen oder mit einem 5`-verkuerzten SVA-Retrotranspositionsreporterkonstrukt
sowie mit einem L1-Expressionsplasmid bzw. Leervektor kotransfiziert und dann die
jeweiligen Raten der SVA-Retrotransposition anhand Neo-resistenter Kolonien, die
mindestens ein de novo-Retrotranspositionsereignis widerspiegeln, bestimmt. Die
Experimente zeigen, dass die Entstehung der Neo-resistenten Kolonien von der
Koexpression L1-kodierter Proteine abhaengig ist. Ich konnte auch zeigen, dass das
vollstaendige SVA-Testkonstrukt - im Gegensatz zum 5`-verkuerzten SVA-Konstrukt -
mit einer signifikant hoeheren Retrotranspositionsrate als die Kontrollkonstrukte, die zur
Generierung der prozessierten Pseudogenformation eingesetzt wurden, trans-mobilisiert
wird. Die Ergebnisse der Trans-Mobilisierungsassays belegen, dass SVA-Elemente ein
bevorzugtes Substrat fuer die L1-Proteinmaschinerie darstellen, und ihre 5`-Region
einschliesslich der Alu-homologen Sequenz fuer die hohe Retrotranspositionsrate essentiell
ist. Die elf analysierten SVA de novo-Integrationsereignisse weisen Merkmale der L1-
vermittelten Retrotransposition auf, wie Poly(A)-Enden, L1-EN-spezifische Konsensus-
Zielsequenz (NNAUNA), Zielsequenz-Verdoppelungen (TSDs), Mikrohomologien und
zusaetzliche Guanosin-Nukleotide am 5`-UEbergang.
Zusammenfassend demonstrieren die Ergebnisse dieser Studien, dass ein signifikanter Teil
der Mitglieder der human-spezifischen SVA-Subfamilie aus transkriptioneller Kontrolle
ihrer Source-Elemente durch externe Promotoren hervorgeht. Durch die in dieser Arbeit
durchgefuehrten in silico-Analysen wurde auch gezeigt, dass SVA-vermittelte 5`-
Transduktionsereignisse zur strukturellen Vielfalt der SVA-Elemente fuehren, und eine
neue Art von genomischen Umstrukturierungen darstellen, die zur Plastizitaet des
humanen Genoms beitragen. Ausserdem bestaetigen die Ergebnisse der Trans-
Mobilisierungsassays die Hypothese, dass SVA-Elemente tatsaechlich durch die L1-
kodierte Proteinmaschinerie trans-mobilisiert werden. Dabei sind Module am 5`-Ende der
SVA-Elemente fuer diesen Prozess hoechst relevant.
Die Ergebnisse der Dualen-Luciferase-Reportergen-Assays unterstuetzen die Hypothese,
dass innerhalb der SINE-R-Sequenz von SVA H19_27 cis-aktive Elemente vorhanden
sind, die auf aehnliche Weise wie die cis-aktiven Elemente innerhalb der 5`LTR von
HERV-K reguliert werden.
Ausserdem wurde in dieser Arbeit die Existenz interner reguatorischer Sequenzen
innerhalb der SVA-Sequenz bestaetigt. Mit Hilfe der Dualen-Luciferase-Reportergen-
Assays konnte zum ersten Mal gezeigt werden, dass SVA-Elemente cis-aktive Elemente
enthalten, die hauptsaechlich in der SINE-R-Region lokalisiert sind. Diese cis-aktiven
Elemente werden auf aehnliche Weise wie die cis-aktiven Elemente innerhalb der 5`LTR
von HERV-K reguliert. Die starke transkriptionelle Aktivitaet des vollstaendigen SVA-
Testelements und des L1RP-Promotors in den Teratokarzinom-Zelllinien bekraeftigen die
Annahme, dass haeufige SVA-Mobilisierung in Keimzellen durch die gleichzeitig
hochregulierte SVA- und L1-Transkription bedingt sein koennte.
Es konnte gezeigt werden, dass SVA-Elemente cis-aktive Elemente enthalten, die
hauptsaechlich in der SINE-R-Region lokalisiert sind, und auf aehnliche Weise wie die cis-
aktiven Elemente innerhalb der 5`LTR von HERV-K reguliert werden. Die starke
transkriptionelle Aktivitaet des vollstaendigen SVA-Testelements und des L1RP-Promotors
in Teratokarzinom-Zelllinien bestaetigen die Annahme, dass haeufige SVA-
Retrotransposition in Keimzellen durch die gleichzeitig hochregulierte SVA- und L1-
Transkription bedingt sein koennte.
PaCATB : a secreted catalase protecting Podospora anserina against exogenous oxidative stress
(2011)
A differential mass spectrometry analysis of secreted proteins from juvenile and senescentPodospora anserina cultures revealed age-related differences in protein profiles. Among other proteins with decreased abundance in the secretome of senescent cultures a catalase, termed PaCATB, was identified. Genetic modulation of the abundance of PaCATB identified differential effects on the phenotype of the corresponding strains. Deletion of PaCatB resulted in decreased resistance, over-expression in increased resistance against hydrogen peroxide. While the lifespan of the genetically modified strains was found to be unaffected under standard growth conditions, increased exogenous hydrogen peroxide stress in the growth medium markedly reduced the lifespan of the PaCatB deletion strain but extended the lifespan of PaCatB over-expressors. Overall our data identify a component of the secretome of P. anserina as a new effective factor to cope with environmental stress, stress that under natural conditions is constantly applied on organisms and influences aging processes.
A decade since the availability of Mycobacterium tuberculosis (Mtb) genome sequence, no promising drug has seen the light of the day. This not only indicates the challenges in discovering new drugs but also suggests a gap in our current understanding of Mtb biology. We attempt to bridge this gap by carrying out extensive re-annotation and constructing a systems level protein interaction map of Mtb with an objective of finding novel drug target candidates. Towards this, we synergized crowd sourcing and social networking methods through an initiative ‘Connect to Decode’ (C2D) to generate the first and largest manually curated interactome of Mtb termed ‘interactome pathway’ (IPW), encompassing a total of 1434 proteins connected through 2575 functional relationships. Interactions leading to gene regulation, signal transduction, metabolism, structural complex formation have been catalogued. In the process, we have functionally annotated 87% of the Mtb genome in context of gene products. We further combine IPW with STRING based network to report central proteins, which may be assessed as potential drug targets for development of drugs with least possible side effects. The fact that five of the 17 predicted drug targets are already experimentally validated either genetically or biochemically lends credence to our unique approach.
We describe and analyze a Neandertal postcranial skeleton and dentition, which together show unambiguous signs of right-handedness. Asymmetries between the left and right upper arm in Regourdou 1 were identified nearly 20 years ago, then confirmed by more detailed analyses of the inner bone structure for the clavicle, humerus, radius and ulna. The total pattern of all bones in the shoulder and arm reveals that Regourdou 1 was a right-hander. Confirmatory evidence comes from the mandibular incisors, which display a distinct pattern of right oblique scratches, typical of right-handed manipulations performed at the front of the mouth. Regourdou's right handedness is consistent with the strong pattern of manual lateralization in Neandertals and further confirms a modern pattern of left brain dominance, presumably signally linguistic competence. These observations along with cultural, genetic and morphological evidence indicate language competence in Neandertals and their European precursors.
Background: Cyanobacteria possess several cytochrome P450s, but very little is known about their catalytic functions. CYP110 genes unique to cyanaobacteria are widely distributed in heterocyst-forming cyanobacteria including nitrogen-fixing genera Nostoc and Anabaena. We screened the biocatalytic functions of all P450s from three cyanobacterial strains of genus Nostoc or Anabaena using a series of small molecules that contain flavonoids, sesquiterpenes, low-molecular-weight drugs, and other aromatic compounds.
Results: Escherichia coli cells carrying each P450 gene that was inserted into the pRED vector, containing the RhFRed reductase domain sequence from Rhodococcus sp. NCIMB 9784 P450RhF (CYP116B2), were co-cultured with substrates and products were identified when bioconversion reactions proceeded. Consequently, CYP110E1 of Nostoc sp. strain PCC 7120, located in close proximity to the first branch point in the phylogenetic tree of the CYP110 family, was found to be promiscuous for the substrate range mediating the biotransformation of various small molecules. Naringenin and (hydroxyl) flavanones were respectively converted to apigenin and (hydroxyl) flavones, by functioning as a flavone synthase. Such an activity is reported for the first time in prokaryotic P450s. Additionally, CYP110E1 biotransformed the notable sesquiterpene zerumbone, anti-inflammatory drugs ibuprofen and flurbiprofen (methylester forms), and some aryl compounds such as 1-methoxy and 1-ethoxy naphthalene to produce hydroxylated compounds that are difficult to synthesize chemically, including novel compounds.
Conclusion: We elucidated that the CYP110E1 gene, C-terminally fused to the P450RhF RhFRed reductase domain sequence, is functionally expressed in E. coli to synthesize a robust monooxygenase, which shows promiscuous substrate specificity (affinity) for various small molecules, allowing the biosynthesis of not only flavones (from flavanones) but also a variety of hydroxyl-small molecules that may span pharmaceutical and nutraceutical industries.
The biosynthesis pathway to diadinoxanthin and fucoxanthin was elucidated in Phaeodactylum tricornutum by a combined approach involving metabolite analysis identification of gene function. For the initial steps leading to β-carotene, putative genes were selected from the genomic database and the function of several of them identified by genetic pathway complementation in Escherichia coli. They included genes encoding a phytoene synthase, a phytoene desaturase, a ζ-carotene desaturase, and a lycopene β-cyclase. Intermediates of the pathway beyond β-carotene, present in trace amounts, were separated by TLC and identified as violaxanthin and neoxanthin in the enriched fraction. Neoxanthin is a branching point for the synthesis of both diadinoxanthin and fucoxanthin and the mechanisms for their formation were proposed. A single isomerization of one of the allenic double bounds in neoxanthin yields diadinoxanhin. Two reactions, hydroxylation at C8 in combination with a keto-enol tautomerization and acetylation of the 3′-HO group results in the formation of fucoxanthin.
Background: Hydrolysates of plant biomass used for the production of lignocellulosic biofuels typically contain sugar mixtures consisting mainly of D-glucose and D-xylose, and minor amounts of L-arabinose. The yeast Saccharomyces cerevisiae is the preferred microorganism for the fermentative production of ethanol but is not able to ferment pentose sugars. Although D-xylose and L-arabinose fermenting S. cerevisiae strains have been constructed recently, pentose uptake is still a limiting step in mixed sugar fermentations.
Results: Here we described the cloning and characterization of two sugar transporters, AraT from the yeast Scheffersomyces stipitis and Stp2 from the plant Arabidopsis thaliana, which mediate the uptake of L-arabinose but not of D-glucose into S. cerevisiae cells. A yeast strain lacking all of its endogenous hexose transporter genes and expressing a bacterial L-arabinose utilization pathway could no longer take up and grow with L-arabinose as the only carbon source. Expression of the heterologous transporters supported uptake and utilization of L-arabinose especially at low L-arabinose concentrations but did not, or only very weakly, support D-glucose uptake and utilization. In contrast, the S. cerevisiae D-galactose transporter, Gal2, mediated uptake of both L-arabinose and D-glucose, especially at high concentrations.
Conclusions: Using a newly developed screening system we have identified two heterologous sugar transporters from a yeast and a plant which can support uptake and utilization of L-arabinose in L-arabinose fermenting S. cerevisiae cells, especially at low L-arabinose concentrations.
Amino acids can induce yeast cell adhesion but how amino acids are sensed and signal the modulation of the FLO adhesion genes is not clear. We discovered that the budding yeast Saccharomyces cerevisiae CEN.PK evolved invasive growth ability under prolonged nitrogen limitation. Such invasive mutants were used to identify amino acid transporters as regulators of FLO11 and invasive growth. One invasive mutant had elevated levels of FLO11 mRNA and a Q320STOP mutation in the SFL1 gene that encodes a protein kinase A pathway regulated repressor of FLO11. Glutamine-transporter genes DIP5 and GNP1 were essential for FLO11 expression, invasive growth and biofilm formation in this mutant. Invasive growth relied on known regulators of FLO11 and the Ssy1-Ptr3-Ssy5 complex that controls DIP5 and GNP1, suggesting that Dip5 and Gnp1 operates downstream of the Ssy1-Ptr3-Ssy5 complex for regulation of FLO11 expression in a protein kinase A dependent manner. The role of Dip5 and Gnp1 appears to be conserved in the S. cerevisiae strain ∑1278b since the dip5 gnp1 ∑1278b mutant showed no invasive phenotype.
Secondly, the amino acid transporter gene GAP1 was found to influence invasive growth through FLO11 as well as other FLO genes. Cells carrying a dominant loss-of-function PTR3647::CWNKNPLSSIN allele had increased transcription of the adhesion genes FLO1, 5, 9, 10, 11 and the amino acid transporter gene GAP1. Deletion of GAP1 caused loss of FLO11 expression and invasive growth. However, deletions of FLO11 and genes encoding components of the mitogen-activated protein kinase pathway or the protein kinase A pathway were not sufficient to abolish invasive growth, suggesting involvement of other FLO genes and alternative pathways. Increased intracellular amino acid pools in the PTR3647::CWNKNPLSSIN-containing strain opens the possibility that Gap1 regulates the FLO genes through alteration of the amino acid pool sizes.
NOSTRIN belongs to the recently defined F-BAR protein family. F-BAR proteins are
multi-domain proteins, which serve as adaptors between plasma membrane and
cytoskeleton components in processes such as membrane protrusion formation,
endocytosis and migration. NOSTRIN encompasses a F-BAR domain at the N-terminus,
which mediates membrane association, followed by a HR1 motif and an intermediate
domain (ID) domain in the middle, and a SH3 domain at the C-terminus. The domain
architecture and ability to form oligomers enable NOSTRIN to coordinate several
interaction partners namely dynamin, caveolin, N-WASP and endothelial nitric oxide
synthase (eNOS) in the process of eNOS trafficking. In this context NOSTRIN was
originally identified and hence termed eNOS traffick inducer. NOSTRIN is expressed in
vascularized tissues (e.g. liver and lung) and in primary endothelial cells.
Aims of the present work were (1) to investigate if NOSTRIN is involved in other
processes besides eNOS trafficking, (2) to analyse the function of NOSTRIN in vivo
through knockdown of NOSTRIN in developing zebrafish and (3) to study the
consequences of the loss of NOSTRIN on signal transduction in a primary cell culture
model derived from NOSTRIN knockout mice.
To study the possible involvement of NOSTRIN in other processes besides eNOS
trafficking a yeast two-hybrid screen was performed in which fibroblast growth factor
receptor 1 (FGFR1) was identified as a putative novel interaction partner of NOSTRIN. In
a series of yeast two-hybrid, pulldown and co-immunoprecipitation experiments the
interaction between NOSTRIN and FGFR1 was confirmed to occur between
endogenously expressed proteins and determined to be direct and to depend on the ID
domain of NOSTRIN and the 130 C-terminal amino acid residues of FGFR1. FGFR1 is
activated by binding of fibroblast growth factors (FGFs) and induces several different
signal transduction pathways (e.g. MAPK and Akt pathway). Overexpression of
NOSTRIN in HeLa cells specifically enhanced FGF2-dependent MAPK activation.
Accordingly, depletion of NOSTRIN attenuated FGF2-dependent MAPK activation and
did not affect FGF2-induced Akt activation.
In summary, NOSTRIN has been identified as a novel interaction partner of FGFR1
involved in FGF2-dependent signal transduction.
The morpholino oligonucleotide-mediated knockdown of NOSTRIN in developing
zebrafish caused vascular leakage and irregular vascular patterning e.g. a loss of the
proper trajectory of intersegmental vessel and interruptions of the dorsal longitudinal
anastomotic vessel. The vascular phenotype was consistent upon use of two different
morpholinos and could be rescued in a dose dependent manner by the injection of
zebrafish NOSTRIN mRNA. Detailed analysis involving confocal and time lapse
microscopy in zebrafish with endothelial specific expression of EGFP revealed that the
knockdown of NOSTRIN impacts in vivo on the migration and morphology of endothelial
tip cells and leads to a reduction of filopodia number and length.
Additionally a NOSTRIN knockout mouse was generated. The analysis of FGFR1 signal
transduction in primary mouse lung endothelial cells (MLECs) from NOSTRIN knockout
and wild type mice revealed that FGF2-dependent MAPK activation was attenuated in
MLECs isolated from NOSTRIN knockout mice when compared to MLECs isolated from
wild type mice. The effect of NOSTRIN on FGF2-dependent signal transduction seems to
be specific, since VEGF-induced MAPK activation was not affected in NOSTRIN
knockout MLECs. The importance of NOSTRIN for FGF2 signal transduction in vivo is
demonstrated by the greatly impaired angiogenic response to FGF2 in NOSTRIN
knockout mice in matrigel plug assay. In a detailed biochemical analysis it was
discovered that NOSTRIN interacts with the activated small GTPase Rac1 and that
overexpression of NOSTRIN enhances Rac1 activation. Furthermore, the interactions of
NOSTRIN with both Rac1 and its GEF Sos1 are required for NOSTRIN-mediated
activation of Rac1. In accordance, activation of Rac1 was not detected upon FGF2
stimulation in NOSTRIN knockout MLECs.
In conclusion, the present work describes a novel function of the F-BAR protein
NOSTRIN in FGFR1 signal transduction. Data presented in this work demonstrate that
NOSTRIN is required for the assembly of a complex consisting of FGFR1, Sos1 and
Rac1 and subsequently for the FGF2-dependent activation of Rac1 in endothelial cells.
Die Makrophytenvegetation eines stillgelegten Kanalabschnittes ("Alte Fahrt") bei Senden in Westfalen hat sich seit Beginn der 90er Jahre drastisch verändert. Aus einem typischen Potamogetonetum lucentis sind Reinbestände von Myriophyllum spicatum geworden, denen stellenweise Ceratophyllum demersum beigemischt ist. Die Ursachen für diese gravierenden Vegetationsveränderungen sind nicht klar. Da es sich um einen der bedeutendsten westfälischen Standorte des Potamogetonetum lucentis, einer in Nordrhein-Westfalen stark gefährdeten Pflanzengesellschaft, handelte, sind weiterführende Untersuchungen und Versuche zur Wiederansiedlung zu fordern.
Mitochondrial dynamics and mitophagy play a key role in ensuring mitochondrial quality control. Impairment thereof was proposed to be causative to neurodegenerative diseases, diabetes, and cancer. Accumulation of mitochondrial dysfunction was further linked to aging. Here we applied a probabilistic modeling approach integrating our current knowledge on mitochondrial biology allowing us to simulate mitochondrial function and quality control during aging in silico. We demonstrate that cycles of fusion and fission and mitophagy indeed are essential for ensuring a high average quality of mitochondria, even under conditions in which random molecular damage is present. Prompted by earlier observations that mitochondrial fission itself can cause a partial drop in mitochondrial membrane potential, we tested the consequences of mitochondrial dynamics being harmful on its own. Next to directly impairing mitochondrial function, pre-existing molecular damage may be propagated and enhanced across the mitochondrial population by content mixing. In this situation, such an infection-like phenomenon impairs mitochondrial quality control progressively. However, when imposing an age-dependent deceleration of cycles of fusion and fission, we observe a delay in the loss of average quality of mitochondria. This provides a rational why fusion and fission rates are reduced during aging and why loss of a mitochondrial fission factor can extend life span in fungi. We propose the ‘mitochondrial infectious damage adaptation’ (MIDA) model according to which a deceleration of fusion–fission cycles reflects a systemic adaptation increasing life span.
The long sought molecular function of membrane raft-associated flotillin proteins is slowly becoming resolved, partially owing to the increasing knowledge about their interaction partners. Being ubiquitously expressed and evolutionarily highly conserved, flotillins carry out important cellular functions, one of which is the regulation of signal transduction pathways. This study shows that the signaling adaptor protein fibroblast growth factor receptor substrate 2 (FRS2) directly interacts both in vivo and in vitro with flotillin-1 (flot-1). FRS2 is an important docking protein of many receptor tyrosine kinases. It regulates downstream signaling by forming molecular complexes with other adaptor proteins and tyrosine phosphatases, and seems to be a critical mediator of sustained extracellular signal regulated kinase (ERK) activity. Flot-1 has also been implicated in the regulation of ERK activity upon EGF and FGF stimuli. Furthermore, flot-1 forms signalosomes with EGFR and the downstream components of the MAP kinase pathway. The newly discovered interaction between FRS2 and flot-1 was shown to be mediated by the phosphotyrosine binding (PTB) domain and, to a lesser extent, the C-terminus (CT) of FRS2 and by the C-terminus of flot-1. Flot-1 coprecipitated together with FRS2 from murine tissues and cell lysates, demonstrating that this interaction also takes place in vivo. Interestingly, flot-2, which shows a high homology to flot-1 and forms stable oligomeric complexes with it, does not appear to directly interact with FRS2. Novel insights into the functional role of the interaction between flot-1 and FRS2 were provided by the results showing that depletion of flot-1 affects the cellular localization of FRS2. In hepatocytes stably depleted of flot-1, FRS2 appeared to be more soluble. Furthermore, upon pervanadate stimulation of the cells, a small fraction of FRS2 was recruited into detergent resistant membranes, but the recruitment did not take place in the absence of flot-1. Triggered by the same stimulus, a fraction of FRS2 was translocated to the nucleus independently of flot-1. Overexpression of FRS2 has previously been shown to result in increased ERK activation. However, in cells depleted of flot-1, FRS2 was not able to compensate for the compromised ERK activation after EGF or FGF stimulation. This might imply that FRS2 and flot-1 are functionally interconnected and that FRS2 resides upstream of flot-1. Taken together, the results presented here indicate that this complex may be involved in the control of signaling downstream of receptor tyrosine kinases and is important for ensuring a proper signaling response. In the absence of flot-1, increased Tyr phosphorylation of FRS2 was observed. It is known that Tyr and Thr phosphorylation of FRS2 are reciprocally regulated. Since ERK is a known executor of the FRS2 Thr phosphorylation, and ERK activity was shown to be severely diminished upon flot-1 depletion, the increased Tyr phosphorylation of FRS2 was in agreement with this and might be a direct consequence of a decreased ERK activity upon flot-1 depletion. FRS2 owes its name to the major and the first described function of this protein as a substrate for FGFR. PTB domain of FRS2 was published to constitutively bind the juxtamembrane domain of FGFR. In this study, the PTB domain was mapped to be involved in the constitutive interaction with flot-1 and the competition was shown to exist between flot-1 and FGFR1 for binding to FRS2. Another novel interaction partner of FRS2 was discovered in the present study. Cbl-associated protein (CAP) is an adaptor protein with three SH3 domains and it plays a role during insulin signaling by recruiting the signaling complex to lipid rafts. CAP was previously shown to interact with flot-1 via the SoHo domain, and this interaction was found to be crucial for the lipid raft recruitment of other signaling components. Both the PTB domain and CT of FRS2 were found to mediate the interaction with CAP, whereas in CAP, the SoHo domain, together with the third SH3 domain, seems to bind to FRS2. SH3 domains mediate the assembly of specific protein complexes by binding to proline rich sequences, several of which are present in FRS2. Due to overlapping interaction domains, FRS2 and flot-1 competed for the binding to CAP. However, the interaction with neither CAP nor flot-1 was necessary for the observed nuclear translocation of FRS2. Since CAP is expressed as several tissue- and developmental stage-specific isoforms, a further aim of this study was to analyze the expression of its isoforms in mouse embryonic fibroblasts (MEFs). Many new isoforms were discovered here which have not been described in the literature so far. They all contain the SoHo domain and three SH3 domains, but differ among themselves by the presence and length of a proline-rich region that preceeds the SoHo domain and by a novel 20-amino acid (AA) stretch between the second and the third SH3 domain. The length of the proline-rich region turned out to be an important factor determining the strength of the interaction with FRS2. The interaction was found to be weakened by the increasing length of this region. The new isoforms possessing the 20-AA stretch are specifically expressed in murine muscular tissues, with the highest level in the heart. During adipogenesis, we observed a shift in the abundance of the isoforms, in that only the isoforms without the insertion were shown to be upregulated on mRNA level. However, during myogenesis, preferentially expressed isoforms were those with the insertion. The collected data implicate that isoforms with the 20-AA insertion might be more ubiquitous in nondifferentiated/embryonic cells and that the observed "isoform-switch" might be dependent on the cell fate and differentiation state.
Die nicht-konventionelle Hefe P. ciferrii produziert große Mengen der tetra-acetylierten Sphingoidbase Phytosphingosin (TAPS). Sphingoidbasen sind essentielle Komponenten des stratum corneums, der multilamellaren Barriere der menschlichen Haut, und daher in der Kosmetik-Industrie von großem Interesse. Im Rahmen dieser Arbeit sollte die biotechnologische Produktion der Sphingoidbasen Phytosphingosin, Sphinganin und Sphingosin auf molekularbiologischer Ebene in P. ciferrii charakterisiert und optimiert werden. Die Hefe P. ciferrii konnte durch Etablierung einer einfachen und hoch-effizienten Transformations-Methode auf genetischer Ebene leicht zugänglich gemacht werden. Durch Inaktivierung des für NHEJ essentiellen PcLIG4 Gens konnte die Effizienz zielgerichteter genomischer Integrationen von transformierten DNA-Konstrukten von 1 % auf 87 % erhöht werden. Die Etablierung des Cre-loxP Systems erlaubte das mehrfache Verwenden eines Selektions-Markers wodurch sukzessiv mehrere genomische Integrationen in einem Stamm ermöglicht wurden. Durch diese Errungenschaften konnte das Ziel „Optimierung der Sphingoidbasen-Produktion der nicht-konventionellen Hefe P. ciferrii“ im Folgenden erfolgreich verfolgt werden. Der initiale Schritt der Sphingoidbasen-Biosynthese ist die von der Serin-Palmitoyl-Transferase katalysierte Kondensation von L-Serin und Palmitoyl-CoA. Durch die Deletion von Genen, die am L-Serin-Katabolismus von P. ciferrii beteiligt sind (PcSHM1, PcSHM2und PcCHA1), konnte die de novo Sphingoidbasen-Biosynthese optimiert werden und führte in einem lig4? Stamm zu einer etwa dreifachen Erhöhung der TAPS-Produktion. Weitere Ansätze den (vermutlich durch L-Serin feed back regulierten) L-Serin-Biosyntheseweg bzw. die in vivo L-Serin-Verfügbarkeit zu optimieren, führten nicht zu einer gesteigerten TAPS-Produktion. Durch weitere Deletion und Überexpression von Genen des Sphingolipid-Stoffwechsels konnte die TAPS-Produktion jedoch um ein Vielfaches verbessert werden. So konnte ein Stamm konstruiert werden, der die Gene PcLCB1, PcLCB2 und PcSYR2 überexprimiert und Deletionen der Gene PcSHM1, PcSHM2, PcCHA1, PcLCB4 und PcORM12 trägt. Dieser Stamm (CSS.L4.O.L2.L1.S2) wies eine mehr als fünffach erhöhte maximale spezifische TAPS-Produktbildungsrate (q Pmax ) auf und produzierte mit 2 g * L rund siebenmal mehr TAPS als der lig4? Ausgangsstamm, weshalb ein Einsatz dieses Stammes für die industrielle TAPS-Produktion denkbar wäre. Ausgehend von einem für die TAPS- (und somit Sphingoidbasen-) Produktion optimierten Stamm sollten Stämme mit optimierter TriASa- oder TriASo-Produktion für industrielle Zwecke generiert werden. Es stellte sich allerding heraus, dass erhöhte Mengen dieser Sphingoidbasen wahrscheinlich wachstumshemmend für P. ciferrii sind, weshalb eine weitere Produktions-Optimierung nicht ohne Weiteres möglich ist. In einem Laborstamm gelang es jedoch, durch Konstruktion und anschließende Transformation eines optimierten integrativen Plasmids (trägt die Gene, die für die Produktion von Sphingosin bzw. TriASo nötig sind) eine TriASo-Produktion von bis zu 30 mg * g (BTM) zu erzielen, wobei gleichzeitig die Bildung des Nebenprodukts TriASa auf weniger als 4 mg * g (BTM)reduziert wurde. Weiterhin konnte durch Deletion von PcSCS7 in einem TriASo-Produktionsstamm die TriASa-Produktion mehr als vierfach reduziert werden. Die Bildung eines weiteren von P. ciferrii gebildeten Nebenproduktes [Tri-Acetyl-Sphingadienin (TriASd)] konnte durch Deletion des PcSLD1 Gens unterbunden werden. Nach Inaktivierung von PcSCH9 konnte eine fast 20 %ige Verbesserung der TriASo-Produktion erreicht werden. Es konnten zwei putative Acetyl-Transferasen identifiziert werden (PcAft2 und PcSli1), die an der Acetylierung von Phytosphingosin (zu TAPS), Sphinganin (zu TriASa) und Sphingosin (zu TriASo) beteiligt sind. Die Aufklärung und Optimierung dieser von PcAtf2 und PcSli1 katalysierten Schritte sind vielversprechende Ansatzpunkte die Sphingoidbasen-Produktion in P. ciferrii weiter zu optimieren.
The synthesis of the recently characterized depsipeptide szentiamide (1), which is produced by the entomopathogenic bacterium Xenorhabdus szentirmaii, is described. Whereas no biological activity was previously identified for 1, the material derived from the efficient synthesis enabled additional bioactivity tests leading to the identification of a notable activity against insect cells and Plasmodium falciparum, the causative agent of malaria.
Im Zuge des hessischen Wiederansiedlungsprojektes für die Europäische Sumpfschildkröte (Emys orbicularis) konnten in den Jahren 2002-2007 insgesamt 79 juvenile Sumpfschildkröten an vier Standorten (NSG „Hölle von Rockenberg“, NSG „Reinheimer Teich“, NSG „Nachtweid von Dauernheim“ und NSG „Nidderauen von Stockheim“) in Hessen ausgewildert werden. Ziel der vorliegenden Untersuchung war es, hinreichende Kenntnisse zur Biologie, Physiologie und Ökologie der ausgesetzten Jungtiere zu erhalten. Die generellen Erfolgsaussichten eines solchen Langzeitprojektes, das Verhalten der ausgesetzten Jungtiere und deren Gesundheitszustand standen hierbei im Vordergrund der Arbeit. Anhand verschiedener Methoden (direkte Beobachtung, Radiotelemetrie, Fang-Wiederfang) wurde die Ansiedlung über einen Zeitraum von fünf Jahren überwacht. Radiotelemetrische Studien sowie eine direkte Beobachtung erbrachten hierbei Informationen zur Raum- und Habitatnutzung der Jungtiere und den daraus resultierenden Lebensraumansprüchen. Durch dieses Wissen konnten weitere, sowie bereits bestehende, Wiederansiedlungsgebiete in dieser Region durch individuelle Maßnahmen optimiert werden. Des Weiteren konnte mit temperatursensitiven Messmethoden ein Überblick über das tägliche und saisonale Körpertemperaturspektrum der Art in Hessen ermittelt werden. Vor der Wiederansiedlung sowie im weiteren Verlauf der Untersuchung wurden in den jeweiligen Gebieten diverse Biotopsmaßnahmen durchgeführt. So z.B. das Ausbringen von zusätzlichen Sonnenmöglichkeiten in Form von Stämmen, das Anlegen von permanenten und temporären Flachwasserteichen, verschiedenste Biotopspflegemaßnahmen (Entschlammen, Entbuschen) und die Offenhaltung potentieller Eiablageplätze. Diese Maßnahmen zeigten im Laufe der Untersuchung nicht nur einen positiven Effekt für die Zielart Emys orbicularis, sondern auch für weitere, bestandsbedrohte Begleitarten (z.B. die Wechselkröte Bufo viridis). Die ausgesetzten Jungtiere hatten ein mittleres Alter von 3,44 ± 1,29 Jahren (2-6 Jahre) bei einer mittlere Masse von 197,1 ± 110,2 g (66-619 g) und einer mittleren Carapaxlänge von 9,91 ± 1,77 cm (6,71-14,87 cm). Alle Tiere wurden vor dem Aussetzen durch einen Mikrotransponder und eine individuelle Farbmarkierung auf dem Panzer gekennzeichnet.
Mit Hilfe der Radiotelemetrie wurden die Aufenthaltsbereiche sowie das Wanderverhalten der Sumpfschildkröten in den Gebieten NSG „Hölle von Rockenberg“, NSG „Reinheimer Teich“ und NSG „Nachtweid von Dauernheim“ dokumentiert. Zusätzlich zu den herkömmlichen Radiotelemetriesendern konnten temperatursensitive Radiotelemetriesender verwendet werden, die sowohl über den Standort des Tieres als auch seine momentane Körpertemperatur Auskunft gaben. Es wurden hierbei insgesamt 34 Telemetriesender (9 ohne, 25 mit Temperaturfunktion) für eine Besenderung von 27 Individuen verwendet. Das entspricht einer Besenderungsquote von 42,3 %. Die durchschnittliche Masse der Sumpfschildkröten bei der Erstbesenderung betrug 238,6 ± 68,2 g bei einer Carapaxlänge von 10,80 ± 1,07 cm. Um einen Überblick über das Körpertemperaturspektrum der Art in Hessen zu erhalten, wurden temperatursensitive Radiotelemetriesender und ergänzend Temperaturdatenlogger (iButtons®) verwendet. Es zeigten sich sowohl individuelle als auch stark saisonal geprägte Temperaturmuster. Erwartungsgemäß konnten die höchsten Körpertemperaturen im Sommer (bis zu 44 °C) und die niedrigsten im Winter (bis zu -0,8 °C) dokumentiert werden. Der bevorzugte Temperaturbereich von Emys orbicularis wird aufgrund der vorliegenden Daten bei 25-32 °C vermutet. Die Aktivitätsperiode von Emys orbicularis in Hessen lässt sich von Mitte/Ende März bis Mitte Oktober, mit einem Aktivitätsmaximum in den Monaten Mai und Juni, angeben. Eine Erhöhung bzw. Erniedrigung der Körpertemperatur wurde durch Verhaltensweisen, wie Sonnenbaden oder das Aufsuchen von Wasser, erreicht. Sonnenbadende Sumpfschildkröten konnten in der Zeit von 07:15 bis 19:45 Uhr direkt beobachtet werden, die Hauptsonnenaktivität lag zwischen 09:00-15:00 Uhr. Hierbei konnte eine Tagesrhythmik des Sonnenbadens dokumentiert werden, die im Normalfall einen einphasigen Verlauf hatte. Die Schildkröten erschienen im Laufe des Vormittags auf dem Sonnenplatz und verblieben dort, unterbrochen von kurzzeitigem Aufsuchen des Wassers, bis in den Nachmittag hinein. Die bevorzugten Aufenthaltsbereiche und Strukturen unterlagen sowohl saisonalen als auch individuellen Präferenzen. Die Tiere nutzten zu 69,9 % Baumstämme als Sonnenplatz. Es wurden sowohl größere als auch kleinere Gewässer als Aufenthaltsbereich genutzt. Charakteristisch waren hier vor allem ausgedehnte Unterwasser- und Schwimmblatt-Gesellschaften in den Randbereichen, wie z.B. die „Untergetauchte Laichkrautgesellschaft“.
Die Störanfälligkeit der beobachteten Sumpfschildkröten war sehr stark individuell ausgeprägt. Es konnte aber auch beobachtet werden, dass Tiere, die gerade das Wasser verließen, und noch nicht getrocknet waren, schneller auf eine Störung reagierten, als Tiere, die schon vollständig getrocknet waren. Es ist anzunehmen, dass dieses Verhalten mit der Thermoregulation der Tiere in Zusammenhang steht. Die besenderten Tiere verblieben in den Aussetzgebieten und es konnten nur geringe Wanderbewegungen (bis max. 250 m) notiert werden. Der hierbei ermittelte Aktionsraum („home range“) variierte sowohl individuell als auch in den einzelnen Gebieten. So konnte in dem kleineren Gebiet „Hölle von Rockenberg“ (13 ha) eine zehnmal geringere Aktionsraumgröße notiert werden als in dem weitaus größeren Gebiet „Reinheimer Teich“ (75 ha). Sie betrug in Rockenberg 0,21 ± 0,03 ha (0,19 bis 0,32 ha) und in Reinheim 2,00 ± 1,58 ha (0,24 ha bis 4,71 ha). In der Phase der Überwinterung konnte keinerlei Mortalität dokumentiert werden. Als Überwinterungsplatz nutzten die Tiere in der Regel schilfbewachsene Uferbereiche mit einer Wassertiefe von 50 cm. Im Gebiet „Hölle von Rockenberg“ konnten einige Tiere mehrmalig in der Überwinterung beobachtet werden und es zeigten sich hierbei individuelle Standortpräferenzen. Die Überwinterungsplätze wurden zu 50 % wiederholt aufgesucht. In den Wintermonaten Dezember-Februar betrug die mittlere Körpertemperatur 3,09 ± 1,59 °C. Die verwendeten Fangmethoden (Sonnenfalle, Reusenfalle, Handfang) konnten nur im Gebiet „Hölle von Rockenberg“ erfolgreich eingesetzt werden. Im Gebiet „Reinheimer Teich“ konnte nur einmalig eine Schildkröte wiedergefangen werden. Die wiederangesiedelten Tiere nahmen sowohl an Masse als auch an Größe zu. Die durchschnittliche Massenzunahme betrug im Gebiet „Hölle von Rockenberg“ 40,33 ± 7,20 g (29,38-48,40 g) bei einem Wachstum des Carapax von 0,61 ± 0,08 cm (0,52-0,75 cm). Es konnten keinerlei Krankheiten oder Verhaltensauffälligkeiten dokumentiert werden. Im gesamten Untersuchungszeitraum wurde nur einmalig der Verlust eines Tieres detektiert.
Diese Massen- und Größenzunahmen sowie die Überlebensrate sprechen für die verwendeten Aufzuchtsmethoden und die ausgewählten Wiederansiedlungsgebiete. Es zeigt, dass sich die Methode des „headstarting“ bei Emys orbicularis sehr gut eignet und kann somit für solche Wiederansiedlungsprojekte durchaus empfohlen werden. Eine Stützung der Bestände durch das Auswildern „headstarted“ Emys orbicularis (aufgezogenen unter den hier vorgestellten Bedingungen) wird daher für weitere Projekte empfohlen Basierend auf den Ergebnissen der vorliegenden Arbeit lassen sich die Lebensraumansprüche der Art in Hessen benennen. Ausgehend von diesen speziellen Ansprüchen lässt sich ein optimales Emys orbicularis Habitat (für nördliche Vertreter der Art) definieren.
Zusammenfassende Grundlagen eines idealen Emys orbicularis Habitats:
- begleitendes (natürliches) Fließgewässer
- ausreichend Kleingewässer, auch als Trittsteine zum Fließgewässer
- mind. ein großes Hauptgewässer (mind. 2000 m2) mit einer Tiefe von mind. 1,50 m
- flach abfallendes Gewässerprofil mit sich schnell erwärmenden Flachwasserzonen
- ausreichend Wasser-/Unterwasservegetation
- ausreichend, ganztägig besonnte Sonnenplätze in Form von ins Wasser ragenden Stämmen und Ästen
- breiter, südexponierter Schilfgürtel zur Überwinterung
- geringer Fischbesatz zur Sicherung der Nahrungsgrundlage (Konkurrenz)
- möglichst keine fremdländischen Schildkröten (Konkurrenz)
- südexponierte, xerotherme offene Hanglage mit Magerrasencharakter zur Eiablage (im Bedarfsfall sichergestellt durch Beweidung und/oder Mahd) - keinerlei oder nur eingeschränkte freizeitliche Nutzung in Randbereichen - keine Zerschneidung der Gewässer und Wanderwege durch Straßen.
Die vorliegende Arbeit bestätigt den bisher getätigten Bemühungen zum Schutz der Europäischen Sumpfschildkröte gute Erfolgsaussichten für eine weitere Etablierung der Art in Hessen. Da die untersuchten Tiere noch nicht geschlechtsreif waren und somit noch keine Reproduktion im Freiland dokumentiert werden konnte, lässt sich der langfristige Erfolg noch nicht abschließend beurteilen. Aufgrund der bisher getätigten Untersuchungen lässt sich ein Reproduktionserfolg aber in den nächsten Jahren vermuten. Ein wichtiger Schritt zum Schutz der Europäischen Sumpfschildkröte in Hessen ist mit dem hier vorgestellten Projekt und den verwendeten Aufzuchts- und Wiederansiedlungsmethoden getan.
Many hominin species are best physically represented and understood by the sum of their dental morphologies. Generally, taxonomic affinities and evolutionary trends in development (ontogeny) and morphology (phylogeny) can be deduced from dental analyses. More specifically, the study of dental remains can yield a wealth of information on many facets of hominin evolution, life history, physiology and ecological adaptation; in short, the organisms paleobiomics. Functionally, teeth present information about dietary preferences, that is, the dietary niche in ecological context and, in turn, masticatory function. As the amount and types of information that can be gleaned from 2-dimensional tooth measurement exhaust themselves, 3-dimensional microscopic modeling and analysis presents a largely fertile ground for reexamination and reinterpretation of dental characteristics (Bromage et al., 2005). As such, a novel, non-destructive approach has been developed which combines the work of two established technologies (confocal microscopy and 3D modeling) adapted specifically for the purpose of mineralized tissue imaging. Through this method, 3D functional masticatory and therefore occlusal molar microwear is able to be visualized, quantified and comparatively analyzed to assess dietary preference in Javanese Homo erectus. This method differs from other microwear investigative techniques (defining 'pits'- vs- 'scratches', microtexture analysis etc.) in that it defines a molars masticatory microwear functional interactions in 3-dimensions as its baseline dataset for further interpretations and analyses. Due to poor specimen collection techniques employed during the first half of the 20th century, the very complex geologic nature of the Sangiran Dome and disagreements over its chronostratigraphy, only very few scientific works have addressed the Sangiran 7 (S7) Homo erectus molar collection (n=25) (e.g. Grine and Franzen, 1994; Kaifu, 2006). Grine and Franzen's (1994) work was a predominantly qualitative initial assessment of the specimens and identified five specimens that might better be ascribed to a fossil pongid rather than H. erectus. They also noted several molars to which tooth position (M1 or M2) was unable to be ascribed (Grine and Franzen, 1994). Kaifu (2006) comparatively examined crown sizes in several S7 molars.
The Sangiran 7 collection originates from two distinct geologic horizons: ten from the older Sangiran Formation (S7a, ~1.7 to 1.0mya) and fifteen from the younger, overlying Bapang Formation (S7b, ~1.0 to .7mya). During this million year period, Java was connected to the mainland during various glacio-eustatic low-stands in sea level. These mainland connections varied in size, extent, climatic condition and therefore in faunal and floral composition. As the S7 sample may be representative of the earliest Homo erectus migrants into Java and spans long durations of occupation, its investigation yields potential to understand the various influences climatic and ecogeographic fluctuations had on these populations. Since the sample consists only of teeth, an ecodietary approach has been deemed the most logical and appropriate investigative approach. Questions regarding the intra- and inter- S7 sample
relationships will also be addressed.
By comparing various aspects of the H. erectus dentition against that of hunter/ gatherer's (H/G) whose diet is known, functional dietary similarity can be directly correlated. Thus a comparative molar sample consisting of the below historic hunter/ gather's (n=63) has been included in order to assess H. erectus's diet in ecological context: Inuit (n=9), Pacific Northwest Tribes (n=11), Fuegians (n=11), Australian Aborigines (n=12) and Bushman (n=20). Methodologically, this approach produces a 3D facet microwear vector (fmv) signature for each molar which can then be compared for statistical similarity.
Microwear (and, as such, the fmv signatures) was defined by the regular, parallel striations found on specific cusp facets known to arise from patterned, directional masticatory movements. This differs significantly from post-mortem or taphonomic microwear which produces striations at irregular angles on multiple, non-masticatory surfaces (Peuch et al.1985, Teaford, 1988). A 'match value' is produced to determine the similarity of two molars fmv's. The 'match values' are ranked (high to low) and these rankings are used to statistically analyze and infer dietary preference: between Sangiran 7 (as an entire sample) compared against that of the historic hunter/ gatherer H. sapiens whose diet and ecogeography is known; within S7a and S7b and then among the S7 sample (eg. S7a-vs-S7b); whether the purported Pongo molars actually affiliate well with H. erectus, the hunter-gatherer's or if they demonstrate distinctly different fmv signatures altogether; whether fmv signatures are useful in distinguishing molars whose tooth position is in doubt (eg. M1 or M2).
When compared against individual H/G molars, the results show that Sangiran 7 H. erectus most closely correlates with Bushmen across all areas of fmv signature analysis. However, within broader dietary categories (yearly reliant on proteinaceous foods; seasonally reliant on proteinaceous foods; not reliant on proteinaceous foods), it was found that H. erectus most closely allied with the two hunter/ gatherer subpopulations associated with the 'Seasonally reliant on proteinaceous foods' (Australian Aboriginals and Pacific Northwest Tribes). There was also evidence for dietary change or specialization over time. As the environment changed during occupation by the earlier Sangiran to the later Bapang individuals, the dietary preference shifted from a focus on vegetative foods to a diet much more inclusive of proteinaceous resources.
These results are considered logical within the larger ecogeographic and chronostratigraphic context of the Sangiran Dome during the Pleistocene. However, a larger sample would be needed to confirm this. Although general dietary preferences can be drawn from this method, it is not possible at present to define specific foods consumed on a daily basis (eg. tubers or tortoise meat).
Out of the five specimens possibly allied with Pongo, S7-14 matched at the 'high' designation with a hunter/ gatherer, S7-62 matched 'moderately', S7-20 matched 'low' while the remaining two were not able to be matched with any other teeth for various reasons. Although designation to Pongo cannot be ruled on at this time using this method, it does demonstrate that at least two of the teeth correlate well with various hunter/ gatherer's who do not share dietary similarity with Pongo. This suggests their designation as Pongo should be more closely reevaluated. As for the four specimens whose tooth position was unsure, S7-14 matched 'highly' with 1st molars, S7-62 and S7-78 matched 'moderately' with 2nd and 1st molars respectively while S7-20 only matched at the 'low' designation. Although this approach is still exploratory, it adds another analytical tool for use in defining tooth position.
In sum, this method has demonstrated its usefulness in defining and functionally analyzing a novel 3D molar microwear dataset to interpret dietary preference. Future work would include a pan- H. erectus molar sample in order to illuminate broader populational, taxonomic and dietary correlations within and amoung all H. erectus specimens. A larger, more heterogenous historic H/G sample would also be included in order to provide a wider dietary comparative population. This method can be further extended to include and compare any and all hominins as well as any organism which produces micro wear upon it molars. Also, the data obtained and resultant fmv signature diagrams have the potential to be incorporated into 3D VR reconstructions of mandibular movement thus recreating mastication in extinct organisms and leading to more robust anatomical and physiological investigations especially when viewed in the context of larger environmental conditions or changes.
Synaptic plasticity is the basis for information storage, learning and memory and is achieved by modulation of the synaptic transmission. The amount of active AMPA (α-amino-3-hydroxy-5-methyl-4-isoxazol-propionic acid) receptors at the synapse determines the transmission properties, therefore the regulation of AMPA receptor trafficking affects the synaptic strength. The protein GRIP (glutamate receptor interacting protein) binds to AMPA receptors and is one of the important regulators of AMPA receptor stability at the synapse (Dong et al., 1997; Osten et al., 2000). Previous studies have shown that the ablation of ephrinB2 or ephrinB3 in the nervous system leads to severe defects in hippocampal LTP (long term potentiation) and LTD (long term depression) (Grunwald et al., 2004). We found that ephrinB2 ligands play an important role in the stabilization of AMPA receptors at the cellular membrane (Essmann et al., 2008). Treating cultured hippocampal neurons with AMPA resulted in a robust AMPA receptor internalization, which could be inhibited by simultaneous ephrinB2 activation with soluble EphB4-Fc fusion proteins. Conditional hippocampal ephrinB2 knock-out (KO) neurons showed enhanced constitutive internalization of AMPA receptors. Interaction and interference experiments revealed that ephrinB ligands and AMPA receptors are bridged by GRIP. This interaction is regulated by phosphorylation of a single serine residue in close proximity to the C-terminal PDZ protein target site in ephrinB ligands (Essmann et al., 2008). To investigate the in vivo relevance of this previously undescribed feature of ephrinB reverse signaling, we generated ephrinB2 S-9>A knock-in mice, where the serine at position -9 was replaced by an alanine to prevent phosphorylation. The mutated ephrinB2 of this mouse line was expressed and able to form clusters following stimulation with the preclustered receptor EphB4-Fc. Surface ephrinB2 cluster size and cluster number was slightly smaller in comparison to wild type (WT) mice. Analyzing AMPA receptor internalization, we oserved an increased basal GluR2 endocytosis in cultured hippocampal neurons of ephrinB2 S-9>A mice. Dendrite and spine morphology was similar in pyramidal CA1 neurons of brain slices from adult ephrinB2 S-9>A and WT mice, suggesting a redundancy between the different ephrinB familily members.
Apart from regulating AMPA receptor stability at the synapse, GRIP1 also has an important role in the secretory pathway to deliver cargo proteins along microtubules to dendrites and synapses (Setou et al., 2002). Proteins involved in synaptic transmission and plasticity, as well as lipids required for the outgrowth and remodeling of dendrites and axons have to be transported. We showed in our laboratory with a directed proteomic analysis using the tandem affinity purification-mass spectrometry methodology (Angrand et al., 2006) and with immunoprecipitation assays with brain lysates that the small regulatory protein 14-3-3 interacts with GRIP1. Further immunoprecipitation assays with lysates from HeLa cells transfected with various parts and sequence mutants of GRIP1 revealed that threonine 956 in the linker region L2 between PDZ6 and PDZ7 of GRIP1 is necessary for the interaction with 14-3-3. GRIP1 has been postulated to influence dendritic arborization and maintenance in hippocampal neurons in culture due to defective kinesin-dependent transport along microtubules (Hoogenraad et al 2005). In order to address the role of the association of GRIP1 and 14-3-3 in dendritogenesis, we transfected rat hippocampal neurons with GRIP1-WT and GRIP1 mutants and performed Sholl analysis to evaluate dendritic arborization defects. We could observe striking increased formation and growth of dendrites in developing neurons as well as in mature neurons overexpressing GRIP1-WT. However, overexpression of GRIP1-T956A, where the threonine 956 was replaced by an alanine to prevent phosphorylation, did not show enhanced dendritogenesis, indicating a role for threonine 956 phosphorylation in dendrite branching. To investigate the importance of the interaction between GRIP1 and 14-3-3 in vivo, we generated transgenic mouse lines with a GRIP1-T956A transgene or a GRIP1-WT transgene as control. These mice were crossed with heterozygous GRIP1 mice and by further breedings we obtained some surviver mice carrying either the wild type or the mutated GRIP1 transgene in the usually embryonic lethal GRIP1-KO background (Bladt et al., 2002; Takamiya et al., 2004). In embryonic day (E) 14.5 cultured hippocampal GRIP1-KO neurons we could observe reduced dendritic growth. We also showed reduced GluR2 staining on the dendritic surface in cultured hippocampal neurons from GRIP1-KO and GRIP1-KO neurons containing the GRIP1-T956A transgene. GRIP1-KO neurons containing the GRIP1-WT transgene showed a similar surface GluR2 signal intensity as WT neurons. Reduced surface GluR2 staining in GRIP1-KO neurons and GRIP1-KO neurons with the GRIP1-T956A transgene might be a consequence of defective kinesin-dependent transport of GluR2 to dendrites, indicating an important role of threonine 956 phosphorylation of GRIP1 for GluR2 trafficking.
Stem cells are often referred to as potential candidates for the treatment of different pathologies. Their ability to differentiate into various tissue specific cell types offers the possibility to engineer cell systems or organs for replacement. One of the main questions in stem cell biology is how stemness properties are regulated and to what extend this regulation is intrinsic or conveyed by the direct microenvironment (‘niche’). In order to elucidate such regulatory processes, it is informative to analyze processes or molecules that are shared between different stem cell populations.
One such molecule that is expressed on a wide range of different embryonic and adult as well as tumor stem cells is the ABC transporter Abcg2. ABC transporters in general are transmembrane proteins that actively extrude endo- and exotoxins as well as xenobiotics, thereby protecting cells and organs. Additionally, ABC transporters are responsible for drug resistance in many cancers. A well-described characteristic of stem cells expressing Abcg2 is the formation of the ‘side population’ (SP) phenotype: An active Abcg2 transporter mediates the efflux of a particular fluorescent dye that is taken up by all cells, thus leading to a less brightly stained population. This phenomenon is widely used to characterize and isolate the most primitive stem cell subpopulation from embryonic and adult tissues, including tumors. Besides its role as toxin transporter little is known about the function of Abcg2 in stem cells. This is mainly due to the fact that its physiological substrate in stem cells remains unknown. The identification of such substrates is therefore of high interest because it would directly link the activity of ABC transporters to regulatory mechanisms in stem cell biology.
In the present study we wanted to test the hypothesis that the sphingolipid ceramide is a physiological substrate of the ABC transporter Abcg2. Sphingolipids are potent second messengers and are known to have regulatory functions in stem cells. In particular, the sphingolipid ceramide is described as a mediator of controlled cell death and inducer of differentiation. It is suggested that stem cells need to keep their intracellular ceramide content at low levels in order to prevent apoptosis or differentiation. We propose that Abcg2 and ceramide interact and that this interaction leads to changes in the absolute or relative amounts of ceramide. This in turn influences basic stem cell functions such as self renewal and differentiation.
We show that Abcg2 prevents cells from accumulating fluorescence labeled ceramide. Furthermore, exogenously applied ceramides inhibit the transport activity of Abcg2, measured by a decrease of the side population phenotype. This inhibitory effect is consistent with a competitive inhibition mechanism. Additionally, we show that active Abcg2 can increase the ceramide concentration in cell culture supernatant. Finally we demonstrate that Abcg2 protects from ceramide induced cytotoxicity in human cell lines. In summary, these in vitro results strongly suggest that Abcg2 has the ability to regulate ceramide levels.
Murine hematopoietic stem cells (HSCs) are the best characterized adult stem cell system so far. By using 7-colour fluorescence-activated cell sorting (FACS) we established the purification of the most primitive HSCs, reflected by their high engraftment capability when transplanted to lethally irradiated mice. By using this sorted cell populations it was in addition possible to establish a system to reproducibly manipulate HSCs ex vivo. This experimental system will serve in further elucidating the physiological consequences of Abcg2 mediated changes in ceramide levels on stem cells in vivo.
Taken together, this study shows that Abcg2 has the ability to regulate ceramide levels in cells. This in turn can lead to cellular protection from ceramide induced apoptosis. Additionally, the experimental techniques to further analyze the role of Abcg2 and ceramide in the most primitive hematopoietic stem cells were successfully established, enabling more detailed analysis in the future.
Conclusion: Proteins containing a Jumonji C (JmjC) domain appear in almost all living organisms and catalyze a variety of oxidation reactions. Therefore, they are important regulators in many biological processes such as proliferation and differentiation. They act either as protein hydroxylases, histone demethylases or by regulate mRNA splicing. Given the fact that some of the JmjC domain-containing proteins are shown to be upregulated in response to hypoxia as well as the dependency of JmjC domain catalytic activity on oxygen led to the assumption of an involvement in angiogenesis. For Jmjd6, a member of the JmjC domain-containing protein family, a regulatory involvement in mRNA splicing has been shown. The Jmjd6-/- mouse dies perinatally due to several severe organ malformations, especially in the heart. Despite the pale appearance, the growth retardation and the cardiac defects, it is unclear whether these mice exhibit defects of cells comprising the vasculature. Therefore, the involvement of Jmjd6 in angiogenesis was examined in vitro using angiogenesis assays as well as in vivo using the Jmjd6+/- mouse. An siRNA-mediated knockdown of Jmjd6 in ECs significantly impaired the formation of capillary-like networks in the tube formation assay as well as sprouting in the spheroid assay. Moreover, after siRNA-mediated knockdown of Jmjd6 in ECs cell migration was significantly reduced. These findings were confirmed in the matrigel plug assay in vivo. Implanted matrigel plugs of Jmjd6+/- mice exhibited significantly less perfused vessels compared to wildtype littermates. Furthermore, cultured lung ECs from Jmjd6+/- mice exhibited impaired network forming activity ex vivo compared to cells isolated from wildtype littermates. To elucidate the mechanisms underlying the requirement of Jmjd6 in angiogenesis, an Affymetrix exon-array was performed, which allows detection of changes in gene expression as well as splicing. The siRNA-mediated knockdown of Jmjd6 altered the expression of genes known to play a role in vascular biology. The bioinformatic assessment of alternative splice variants revealed that Jmjd6 silencing affects the splicing of the VEGF receptor 1 (Flt1). Differential splicing of Flt1 was shown to generate a short and soluble form of Flt1 (sFlt1), which sequestrates VEGF and PlGF, and thereby inhibits angiogenesis. In particular, a significant increase in sFlt1 expression was observed. Jmjd6 was recently reported to hydroxylate the splicing factor U2AF65. Therefore, we investigated whether U2AF65 might mediate Flt1 splicing and binds to Flt1 mRNA. Indeed, U2AF65 co-immunoprecipitated with Jmjd6 in ECs, while an interaction of U2AF65 with sFlt1 was demonstrated. Moreover, inhibition of Jmjd6 catalytic function by reduced oxygen concentration altered splicing of Flt1 resulted in an increase of the sFlt1 splice variant. Finally, saturating concentrations of VEGF or PlGF or neutralizing antibodies against sFlt1 significantly reduced the inhibition of sprouting caused by Jmjd6 knockdown in vitro.
Collectively, our results indicate that Jmjd6 has an essential role in the oxygen-dependent regulation of angiogenesis by controlling the splicing of Flt1 mRNA, thereby adjusting the generation of the anti-angiogenic short splice variant sFlt1. Several publications demonstrated a major importance for sFlt1 as a biomarker for many severe human diseases such as preeclampsia, sepsis, cancer, myocardial infarction as well as chronic heart failure. Therefore, the identification of the molecular mechanism behind the generation of sFlt1 might enable the development of new or more precise clinical markers for the diagnosis of the corresponding diseases. Furthermore, the discovery of the enzymes involved in the generation of sFlt1 provides further possibilities to modulate sFlt1 levels and thereby may potentially gives rise to the development of new therapies.
The translocation of nuclear-encoded precursor proteins into chloroplasts is a highly ordered process involving the action of several components to regulate this molecular ensemble. Not only GTP hydrolysis and GDP release but also the phosphorylation of TOC GTPases is a widely discussed mechanism to regulate protein import. The receptor component (Toc34) and its isoform of A. thaliana (atToc33) were found to be regulated by phosphorylation. Although the phosphorylation of Toc33 is already known for several years, several questions regarding the molecular components involved in the regulation of the phosphorylation process, precisely what is the protein kinase and where this kinase is initially localized, so far remained unclear.
This thesis aimed at the defining of the phosphorylation status of TOC GTPases in monomeric and/or dimeric states, the identification of the nature of Toc33-PK (protein kinase), and in the same context it aimed at gaining first insights into the physiological significance of Toc33 phosphorylation. To this end, (I) An in vitro and in vivo system for investigating of TOC GTPases Phosphorylation (in monomeric or dimeric state) was developed. Since no information is available about the phosphorylation status of the Toc159 isoforms, the second receptor of the TOC complex, it was interesting to investigate whether these isoforms undergo phosphorylation or not. The results indicated that atToc159 isoforms are able to be phosphorylated by the kinase activity in purified outer envelope membranes (OEMs) of pea, but not atToc132. Moreover, an artificial dimer of psToc34 based on the interaction of a C-terminally fused leucine zipper was not phosphorylated. This result reflected the inability of the OEM kinase to phosphorylate the dimers of TOC GTPases. Also, In vivo labeling of atToc33 was developed and occurred in a dose-dependent manner. Therefore, this results evidenced that in vitro phosphorylation of atToc33 (both endogenous wild type and recombinant expressed proteins) is not artificial labeling but represents a physiological relevance. CD (circular dichroism) measurements revealed that recombinant GTPase domain of atToc33 is preferentially phosphorylated in its folded state. Therefore, it could be suggested that folding of atToc33rec is a prerequisite for its phosphorylation and the phosphorylation event occurs as a posttranslational modification most likely after insertion of Toc33 (Toc34) into the OE of chloroplasts.
Secondly, (II) Isolation and identification of Toc33-PK from OEMs of chloroplasts was performed. Four independent strategies were developed to identify the Toc33-protein kinase: UV-induced and chemically-based crosslinking, different applied chromatographic techniques, identification of PK-Toc33 interaction by means of HDN-PAGE (histidine- and deoxycholate-based native PAGE), and finally mass spectrometric approaches were performed on fractions including the potential kinase activity. UV-induced crosslinking procedure was developed and resulted in covalent bonding of nine proteins to [a-32P] ATP, while chemically-based one was not significant. The applied chromatographic and HDN-PAGE approaches, including mass spectrometry, have revealed the identification of 13 protein kinases. Of these identified kinases, phototropin2 (Phot2, AT5G58140), leucine-rich repeat PK (LRR-PK, AT4G28650.1), and receptor-like transmembrane PK (RLK, AT5G56040.2) were selected as the most promising candidates (ca. kinase type and one transmembrane helix for membrane localization).
(III) The physiological significance of Toc33 phosphoryation was shown to link this process with the environmental changes (especially, the light conditions). Identification of chloroplast OE-located PKs performed by nLC-MALDI-MS/MS resulted in the detection of Phot2. Furthermore, the subcellular localization of Phot2 in OEM of chloroplasts was confirmed by immunoblotting experiments using a-Phot2 antibody. The kinase activity of Phot2 towards TOC GTPases was characterized and revealed that fused GST-KD (kinase domain) protein able to specifically phosphorylate atToc33rec, but not atToc159rec. Also, endogenous atPhot2 was upregulated and heavily detected in the ppi1-S181A plant line (where serine to alanine exchange was performed to abolish the phosphorylation of atToc33). Hence, we suggested that certain signal cascades may directly or indirectly link Toc33 receptor phosphorylation, protein levels of Phot2 (as promising PK candidate), and irradiation conditions (as an inducing signal of the subsequent phosphorylation events). Light-dependent phosphorylation of Toc33 was shown either after de-etiolation conditions or after high light intensities of blue light was performed. Therefore, phosphorylation of Toc33 might be identified as an external regulatory signal to regulate preproteins import into chloroplasts in response to environmental conditions (e.g. light changes) or as a signal of chloroplast biogenesis.
Development of lentiviral vectors for the gene therapy of X-linked chronic granulomatous disease
(2010)
Es gibt eine Vielzahl von Erkrankungen, die auf einen einzelnen Gendefekt zurückzuführen sind (monogene Erkrankungen). Darunter befindet sich auch die Gruppe der primären Immundefizienzen (PIDs), von denen aktuell über 150 verschiedene Typen von der Weltgesundheitsorganisation registriert sind. In vielen fällen leiden betroffene Individuen unter einem stark erhöhten Infektionsrisiko durch bakterielle oder virale Pathogene, sowie den damit verbundenen schweren Symptomen - bis hin zum verfrühten Tod der Patienten. Meist können PIDs mit konventionellen Methoden präventiv behandelt werden. Dazu gehören zum Beispiel die regelmässige Gabe von Antibiotika, Antimykotika, Zytokinen oder Immunglobulinen. Der einzige zur Verfügung stehende kurative Behandlungsansatz beruht auf der Transplantation von hämatopoietischen Stammzellen (HSZT) eines gesunden und passenden Spenders. Häufig steht jedoch kein histokompatibler Spender zur Verfügung.
Für diese Patientengruppe hat sich die gentherapeutische Behandlung mit autologen hämatopoietischen Stammzellen als eine gute Option herausgestellt. Der Beweis hierfür wurde eindrucksvoll in klinischen Heilversuchen für zwei Formen des Schweren Kombinierten Immundefekts (X-SCID und ADA-SCID) geführt, einer Erkrankung die durch das vollständige Fehlen bzw. die nicht-Funktionalität der lymphoiden Immunzellen charakterisiert ist. Autologe hämatopoietische Stammzellen der Patienten wurden hier ex vivo mittels eines gamma-retroviralen Vektors mit einer funktionellen Kopie der defekten cDNA genetisch modifiziert und anschliessend zurück infundiert. In der Summe wurde bei über 30 Patienten eine deutliche Verbesserung des Gesundheitszustandes bis hin zur vollständigen Heilung erzielt. Bei einem vergleichbaren Ansatz wurden in Frankfurt, in einem Heilversuch für die septische Granulomatose (X-CGD), erstmals klinisch relevante Erfolge in der Gentherapie für einen Defekt in der myeloischen Linie von Immunzellen erzielt. Ursache der X-chromosomal gekoppelten Form der septischen Granulomatose sind Mutationen in dem Gen für gp91phox (CYBB), einer essentiellen Untereinheit des in Phagozyten benötigten NADPH-Oxidase Komplexes. In der Folge sind die Phagozyten dieser Patienten nicht mehr in der Lage, die für das Abtöten von Krankheitserregern nötigen reaktiven Sauerstoffspezies zu bilden. Ständig wiederkehrende schwere Infektionen mit sonst unproblematischen Erregern sind die Folge.
Neben klaren gesundheitlichen Verbesserungen in der Mehrzahl der Patienten hatte diese Gentherapeutische Behandlungsstrategie in einigen Fällen auch klare Nebenwirkungen. In fünf von 20 Patienten mit X-SCID, sowie in beiden behandelten X-CGD Patienten, kam es infolge der Therapie zu hämatologischen Veränderungen, die in der Ausbildung eines myelodysplastischen Syndroms (bei X-CGD) und Leukämie (bei X-SCID) mündeten. In allen Fällen war die Ursache eine Hochregulierung von Proto-Onkogenen in der Nähe von g-retroviralen Integrationsstellen. Diese Probleme demonstrieren deutlich die unbedingte Notwendigkeit zur Verbesserung der verwendeten therapeutischen Vektoren.
In der vorliegenden Arbeit wurden lentivirale Vektoren mit myeloid-spezifischen Promotoren entwickelt und auf ihre Eignung für die Gentherapie der X-chromosomal gekoppelten septischen Granulomatose getestet. Lentivirale Vektoren besitzen ein stark verringertes Risiko für Insertionsmutagenese, sowie die exklusive Fähigkeit ruhende Zellen zu transduzieren. Die Verwendung von myeloid-spezifischen Promotoren für die Transgenexpression verringert die Wahrscheinlichkeit der Proto-Onkogen Aktivierung in unreifen Stamm- und Vorläuferzellen – einer Zellpopulation die besonders sensitiv für die in der Leukämieentstehung obligaten Schritte der Immortalisierung und Transformation ist. Gleichzeitig bleibt der volle therapeutische Nutzen erhalten, da das Transgen gp91phox nur in reifen myeloischen Zellen benötigt wird.
Die entwickelten lentiviralen Vektoren exprimieren eine kodonoptimierte gp91phox cDNA unter der Kontrolle des microRNA223-Promoters (223), des MRP8-Promotors (M) oder eines chimären Fusionspromoters bestehend aus den regulatorischen Bereichen des Cathepsin G und des cFes-Promotors (Chim). Zusätzlich wurde ein sogenanntes „ubiquitär aktives Chromatin-öffnendes Element“ (UCOE) in beiden Orientierungen vor den MRP8-Promotor kloniert, um eine erhöhte und stabile Langzeitexpression des Transgens zu erreichen. Ziel der Arbeit war die Selektion eines geeigneten Kandidaten für präklinische Versuchsreihen.
Die für die Evaluierung der Vektoren relevanten Parameter waren die Transgenexpressionslevel, die Spezifität der Expression für myeloische Zellen sowie die vermittelte funktionelle Rekonstitution der NADPH-Oxidase Aktivität. Die Fragestellungen der Langzeitexpression, der Anfälligkeit für CpG-Methylierung sowie der Genotoxizität der Vektoren wurden ebenfalls bearbeitet. Die Vektoren wurden in vitro in verschiedenen Zelllinien sowie in in vitro differenzierten primären murinen und humanen Blutstammzellen getestet. Die beiden besten Kandidaten (223 und Chim) wurden in vivo in Maustransplantationsexperimenten (Maus-Maus und humane Stammzellen in NOD/SCID-Mäuse) analysiert.
Die beiden lentiviralen Vektoren 223 und Chim eignen sich beide für eine effiziente Expression in myeloische Zellen, die zur funktionellen Rekonstitution der NADPH-Oxidase Aktivität in vitro und in vivo führen. Sie sind den bisher in klinischen Anwendungen verwendeten Vektoren in allen Parametern klar überlegen. Daher ist in zukünftigen klinischen Anwendungen ein verbesserter therapeutischer Nutzen für die Patienten sowie eine Verminderung des Risikos von Nebenwirkungen zu erwarten.
Plastids are complex organelles that fulfil numerous essential cellular functions, such as
photosynthesis, amino acid and fatty acid synthesis. he majority of proteins required for
these functions are encoded in the nuclear genome and synthesised on cytosolic ribosomes as
precursors, which are posttranslationally transported to and imported into the organelle by
concerted actions of translocons in the outer and inner chloroplast membrane. For most
preproteins, targeting to the organelle is ensured by a specific import signal, a so called
transit peptide, which is specifically recognised by receptors at the chloroplastês surface. A transit peptide is generally defined as essential and sufficient for precursor targeting to and
translocation into chloroplasts, (however, an analysis of the ability of transit peptides to drive translocation of tightly folded passenger domain revealed that the transit peptide is not
always sufficient for the translocation event. A critical signal length requirement of amino
acids has been determined in vivo and in vitro. In the case of shorter transit peptide, the
succeeding portion of the mature domain provides an extension of an unfolded polypeptide
stretch required for successful translocation. The analysis of the unfolding mode of a folded
model passenger during translocation links the observed transit peptide length requirement
to the action of an energising unit present in the intermembrane space of chloroplasts.
The likely candidate for this energising unit space is putative imsHsp70, previously hypothesised to function in translocation of precursor proteins across the outer membrane. However, as the identity of this protein has up to now remained unknown, its existence has
been a matter of debate. The present study focuses on the isolation and characterisation of
imsHsp70 at the molecular level. Mass spectrometry analyses and in vivo localisation studies
demonstrate that while no specific imsHsp70 exists, multiple cytosolic Hsp70 isoforms are
targeted to the intermembrane space, but not to the stroma of chloroplasts. Thus, a so far unrecognised mode of dual targeting to chloroplasts and cytosol is most likely to ensure the
allocation of (sp s into the intermembrane space.
Crista junctions (CJs) are tubular invaginations of the inner membrane of mitochondria that connect the inner boundary with the cristae membrane. These architectural elements are critical for mitochondrial function. The yeast inner membrane protein Fcj1, called mitofilin in mammals, was reported to be preferentially located at CJs and crucial for their formation. Here we investigate the functional roles of individual domains of Fcj1. The most conserved part of Fcj1, the C-terminal domain, is essential for Fcj1 function. In its absence, formation of CJ is strongly impaired and irregular, and stacked cristae are present. This domain interacts with full-length Fcj1, suggesting a role in oligomer formation. It also interacts with Tob55 of the translocase of outer membrane β-barrel proteins (TOB)/sorting and assembly machinery (SAM) complex, which is required for the insertion of β-barrel proteins into the outer membrane. The association of the TOB/SAM complex with contact sites depends on the presence of Fcj1. The biogenesis of β-barrel proteins is not significantly affected in the absence of Fcj1. However, down-regulation of the TOB/SAM complex leads to altered cristae morphology and a moderate reduction in the number of CJs. We propose that the C-terminal domain of Fcj1 is critical for the interaction of Fcj1 with the TOB/SAM complex and thereby for stabilizing CJs in close proximity to the outer membrane. These results assign novel functions to both the C-terminal domain of Fcj1 and the TOB/SAM complex.
BACKGROUND: The identification of beta-barrel membrane proteins out of a genomic/proteomic background is one of the rapidly developing fields in bioinformatics. Our main goal is the prediction of such proteins in genome/proteome wide analyses.
RESULTS: For the prediction of beta-barrel membrane proteins within prokaryotic proteomes a set of parameters was developed. We have focused on a procedure with a low false positive rate beside a procedure with lowest false prediction rate to obtain a high certainty for the predicted sequences. We demonstrate that the discrimination between beta-barrel membrane proteins and other proteins is improved by analyzing a length limited region. The developed set of parameters is applied to the proteome of E. coli and the results are compared to four other described procedures.
CONCLUSION: Analyzing the beta-barrel membrane proteins revealed the presence of a defined membrane inserted beta-barrel region. This information can now be used to refine other prediction programs as well. So far, all tested programs fail to predict outer membrane proteins in the proteome of the prokaryote E. coli with high reliability. However, the reliability of the prediction is improved significantly by a combinatory approach of several programs. The consequences and usability of the developed scores are discussed.
Enzymes involved in tRNA maturation are essential for cytosolic, mitochondrial, and plastid protein synthesis and are therefore localized to these different compartments of the cell. Interestingly, only one isoform of tRNA nucleotidyltransferase (responsible for adding the 3′-terminal cytidine–cytidine–adenosine to tRNAs) has been identified in plants. The present study therefore explored how signals contained on this enzyme allow it to be distributed among the different cell compartments. It is demonstrated that the N-terminal portion of the protein acts as an organellar targeting signal and that differential use of multiple in-frame start codons alters the localization of the protein. Moreover, it is shown that the mature domain has a major impact on the distribution of the protein within the cell. These data indicate that regulation of dual localization involves not only specific N-terminal signals, but also additional factors within the protein or the cell.
Eukaryotic ribosome biogenesis requires the concerted action of numerous ribosome assembly factors, for most of which structural and functional information is currently lacking. Nob1, which can be identified in eukaryotes and archaea, is required for the final maturation of the small subunit ribosomal RNA in yeast by catalyzing cleavage at site D after export of the preribosomal subunit into the cytoplasm. Here, we show that this also holds true for Nob1 from the archaeon Pyrococcus horikoshii, which efficiently cleaves RNA-substrates containing the D-site of the preribosomal RNA in a manganese-dependent manner. The structure of PhNob1 solved by nuclear magnetic resonance spectroscopy revealed a PIN domain common with many nucleases and a zinc ribbon domain, which are structurally connected by a flexible linker. We show that amino acid residues required for substrate binding reside in the PIN domain whereas the zinc ribbon domain alone is sufficient to bind helix 40 of the small subunit rRNA. This suggests that the zinc ribbon domain acts as an anchor point for the protein on the nascent subunit positioning it in the proximity of the cleavage site.
Organelles are surrounded by membranes with a distinct lipid and protein composition. While it is well established that lipids affect protein functioning and vice versa, it has been only recently suggested that elevated membrane protein concentrations may affect the shape and organization of membranes. We therefore analyzed the effects of high chloroplast envelope protein concentrations on membrane structures using an in vivo approach with protoplasts. Transient expression of outer envelope proteins or protein domains such as CHUP1-TM–GFP, outer envelope protein of 7 kDa–GFP, or outer envelope protein of 24 kDa–GFP at high levels led to the formation of punctate, circular, and tubular membrane protrusions. Expression of inner membrane proteins such as translocase of inner chloroplast membrane 20, isoform II (Tic20-II)–GFP led to membrane protrusions including invaginations. Using increasing amounts of DNA for transfection, we could show that the frequency, size, and intensity of these protrusions increased with protein concentration. The membrane deformations were absent after cycloheximide treatment. Co-expression of CHUP1-TM–Cherry and Tic20-II–GFP led to membrane protrusions of various shapes and sizes including some stromule-like structures, for which several functions have been proposed. Interestingly, some structures seemed to contain both proteins, while others seem to contain one protein exclusively, indicating that outer and inner envelope dynamics might be regulated independently. While it was more difficult to investigate the effects of high expression levels of membrane proteins on mitochondrial membrane shapes using confocal imaging, it was striking that the expression of the outer membrane protein Tom20 led to more elongate mitochondria. We discuss that the effect of protein concentrations on membrane structure is possibly caused by an imbalance in the lipid to protein ratio and may be involved in a signaling pathway regulating membrane biogenesis. Finally, the observed phenomenon provides a valuable experimental approach to investigate the relationship between lipid synthesis and membrane protein expression in future studies.
The conformational dynamics induced by ligand binding to the tetracycline-binding aptamer is monitored via stopped-flow fluorescence spectroscopy and time-correlated single photon counting experiments. The fluorescence of the ligand is sensitive to changes within the tertiary structure of the aptamer during and after the binding process. In addition to the wild-type aptamer, the mutants A9G, A13U and A50U are examined, where bases important for regulation are changed to inhibit the aptamer’s function. Our results suggest a very fast two-step-mechanism for the binding of the ligand to the aptamer that can be interpreted as a binding step followed by a reorganization of the aptamer to accommodate the ligand. Binding to the two direct contact points A13 and A50 was found to occur in the first binding step. The exchange of the structurally important base A9 for guanine induces an enormous deceleration of the overall binding process, which is mainly rooted in an enhancement of the back reaction of the first binding step by several orders of magnitude. This indicates a significant loss of tertiary structure of the aptamer in the absence of the base A9, and underlines the importance of pre-organization on the overall binding process of the tetracycline-binding aptamer.
BACKGROUND:
Horizontal gene transfer through natural transformation of members of the microbiota of the lower gastrointestinal tract (GIT) of mammals has not yet been described. Insufficient DNA sequence similarity for homologous recombination to occur has been identified as the major barrier to interspecies transfer of chromosomal DNA in bacteria. In this study we determined if regions of high DNA similarity between the genomes of the indigenous bacteria in the GIT of rats and feed introduced DNA could lead to homologous recombination and acquisition of antibiotic resistance genes.
RESULTS:
Plasmid DNA with two resistance genes (nptI and aadA) and regions of high DNA similarity to 16S rRNA and 23S rRNA genes present in a broad range of bacterial species present in the GIT, were constructed and added to standard rat feed. Six rats, with a normal microbiota, were fed DNA containing pellets daily over four days before sampling of the microbiota from the different GI compartments (stomach, small intestine, cecum and colon). In addition, two rats were included as negative controls. Antibiotic resistant colonies growing on selective media were screened for recombination with feed introduced DNA by PCR targeting unique sites in the putatively recombined regions. No transformants were identified among 441 tested isolates.
CONCLUSIONS:
The analyses showed that extensive ingestion of DNA (100 μg plasmid) per day did not lead to increased proportions of kanamycin resistant bacteria, nor did it produce detectable transformants among the aerobic microbiota examined for 6 rats (detection limit < 1 transformant per 1,1 × 108 cultured bacteria). The key methodological challenges to HGT detection in animal feedings trials are identified and discussed. This study is consistent with other studies suggesting natural transformation is not detectable in the GIT of mammals.
Background: In mixed sugar fermentations with recombinant Saccharomyces cerevisiae strains able to ferment D-xylose and L-arabinose the pentose sugars are normally only utilized after depletion of D-glucose. This has been attributed to competitive inhibition of pentose uptake by D-glucose as pentose sugars are taken up into yeast cells by individual members of the yeast hexose transporter family. We wanted to investigate whether D-glucose inhibits pentose utilization only by blocking its uptake or also by interfering with its further metabolism.
Results: To distinguish between inhibitory effects of D-glucose on pentose uptake and pentose catabolism, maltose was used as an alternative carbon source in maltose-pentose co-consumption experiments. Maltose is taken up by a specific maltose transport system and hydrolyzed only intracellularly into two D-glucose molecules. Pentose consumption decreased by about 20 - 30% during the simultaneous utilization of maltose indicating that hexose catabolism can impede pentose utilization. To test whether intracellular D-glucose might impair pentose utilization, hexo-/glucokinase deletion mutants were constructed. Those mutants are known to accumulate intracellular D-glucose when incubated with maltose. However, pentose utilization was not effected in the presence of maltose. Addition of increasing concentrations of D-glucose to the hexo-/glucokinase mutants finally completely blocked D-xylose as well as L-arabinose consumption, indicating a pronounced inhibitory effect of D-glucose on pentose uptake. Nevertheless, constitutive overexpression of pentose-transporting hexose transporters like Hxt7 and Gal2 could improve pentose consumption in the presence of D-glucose.
Conclusion: Our results confirm that D-glucose impairs the simultaneous utilization of pentoses mainly due to inhibition of pentose uptake. Whereas intracellular D-glucose does not seem to have an inhibitory effect on pentose utilization, further catabolism of D-glucose can also impede pentose utilization. Nevertheless, the results suggest that co-fermentation of pentoses in the presence of D-glucose can significantly be improved by the overexpression of pentose transporters, especially if they are not inhibited by D-glucose.
Saccharomyces cerevisiae CEN.PK 113-7D is widely used for metabolic engineering and systems biology research in industry and academia. We sequenced, assembled, annotated and analyzed its genome. Single-nucleotide variations (SNV), insertions/deletions (indels) and differences in genome organization compared to the reference strain S. cerevisiae S288C were analyzed. In addition to a few large deletions and duplications, nearly 3000 indels were identified in the CEN.PK113-7D genome relative to S288C. These differences were overrepresented in genes whose functions are related to transcriptional regulation and chromatin remodelling. Some of these variations were caused by unstable tandem repeats, suggesting an innate evolvability of the corresponding genes. Besides a previously characterized mutation in adenylate cyclase, the CEN.PK113-7D genome sequence revealed a significant enrichment of non-synonymous mutations in genes encoding for components of the cAMP signalling pathway. Some phenotypic characteristics of the CEN.PK113-7D strains were explained by the presence of additional specific metabolic genes relative to S288C. In particular, the presence of the BIO1 and BIO6 genes correlated with a biotin prototrophy of CEN.PK113-7D. Furthermore, the copy number, chromosomal location and sequences of the MAL loci were resolved. The assembled sequence reveals that CEN.PK113-7D has a mosaic genome that combines characteristics of laboratory strains and wild-industrial strains.
Clathrin-mediated endocytosis (CME) involves spatially and temporally restricted molecular dynamics.
Although protein kinases and the actin cytoskeleton contribute to the process, whether and how
functions of kinases and actin are integrated remains unknown. Here, we demonstrate that neural
Wiskott-Aldrich syndrome protein (N-WASP) and protein kinase CK2 form a complex and localize on
clathrin-coated vesicles (CCVs). N-WASP binds to and is phosphorylated by CK2, thereby reducing the
kinase activity of CK2. By contrast, N-WASP-promoted actin polymerization is decreased upon both
phosphorylation and binding of CK2. Knockdown of N-WASP and CK2, alone or in combination, results
in impaired endocytosis of epidermal growth factor (EGF) and increased cell-surface levels of EGF
receptor (EGFR). In order to rescue the phenotype of N-WASP-CK2 knockdown cells, both N-WASP and
CK2 activities and abilities to assemble in a complex are required. In summary, this study shows that the
N-WASP-CK2 complex integrates in a single circuit different activities contributing to CME of EGFR and
that the interplay between the two proteins optimizes this process.
The Alpine Region, constituting the Alps and the Dinaric Alps, has played a major role in the formation of current patterns of biodiversity either as a contact zone of postglacial expanding lineages or as the origin of genetic diversity. In our study, we tested these hypotheses for two widespread, sympatric microgastropod taxa - Carychium minimum O.F. Müller, 1774 and Carychium tridentatum (Risso, 1826) (Gastropoda, Eupulmonata, Carychiidae) - by using COI sequence data and species potential distribution models analyzed in a statistical phylogeographical framework. Additionally, we examined disjunct transatlantic populations of those taxa from the Azores and North America. In general, both Carychium taxa demonstrate a genetic structure composed of several differentiated haplotype lineages most likely resulting from allopatric diversification in isolated refugial areas during the Pleistocene glacial periods. However, the genetic structure of Carychium minimum is more pronounced, which can be attributed to ecological constraints relating to habitat proximity to permanent bodies of water. For most of the Carychium lineages, the broader Alpine Region was identified as the likely origin of genetic diversity. Several lineages are endemic to the broader Alpine Region whereas a single lineage per species underwent a postglacial expansion to (re)colonize previously unsuitable habitats, e.g. in Northern Europe. The source populations of those expanding lineages can be traced back to the Eastern and Western Alps. Consequently, we identify the Alpine Region as a significant 'hot-spot' for the formation of genetic diversity within European Carychium lineages. Passive dispersal via anthropogenic means best explains the presence of transatlantic European Carychium populations on the Azores and in North America. We conclude that passive (anthropogenic) transport could mislead the interpretation of observed phylogeographical patterns in general.
European pea crabs - taxonomy, morphology, and host-ecology (Crustacea: Brachyura: Pinnotheridae)
(2010)
Pinnotherids are small crabs symbiotic to a variety of invertebrates. The European species infest bivalves and sea squirts. Their way of life is parasitic and poses a threat to commercially exploited bivalves. While juveniles of both sexes still look very similar - being agile swimmers and partially free living - a metamorphosis takes place in the female after mating and results in a conspicuous sexual dimorphism. Thereafter, the female settles in its host definitely and is morphologically strongly adapted to the parasitic life phase. A very high reproductive output was demonstrated among several pea crab species infesting bivalves. Despite from that, hardly any information is present in the literature on the pinnotherids’ reproductive biology and the underlying morphology.
Due to their cryptic way of life, the sexual dimorphism, and the different morphotypes of the female, the taxonomy of the Pinnotheridae is a serious challenge. Two widely accepted species are recognized on European coasts: Pinnotheres pisum and Nepinnotheres pinnotheres. Pinnotheres pectunculi was so far only known from the bivalve Glycymeris glycymeris in its type locality Roscoff (France), while Pinnotheres ascidicola and Pinnotheres marioni were described as living exclusively in ascidians without careful comparison with the previously described species. In order to produce standardized comparative descriptions, pea crabs were collected and studied from different hosts and localities in the Northeast Atlantic and in the Mediterranean. Nepinnotheres pinnotheres and Pinnotheres pisum were redescribed with consideration to characters of female and male. According to our morphological analysis, Pinnotheres ascidicola and Pinnotheres marioni are junior synonyms of Nepinnotheres pinnotheres, whereas the status of Pinnotheres pectunculi as a valid species was ascertained. Important characters are the mouthparts, the male gonopods, and especially chelipeds that showed consistent characteristics among different crab stages of both sexes.
Based on our sampling, we estimated the host-range of the European species. Nepinnotheres pinnotheres lives in ascidians and in the pen shell Pinna nobilis. Pinnotheres pisum infests numerous bivalve species - Pinna nobilis included. For Pinnotheres pectunculi novel host records are presented, all from the bivalve family Veneridae. Furthermore, feeding of the Pinnotheres-species was observed. They use a setae comb ventrally on the claw to brush mucus (and the accumulated food particles) from the bivalve gills. Feeding strategies and host-ecology will be thoroughly discussed in consideration to other Pinnotheridae.
We investigated the reproductive systems of European pinnotherids by histological methods, scanning and transmission electron microscopy, and confocal laser scanning microscopy.
The Eubrachyura have internal fertilization: paired vaginas enlarge into storage structures, the spermathecae, which are connected to the ovaries by oviducts. Sperm is stored until the oocytes are mature and transported into the spermathecae, where fertilization takes place. In the investigated pinnotherids, the vagina is of the ‘concave pattern’. Musculature is attached alongside flexible parts of the vagina-wall to control the dimension of its lumen. The genital opening is closed by a muscular mobile operculum.
The spermatheca can be divided into two distinct regions by function and morphology. The ventral part includes the connection with vagina and oviduct and is regarded as the zone where fertilization takes place. It is lined with cuticle except where the oviduct enters the spermatheca by the ‘holocrine transfer tissue’. At ovulation, the oocytes have to pass through this multi-layered glandular epithelium, which has a holocrine mode secretion. The dorsal part of the spermatheca is lined by a highly secretory apocrine glandular epithelium, which was to date only found in fiddler crabs of the genus Uca.
The male internal reproductive system consists of paired testes and corresponding vasa deferentia. The sperm morphology of pinnotherids conforms to other thoracotremes, with slight differences between Nepinnotheres pinnotheres and Pinnotheres pisum. Spermatozoa become enveloped into spermatophores in the secretory proximal vas deferens. The medial vas deferens is strongly enlarged and stores spermatophores embedded in seminal plasma. The distal vas deferens holds tubular appendices, which extend into the ventral cephalothorax and slightly into the pleon. These appendices produce and store vast quantities of seminal plasma. The copulatory system of the Brachyura is formed by paired penes and two pairs of gonopods, which function in sperm transfer. In pinnotherids, the long first gonopods transfers the sperm mass to the female. It holds the ejaculatory canal inside, which opens proximally and distally. The second gonopod is solid, short and conical. During copulation, the penis and the second gonopod are inserted into the base of the tubular first gonopod. The second gonopod functions in the transport of the sperm mass inside the ejaculatory canal towards its distal opening. The specific shape of the second gonopod is strongly adapted for a sealing of the tubular first gonopod with longitudinal cuticle foldings that interlock inside the first gonopod. The presented results are discussed concerning their function in reproduction and in respect of the systematic account.
The role of secretion in sperm transfer, storage and fertilization among the Brachyura is still under debate. It is notable that structure and function of secretion are more complex in pinnotherids and probably more efficient than in other brachyuran crabs, which will be discussed, in view of the parasitic way of life and the high fecundity of pinnotherids.
Das geographische Verbreitungsgebiet von Arten ist ein fundamentales Struktur gebendes Merkmal der biologischen Welt. Warum Arten so verteilt sind, wie sie sind ist seit langem eine der zentralen Fragen in Ökologie, Biogeographie und Evolution. Gegenwärtig verändern sich, im Wesentlichen als unbeabsichtigtes Nebenprodukt menschlicher ökonomischen Aktivitäten und Populationsdynamik, die geographischen Verbreitungsgebiete von Arten mit entscheidender Bedeutung für Land- und Forstwirtschaft, als Krankheitsvektoren oder als Teil der biologischen Systeme, die Ökosystemfunktionen bereitstellen. Daher ist es dringend notwendig, dass wir unser Verständnis über die Dynamiken, aus denen die geographische Verbreitung von Arten erwachsen, verbessern. Mit dieser Doktorarbeit versuche ich, in drei Untersuchungen zur Dynamik der Verbreitungsgebiete von Singvögeln einen Beitrag zu unserem in Entwicklung begriffenen Verständnis der multiplen Faktoren die Artverbreitungsgebiete beeinflussen, zu leisten.
1) Zu einem mechanistischeren Verständnis von Artmerkmalen und Verbreitungsgebietsgrößen: Ein wichtiger, ungelöster Fragenkomplex in der Makroökologie ist, die immense interspezifische Variation in der Größe geographischer Verbreitungsgebiete zu verstehen. Während man davon ausgeht, dass Artmerkmale wie Fekundität und Körpergröße einen Effekt auf Verbreitungsgebietsgrößen haben, fehlt ein allgemeines Verständnis davon, wie Verbreitungsgebietsgrößen von mehreren Merkmalen gemeinsam beeinflusst werden. Hier beurteilen wir den Effekt von Lebensgeschichtsmerkmalen (Fekundität, Ausbreitungsfähigkeit), ökologischen Merkmalen (Habitatnische, Nahrungsnische, Zugverhalten, Flexibilität im Zugverhalten) und morphologischen Merkmalen (Körpergröße) auf die globale Verbreitungsgebietsgröße von 165 europäischen Singvögeln. Wir identifizieren Hypothesen zur Beziehung von Artmerkmalen und Verbreitungsgebietsgrößen aus der Literatur und verwenden die Methodik der Pfadanalyse, um sie zu testen. Die Größe der globalen geographischen Verbreitungsgebiete europäischer Singvögel wurde von Lebensgeschichtsmerkmalen (Fekundidtät und Ausbreitungsfähigkeit), ökologischen Merkmalen (Habitatnischenbreite, Nahrungsnischenposition und Zugverhalten) und von Körpergröße beeinflusst. Artmerkmale beeinflussten Verbreitungsgebietsgrößen auf direktem und indirektem Weg. Insbesondere der Einfluss von Körpergröße war komplex mit positiven und negativen Effekten über verschiedene Pfade. Die Größe von Verbreitungsgebieten ist sehr wahrscheinlich auch von anderen Faktoren als von Artmerkmalen abhängig. Wir zeigen, dass es notwendig ist, den direkten und indirekten Einfluss einer Vielzahl von Merkmalen zu entwirren, um die Mechanismen, die makroökologische Beziehungen generieren, aufzuklären.
2) Konkurrenz und Ausbreitungsfähigkeit interagieren bei der Bestimmung der geographischen Verbreitung von Vögeln: Es ist weiterhin eine Herausforderung für Ökologie und Evolutionsbiologie, die Faktoren zu verstehen , die die geographische Verbreitung von Arten beeinflussen. Wir untersuchen wie Konkurrenz, Ausbreitungsfähigkeit, das Alter eines Taxons und Habitatverschiebungen seit dem letzten glazialen Maximum das Ausmaß beeinflussen, in dem Arten der Vogelgattung Sylvia in allen Gegenden mit geeigneten Umweltbedingungen vorkommen (d.h. range filling).
Wir haben range filling in der Vogelgattung Sylvia (Grasmücken) unter Verwendung von Boosted Regression Trees und Ridge-Regression quantifiziert. Mittels multipler Regression haben wir für die Effekte von intragenerischer Konkurrenz, Ausbreitungfähigkeit, Alter des Taxons und Habitatverschiebung seit dem letzten glazialen Maximum auf range filling getestet.
Grasmücken mit hoher Ausbreitungsfähigkeit zeigten höheres range filling, aber nur wenn Konkurrenz in Gebieten mit weniger geeignetem Habitat innerhalb ihres potentiellen Verbreitungsgebietes niedrig war. Das Alter eines Taxon und Habitatverschiebung seit dem letzten glazialen Maximum hatten keinen konsistenten Effekt. Wir zeigen, dass die Verbreitungsgebiete von Grasmücken mit hoher Wahrscheinlichkeit durch den simultanen, interaktiven Effekt von Konkurrenz und Ausbreitungsfähigkeit geformt werden. Wenn biotische Interaktionen wie Konkurrenz generell die Fähigkeit von Arten beeinflussen auf der kontinentalen Skala neue Gebiete zu kolonisieren, wird es eine Herausforderung sein, den Effekt von Klimawandel auf Biodiversität vorherzusagen.
3) Nischenverfügbarkeit in Zeit und Raum: Vogelzug der Grasmücken: Im Kontext neuer Fortschritte in der ökologischen Nischenmodellierung sind sowohl die Umwelt als auch die ökologische Nische einer Art als statische Entitäten behandelt und quantifiziert worden. In der Realität sind aber die Umwelt und die Nischenanforderungen einer Art auf einer Vielzahl von Skalen dynamisch. Wir schlagen ein konzeptionelles System vor das berücksichtigt, wie die realisierte Nische und geographische Verbreitung von Arten durch die entkoppelte raumzeitliche Verfügbarkeit unterschiedlicher Umweltbedingungen und durch Veränderungen der Nischenanforderungen über die Lebenszeit eines Organismus geformt werden. Das Testen von aus dem konzeptionellen System abgeleiteten Vorhersagen am Beispiel des Vogelzugs der Grasmücken ergab neue Erkenntnisse: Das Verfolgen der Klimanische im geographischen Raum war höchstwahrscheinlich nicht die treibende Kraft für Migration in der Gattung und steht potentiell im Konflikt mit dem Verfolgen der Landnutzungsnische. Die Nischen der Grasmücken waren während der Brutsaison schmaler, was zeigt, dass Nischenanforderungen zeitlich dynamisch sein können. Wir legen nahe, dass die Berücksichtigung dynamischer Umwelten und Nischenanforderungen zu einer entscheidenden Verbessserung unseres Verständnisses der treibenden Faktoren hinter der Bewegung von Organismen im Raum und der Dynamik ihrer Nischen und Verbreitungsgebiete führt.
Axonal growth is essential for establishing neuronal circuits during brain development and for regenerative processes in the adult brain. Unfortunately, the extracellular signals controlling axonal growth are poorly understood. Here we report that a reduction in extracellular ATP levels by tissue-nonspecific alkaline phosphatase (TNAP) is essential for the development of neuritic processes by cultured hippocampal neurons. Selective blockade of TNAP activity with levamisole or specific TNAP knockdown with short hairpin RNA interference inhibited the growth and branching of principal axons, whereas addition of alkaline phosphatase (ALP) promoted axonal growth. Neither activation nor inhibition of adenosine receptors affected the axonal growth, excluding the contribution of extracellular adenosine as a potential hydrolysis product of extracellular ATP to the TNAP-mediated effects. TNAP was colocalized at axonal growth cones with ionotropic ATP receptors (P2X7 receptor), whose activation inhibited axonal growth. Additional analyses suggested a close functional interrelation of TNAP and P2X7 receptors whereby TNAP prevents P2X7 receptor activation by hydrolyzing ATP in the immediate environment of the receptor. Furthermore inhibition of P2X7 receptor reduced TNAP expression, whereas addition of ALP enhanced P2X7 receptor expression. Our results demonstrate that TNAP, regulating both ligand availability and protein expression of P2X7 receptor, is essential for axonal development.
Splicing of pre-mRNA is a critical step in mRNA maturation and disturbances cause several genetic disorders. We apply the synthetic tetracycline (tc)-binding riboswitch to establish a gene expression system for conditional tc-dependent control of pre-mRNA splicing in yeast. Efficient regulation is obtained when the aptamer is inserted close to the 5′splice site (SS) with the consensus sequence of the SS located within the aptamer stem. Structural probing indicates limited spontaneous cleavage within this stem in the absence of the ligand. Addition of tc leads to tightening of the stem and the whole aptamer structure which probably prevents recognition of the 5′SS. Combination of more then one aptamer-regulated intron increases the extent of regulation leading to highly efficient conditional gene expression systems. Our findings highlight the potential of direct RNA–ligand interaction for regulation of gene expression.
Einfluss des Transkriptionsfaktors Tal1 auf die Osteoklastogenese durch Regulation von DC-STAMP
(2012)
Das menschliche Knochengewebe unterliegt einem ständigen Auf- und Abbau. Der Knochenumbau, die so genannte Knochenremodellierung, findet stetig statt und etwa 10 % des gesamten Knochengewebes werden innerhalb eines Jahres erneuert (Lerner UH, 2006). Während der Knochenremodellierung befindet sich die Zellaktivität der Knochenaufbauenden Osteoblasten und der Knochen-abbauenden Osteoklasten in einem empfindlichen Gleichgewicht (Karsenty G und Wagner EF, 2002; Teitelbaum SL, 2000).
Durch Störung des Gleichgewichts zwischen Osteoblasten und Osteoklasten kann es zu Knochen-assoziierten Krankheiten wie Osteoporose oder Osteopetrose kommen (Helfrich MH, 2003; Sambrook P und Cooper C, 2006). Osteoklasten sind multinukleäre Zellen, die in der Lage sind die Knochenmatrix zu resorbieren (Teitelbaum SL, 2000). Sie entstehen aus pluripotenten, hämatopoetischen Stammzellen durch Differenzierung und Zellfusion von Monozyten/Makrophagen-Vorläuferzellen (Menaa C et al., 2000, Yavropoulou MP und Yovos JG, 2008). Die Osteoklasten-Differenzierung wird hauptsächlich durch die Zytokine M-CSF (macrophage colony stimulating factor) und RANKL (receptor activator of nuclear factor k b ligand) induziert. Sie initiieren ein spezifisches Expressionsmuster Osteoklasten-spezifischer Gene und aktivieren die Zellfusion in Osteoklasten-Vorläuferzellen zur Bildung reifer Osteoklasten (Boyle WJ et al., 2003; Asagiri M und Takayanagi H, 2007). Die RANKL-vermittelte Induktion der Osteoklastogenese beruht auf der Initiierung eines streng regulierten Netzwerks aus Transkriptionsfaktoren (Yang X und Karsenty G, 2002). Einige Transkriptionsfaktoren, die während der Osteoklasten-Differenzierung induziert und exprimiert werden, sind nicht auf Osteoklasten beschränkt. Sie erfüllen auch Aufgaben in anderen hämatopoetischen Differenzierungsprozessen (Engel I und Murre C et al., 1999), so dass vermutlich die Kombination der Transkriptionsfaktoren entscheidend für die Osteoklastogenese ist.
Der basic helix-loop-helix-Transkriptionsfaktor Tal1 (T-cell acute lymphocytic leukemia 1, auch Scl1, stem cell leukemia 1) ist ein entscheidender Faktor in der primitiven und der definitiven Hämatopoese (Bloor AJ et al., 2002; Shivdasani RA et al., 1996). Die Expression von Tal1 konnte bisher in verschiedenen hämatopoetischen Zelllinien gezeigt werden, u.a. in monozytischen Zellen (Elefanty AG et al., 1998; Green AR et al., 1992; Pulford K et al., 1995; Dey S et al., 2010).
In der vorliegenden Arbeit wurde der Einfluss des Transkriptionsfaktors Tal1 in Monozyten und reifen Osteoklasten, vor allem in Bezug auf genregulatorische Prozesse während der Osteoklasten-Differenzierung, untersucht. Der Transkriptionsfaktor Tal1 wird in vitro und in vivo in Osteoklasten-Vorläuferzellen und reifen Osteoklasten exprimiert. Die Proteinexpression von Tal1 wird durch die Inkubation der Zellen mit RANKL induziert, jedoch wurde dies in Bezug auf die mRNA-Expression von Tal1 nicht beobachtet, so dass vermutlich eine posttranskriptionelle Regulation von Tal1 vorliegt.
Die Überexpression von Tal1 sorgte für eine Blockade der Differenzierung von Osteoklasten-Vorläuferzellen in reife Osteoklasten. Der Verlust von Tal1 in primären Monozyten/Makrophagen-Zellen führte zur veränderten Expression von über 1200 Genen, wobei jeweils etwa 600 Gene herauf- bzw. herabreguliert waren. Dies verdeutlicht, dass Tal1 sowohl an der Aktivierung als auch an der Reprimierung der Genexpression in Osteoklasten-Vorläuferzellen beteiligt ist. Die Liste der herabregulierten Gene beinhaltete u.a. das Osteoklasten-spezifische Enzym Acp5 (auch TRAP, tartrate resistant acid phosphatase), die Liste der herauf regulierten Gene beinhaltete u.a. DC-STAMP (dendritic cell specific transmembrane protein) und ATP6V0D2 (d2 isoform of vascuolar ATPase V0 domain), beide werden im Zusammenhang mit der Zellfusion während der Osteoklasten-Differenzierung beschrieben (Kim K et al., 2008; Kim T et al., 2010; Yagi M et al., 2005). Der Promotor von DC-STAMP beinhaltet mehrere potentielle Bindestellen für Tal1 und Osteoklastenspezifische Transkriptionsfaktoren. Es konnte gezeigt werden, dass Tal1, PU.1 und MITF im Bereich um 343 bp vor dem Transkriptionsstartpunkt des DC-STAMP-Promotors binden und dass Tal1 mit den Osteoklasten-spezifischen Transkriptionsfaktoren PU.1 und MITF interagiert. Der inhibitorische Effekt von Tal1 auf die Osteoklasten-Differenzierung kommt durch die Reprimierung der Aktivität der Osteoklasten-spezifischen Transkriptionsfaktoren PU.1 und MITF auf dem DC-STAMP-Promotor in Osteoklasten-Vorläuferzellen zustande. Während der Osteoklastogenese kommt es zu einer verringerten Tal1-Bindung auf dem DCSTAMP-Promotor, wodurch die Tal1-vermittelte Inhibierung der Expression aufgehoben wird.
Die Bindung von PU.1 und MITF auf dem Promotor von DC-STAMP nimmt während der Osteoklasten-Differenzierung zu. Die Expression von DC-STAMP wird im Verlauf der Osteoklastogenese induziert, wodurch es zur Zell-Zell-Fusion kommt.
Die Analyse des transkriptionellen Netzwerks, das die Fusion mononukleärer Zellen in reife Osteoklasten reguliert, vertieft das molekulare Verständnis der Osteoklasten-Differenzierung und kann zur Entwicklung neuer therapeutischer Ansätze beitragen, die in der Behandlung von Osteoporose, Riesenzelltumoren und anderen Osteoklastenassoziierten Krankheiten verwendet werden können.
For millennia, rural West African communities living in or adjacent of savanna ecosystems have been collecting components of local plant species (e.g. fruits, leaves, bark) in order to fulfil essential household subsistence needs (alimentation, medical care, energy demand etc.), to generate cash income and to overcome times of (financial) crisis. Thus, these non-timber forest products (NTFPs) make a considerable contribution to the well-being of local households. However, climate and land use change severely impact West African savanna ecosystems and, consequently, the safe-guarding of dependent rural livelihoods. The conversion of savanna area into cultivated land for subsistence farming owing to the ongoing population growth, as well as the progressive promotion of cash crops (e.g. cotton) is ever-increasing. As a consequence, present land-use management in West Africa has to cope with serious trade-offs. Within this decision-making NTFPs have been constantly understated due to a lack of appropriate economic figures to use within common cost-benefit analysis, and, thus, have been frequently outcompeted by seemingly more profitable land-use options. Therefore, it is crucial to provide appropriate economic data for NTFPs in order to create positive incentives for both decision-makers and NTFP beneficiaries to conserve NTFP-providing trees. The key finding of this analysis is that income from NTFPs accounts for 39 % on average of an annual total household income in Northern Benin, representing the second largest income share next to crop income and proving the respective households to be economically heavily dependent on NTFPs. Thereby, socio-economic characteristics of NTFP users tremendously shape their preferences for woody species. Particularly ethnicity has a major impact on the species used and the economic return obtained by them. Moreover, the study investigated the impacts of climate and land use change on the economic benefits derived from the three economically most important tree species in the region Vitellaria paradoxa, Parkia biglobosa and Adansonia digitata in 2050: Environmental changes will have primarily negative effects on the economic returns from all the three species. At large, the study underpins the economic relevance of NTFPs for rural communities in West African savannas and, consequently, the necessity to appropriately sustain them in order to safe-guard local livelihoods. Providing key figures on the current and future economic benefits obtained from NTFPs can augment common cost-benefit analysis, and, delivering detailed information about peoples’ use preferences for local species, this study clearly contributes to improve the basis of decision-making with reference to local land-use policies.
Background: Many disabling human retinal disorders involve the central retina, particularly the macula. However, the commonly used rodent models in research, mouse and rat, do not possess a macula. The purpose of this study was to identify small laboratory rodents with a significant central region as potential new models for macular research.
Methodology/Principal Findings: Gerbillus perpallidus, Meriones unguiculatus and Phodopus campbelli, laboratory rodents less commonly used in retinal research, were subjected to confocal scanning laser ophthalmoscopy (cSLO), fluorescein and indocyanine green angiography, and spectral-domain optical coherence tomography (SD-OCT) using standard equipment (Heidelberg Engineering HRA1 and Spectralis™) adapted to small rodent eyes. The existence of a visual streak-like pattern was assessed on the basis of vascular topography, retinal thickness, and the topography of retinal ganglion cells and cone photoreceptors. All three species examined showed evidence of a significant horizontal streak-like specialization. cSLO angiography and retinal wholemounts revealed that superficial retinal blood vessels typically ramify and narrow into a sparse capillary net at the border of the respective area located dorsal to the optic nerve. Similar to the macular region, there was an absence of larger blood vessels in the streak region. Furthermore, the thickness of the photoreceptor layer and the population density of neurons in the ganglion cell layer were markedly increased in the visual streak region.
Conclusions/Significance: The retinal specializations of Gerbillus perpallidus, Meriones unguiculatus and Phodopus campbelli resemble features of the primate macula. Hence, the rodents reported here may serve to study aspects of macular development and diseases like age-related macular degeneration and diabetic macular edema, and the preclinical assessment of therapeutic strategies.
Background: Human primary monocytes are refractory to infection with the human immunodeficiency virus 1 (HIV-1) or transduction with HIV-1-derived vectors. In contrast, efficient single round transduction of monocytes is mediated by vectors derived from simian immunodeficiency virus of sooty mangabeys (SIVsmmPBj), depending on the presence of the viral accessory protein Vpx.
Methods and Findings: Here we analyzed whether Vpx of SIVsmmPBj is sufficient for transduction of primary monocytes by HIV-1-derived vectors. To enable incorporation of PBj Vpx into HIV-1 vector particles, a HA-Vpr/Vpx fusion protein was generated. Supplementation of HIV-1 vector particles with this fusion protein was not sufficient to facilitate transduction of human monocytes. However, monocyte transduction with HIV-1-derived vectors was significantly enhanced after delivery of Vpx proteins by virus-like particles (VLPs) derived from SIVsmmPBj. Moreover, pre-incubation with Vpx-containing VLPs restored replication capacity of infectious HIV-1 in human monocytes. In monocytes of non-human primates, single-round transduction with HIV-1 vectors was enabled.
Conclusion: Vpx enhances transduction of primary human and even non-human monocytes with HIV-1-derived vectors, only if delivered in the background of SIVsmmPBj-derived virus-like particles. Thus, for accurate Vpx function the presence of SIVsmmPBj capsid proteins might be required. Vpx is essential to overcome a block of early infection steps in primary monocytes.
Synthesis of acetate from carbon dioxide and molecular hydrogen is considered to be the first carbon assimilation pathway on earth. It combines carbon dioxide fixation into acetyl-CoA with the production of ATP via an energized cell membrane. How the pathway is coupled with the net synthesis of ATP has been an enigma. The anaerobic, acetogenic bacterium Acetobacterium woodii uses an ancient version of this pathway without cytochromes and quinones. It generates a sodium ion potential across the cell membrane by the sodium-motive ferredoxin:NAD oxidoreductase (Rnf). The genome sequence of A. woodii solves the enigma: it uncovers Rnf as the only ion-motive enzyme coupled to the pathway and unravels a metabolism designed to produce reduced ferredoxin and overcome energetic barriers by virtue of electron-bifurcating, soluble enzymes.
Activation of Notch1 signaling in neural progenitor cells (NPCs) induces self-renewal and inhibits neurogenesis. Upon neuronal differentiation, NPCs overcome this inhibition, express proneural genes to induce Notch ligands, and activate Notch1 in neighboring NPCs. The molecular mechanism that coordinates Notch1 inactivation with initiation of neurogenesis remains elusive. Here, we provide evidence that Prox1, a transcription repressor and downstream target of proneural genes, counteracts Notch1 signaling via direct suppression of Notch1 gene expression. By expression studies in the developing spinal cord of chick and mouse embryo, we showed that Prox1 is limited to neuronal precursors residing between the Notch1+ NPCs and post-mitotic neurons. Physiological levels of Prox1 in this tissue are sufficient to allow binding at Notch1 promoter and they are critical for proper Notch1 transcriptional regulation in vivo. Gain-of-function studies in the chick neural tube and mouse NPCs suggest that Prox1-mediated suppression of Notch1 relieves its inhibition on neurogenesis and allows NPCs to exit the cell cycle and differentiate. Moreover, loss-of-function in the chick neural tube shows that Prox1 is necessary for suppression of Notch1 outside the ventricular zone, inhibition of active Notch signaling, down-regulation of NPC markers, and completion of neuronal differentiation program. Together these data suggest that Prox1 inhibits Notch1 gene expression to control the balance between NPC self-renewal and neuronal differentiation.