Refine
Year of publication
Document Type
- Article (1155)
- Doctoral Thesis (836)
- Preprint (76)
- Book (59)
- Contribution to a Periodical (44)
- Conference Proceeding (10)
- Diploma Thesis (10)
- Review (8)
- diplomthesis (4)
- Report (3)
Has Fulltext
- yes (2206)
Is part of the Bibliography
- no (2206)
Keywords
- Podospora anserina (17)
- aging (17)
- mitochondria (12)
- Saccharomyces cerevisiae (10)
- autophagy (10)
- Archaea (9)
- Haloferax volcanii (9)
- Phylogeny (8)
- climate change (8)
- gene expression (8)
Institute
- Biowissenschaften (2206) (remove)
Cryptochromes are a ubiquitous group of blue-light absorbing flavoproteins that in the mammalian retina have an important role in the circadian clock. In birds, cryptochrome 1a (Cry1a), localized in the UV/violet-sensitive S1 cone photoreceptors, is proposed to be the retinal receptor molecule of the light-dependent magnetic compass. The retinal localization of mammalian Cry1, homologue to avian Cry1a, is unknown and it is open whether mammalian Cry1 is also involved in magnetic field sensing. To constrain the possible role of retinal Cry1, we immunohistochemically analysed 90 mammalian species across 48 families in 16 orders, using an antiserum against the Cry1 C-terminus that in birds labels only the photo-activated conformation. In the Carnivora families Canidae, Mustelidae and Ursidae and in some Primates, Cry1 was consistently labeled in the outer segment of the shortwave-sensitive S1 cones. This finding would be compatible with a magnetoreceptive function of Cry1 in these taxa. In all other taxa, Cry1 was not detected by the antiserum that likely also in mammals labels the photo-activated conformation, although Western blots showed Cry1 in mouse retinal cell nuclei. We speculate that in the mouse and the other negative-tested mammals Cry1 is involved in circadian functions as a non-light-responsive protein.
Correction to: Scientific Reports https://doi.org/10.1038/srep21848, published online 22 February 2016
This Article contains an error. Among the studied species, the orangutan was erroneously specified as Bornean orangutan Pongo pygmaeus. In fact, the studied individual was a Sumatran orangutan Pongo abelii.
Background: The Radical-Pair-Model postulates that the reception of magnetic compass directions in birds is based on spin-chemical reactions in specialized photopigments in the eye, with cryptochromes discussed as candidate molecules. But so far, the exact subcellular characterization of these molecules in the retina remained unknown. Methodology/Principal Findings: We here describe the localization of cryptochrome 1a (Cry1a) in the retina of European robins, Erithacus rubecula, and domestic chickens, Gallus gallus, two species that have been shown to use the magnetic field for compass orientation. In both species, Cry1a is present exclusively in the ultraviolet/violet (UV/V) cones that are distributed across the entire retina. Electron microscopy shows Cry1a in ordered bands along the membrane discs of the outer segment, and cell fractionation reveals Cry1a in the membrane fraction, suggesting the possibility that Cry1a is anchored along membranes. Conclusions/Significance: We provide first structural evidence that Cry1a occurs within a sensory structure arranged in a way that fulfils essential requirements of the Radical-Pair-Model. Our findings, identifying the UV/V-cones as probable magnetoreceptors, support the assumption that Cry1a is indeed the receptor molecule mediating information on magnetic directions, and thus provide the Radical-Pair-Model with a profound histological background.
Es gibt für die Orientierung von Vögel ein allgemeingültiges Konzept, das Karte-Kompass-Prinzip (Kramer 1953, 1957): Der Karten-Schritt besteht darin, den eigenen Standort zu ermitteln und mit dem Ziel in Beziehung zu setzten. Damit wird die geografische Richtung bestimmt, die im Kompass-Schritt in eine konkrete Richtung umgesetzt wird. Für Beides nutzen Vögel auch das Magnetfeld der Erde; in der Karte als einen Faktor den Verlauf der Intensität, im Magnetkompass die Achse der Feldlinien. Der Magnetrezeptor, der die Karte mit Informationen versorgt, ist im Schnabel lokalisiert, der des Kompasses im Auge. Ich habe mich in meiner Arbeit darauf konzentriert, die zwei potenziellen Magnetrezeptoren der Vögel feinstrukturell und immunhistologisch weiter zu charakterisieren.
Für den Magnetkompass wird auf Grund des Radikalpaar-Modells angenommen, dass Cryptochrome die Rezeptormoleküle sein könnten (Ritz et al. 2000). Bei Vögeln sind vier Cryptochrome bekannt, allerdings muss das Rezeptormolekül des Magnetkompasses auch in seiner Lokalisation bestimmte Kriterien erfüllen. Die für meine Arbeit bedeutsamen Kriterien sind: (1) die gleiche Ausrichtung der Proteine in einer Rezeptorzelle und (2), dass die einzelnen Rezeptorzellen alle Raumrichtungen abdecken. Ich habe in meiner Arbeit Cryptochrom 1a (Cry1a) und Cryptochrom 1b (Cry1b) auf ihr Vorkommen in der Retina von Rotkehlchen (Erithacus rubecula) und Hühnern (Gallus gallus) untersucht. Cry1b befindet sich bei Rotkehlchen während der Zugzeit in den Ganglienzellen, in denen es teilweise an Membranen gebunden vorliegt, die jedoch keine bevorzugte Richtung haben. Somit erscheint mir Cry1b als Rezeptormolekül für den Magnetkompass als eher ungeeignet. Cry1b könnte, wie viele Cryptochrome, an der Steuerung von circadianen Rhythmen beteiligt sein. Cry1a hingegen ist bei beiden untersuchten Vogelarten in den UV/V-Zapfen an die Diskmembranen gebunden, was eine Ausrichtung ermöglicht. Die UV/V-Zapfen sind über die gesamte Retina gleichmäßig verteilt, und durch die sphärische Form des Auges decken die einzelnen Rezeptoren jede Raumrichtung ab. Somit erfüllt Cry1a die Bedingungen des Radikalpaar-Modells, und ich schließe daraus, dass es sich hierbei um das Rezeptormolekül des Magnetkompasses handeln könnte. Cry1a ändert nach Lichtabsorption wie viele Cryptochrome seine Konformation. Der von mir verwendete Antikörper bindet nur die lichtaktivierte Form des Proteins. In Versuchen, in denen Hühner verschiedenen monochromatischen Lichtern ausgesetzt wurden, zeigt sich, dass sich Cry1a in UV bis Gelb in lichtaktiviertem Zustand befindet. Dies stimmt sowohl mit der spektralen Empfindlichkeit des Magnetkompasses der Vögel als auch mit der des Flavins, des lichtsensitiven Teils des Cryptochroms, überein. Versuche mit grünem Licht lassen vorsichtige Rückschlüsse auf das für den Magnetkompass relevante Radikalpaar zu: so ist das Flavin erst im zweiten Oxidationsschritt grünlicht-sensitiv, und Cry1a ist nur nachweisbar, also lichtaktiviert, wenn der erste Schritt bereits im Hellen abgelaufen ist. Versuche in denen die Tiere vorab im Dunkeln waren, führen nicht zur erneuten Lichtaktivierung unter grünem Licht. Dies macht nur eines der beiden im Flavinzyklus entstehenden Radikalpaare wahrscheinlich, nämlich das in der Reoxidation entstehende, da das Radikalpaar im ersten Schritt der Oxidation unter Grün nicht entsteht.
In Bezug auf den Magnetrezeptor im Schnabel konnte bereits bei Tauben eine detaillierte Struktur beschrieben werden, die als Magnetrezeptor geeignet ist, nämlich Magnetit- bzw. Maghemit-Teilchen in Dendriten der Nerven (Fleissner et al. 2003). Auch Hühner haben eisenhaltige Strukturen im Oberschnabel, die in ihrer Eisenoxid-Zusammensetzung denen der Tauben entsprechen (Falkenberg et al. 2010). Ich konnte in meiner Arbeit zeigen, dass die eisenhaltigen Strukturen im Oberschnabel der adulten Hühner an oder in Nervenfasern liegen. Elektronenoptisch bestehen diese eisenhaltigen Strukturen im Nervengewebe bei Hühnern, wie bei Tauben beschrieben, aus einem 3-5 µm großen Vesikel, der von eisenhaltigen ‘Schuppen’ besetzt ist, aus circa 1 µm langen Plättchen und Kugeln mit einem Durchmesser von etwa 1 µm. Sie sind in Feldern angeordnet, in denen diese Zellstrukturen gleich ausgerichtet sind. In der Anzahl und Lokalisation der Felder der eisenhaltigen Dendriten gibt es Unterschiede zwischen Hühnern und Tauben, allerdings ist unklar, inwie¬weit dies zu Unterschieden in der Verarbeitung im Gehirn führt. Die Entwicklung der eisenhaltigen Dendriten der Hühner beginnt erst nach dem Schlupf, am Tag des Schlupfes haben Küken noch keine eisenhaltigen Strukturen, abgesehen von roten Blutkörperchen. In den ersten 5 Tagen werden eisenhaltige Makrophagen im frontalen Bereich des Schnabels gebildet, die anschließend wieder reduziert werden. Bei 12 Tage alten Hühnern werden diese auch im lateralen Bereich des Oberschnabels angelegt und ebenfalls dort bis Tag 21 wieder reduziert. 21 Tage alte Hühner haben nur noch wenige eisenhaltige Makrophagen, allerdings ein erstes Feld von eisenhaltigen Dendriten. Die Röntgenabsorption zeigt einen Unterschied in der Eisenoxid-Zusammensetzung zwischen eisenhaltigen Makrophagen und eisenhaltigen Dendriten. Es könnte sein, dass die eisenhaltigen Makrophagen an der Synthese der eisenhaltigen Dendriten beteiligt sind, da sie Eisen aufnehmen, aber auch wieder abgeben können und in demselben Zeitraum reduziert werden, wie die eisenhaltigen Dendriten aufgebaut werden.
Sowohl Tauben als auch Rotkehlchen haben sich phylogenetisch bereits vor 95 Millionen Jahren von den Hühnern abgespalten. Es gibt sowohl in der Lokalisation von Cry1a als auch in der Struktur der einzelnen eisenhaltigen Dendriten keine Unterschiede, so dass es sich bei den beiden Magnetrezeptoren der Vögel vermutlich um sehr alte Mechanismen handelt, die sich in der Evolution kaum verändert haben. Vermutlich sind sie vogelspezifisch, da es in dieser Hinsicht keine erkennbare Gemeinsamkeit mit anderen Wirbeltieren gibt.
Iron is part of many redox and other enzymes and, thus, it is essential for all living beings. Many oxic environments have extremely low concentrations of free iron. Therefore, many prokaryotic species evolved siderophores, i.e., small organic molecules that complex Fe3+ with very high affinity. Siderophores of bacteria are intensely studied, in contrast to those of archaea. The haloarchaeon Haloferax volcanii contains a gene cluster that putatively encodes siderophore biosynthesis genes, including four iron uptake chelate (iuc) genes. Underscoring this hypothesis, Northern blot analyses revealed that a hexacistronic transcript is generated that is highly induced under iron starvation. A quadruple iuc deletion mutant was generated, which had a growth defect solely at very low concentrations of Fe3+, not Fe2+. Two experimental approaches showed that the wild type produced and exported an Fe3+-specific siderophore under low iron concentrations, in contrast to the iuc deletion mutant. Bioinformatic analyses revealed that haloarchaea obtained the gene cluster by lateral transfer from bacteria and enabled the prediction of enzymatic functions of all six gene products. Notably, a biosynthetic pathway is proposed that starts with aspartic acid, uses several group donors and citrate, and leads to the hydroxamate siderophore Schizokinen.
The immune suppressive microenvironment affects efficacy of radio-immunotherapy in brain metastasis
(2021)
The tumor microenvironment in brain metastases is characterized by high myeloid cell content associated with immune suppressive and cancer-permissive functions. Moreover, brain metastases induce the recruitment of lymphocytes. Despite their presence, T-cell-directed therapies fail to elicit effective anti-tumor immune responses. Here, we seek to evaluate the applicability of radio- immunotherapy to modulate tumor immunity and overcome inhibitory effects that diminish anti-cancer activity. Radiotherapy- induced immune modulation resulted in an increase in cytotoxic T-cell numbers and prevented the induction of lymphocyte-mediated immune suppression. Radio-immunotherapy led to significantly improved tumor control with prolonged median survival in experi- mental breast-to-brain metastasis. However, long-term efficacy was not observed. Recurrent brain metastases showed accumula- tion of blood-borne PD-L1+ myeloid cells after radio-immunother- apy indicating the establishment of an immune suppressive environment to counteract re-activated T-cell responses. This finding was further supported by transcriptional analyses indicat- ing a crucial role for monocyte-derived macrophages in mediating immune suppression and regulating T-cell function. Therefore, selective targeting of immune suppressive functions of myeloid cells is expected to be critical for improved therapeutic efficacy of radio-immunotherapy in brain metastases.
Reticulate evolution is considered to be among the main mechanisms of plant evolution, often leading to the establishment of new species. However, complex evolutionary scenarios result in a challenging definition of evolutionary and taxonomic units. In this study, we aimed to examine the evolutionary origin and revise the species status of Campanula baumgartenii, a rare endemic species from the polyploid complex Campanula section Heterophylla. Morphometry, flow cytometric ploidy estimation, amplified fragment length polymorphisms (AFLPs), as well as chloroplast and nuclear DNA sequence markers were used to assess the morphological and genetic differentiation among C. baumgartenii, Campanula rotundifolia and other closely related taxa. Tetra- and hexaploid C. baumgartenii is morphologically and molecularly (AFLP) differentiated from sympatric C. rotundifolia. Contrasting signals from nuclear (ITS) and chloroplast (trnL-rpl32) markers suggest a hybrid origin of C. baumgartenii with C. rotundifolia and a taxon related to the alpine Campanula scheuchzeri as ancestors. Additionally, hexaploid C. baumgartenii currently hybridizes with co-occurring tetraploid C. rotundifolia resulting in pentaploid hybrids, for which C. baumgartenii serves as both seed and pollen donor. Based on the molecular and morphological differentiation, we propose to keep C. baumgartenii as a separate species. This study exemplifies that detailed population genetic studies can provide a solid basis for taxonomic delimitation within Campanula section Heterophylla as well as for sound identification of conservation targets.
Iron uptake is an essential process in all Gram-negative bacteria including cyanobacteria and therefore different transport systems evolved during evolution. In cyanobacteria, however, the iron demand is higher than in proteobacteria due to the function of iron as cofactor in e.g. photosynthesis and nitrogen fixation. Most of the transport systems depend on outer membrane localized TonB-dependent transporters (TBDTs), a periplasma-facing TonB protein and a plasma membrane localized machinery (ExbBD). So far, iron chelators (siderophores), oligosaccharides and polypeptides have been identified as substrates of TBDTs. However, in proteobacteria TonB-dependent outer membrane transporter represent a well-explored subject whereas for cyanobacteria almost nothing is known about possible TonB-dependent uptake systems for iron or other substrates. The heterocyst-forming filamentous cyanobacterium Anabaena sp. PCC 7120 is known to secrete the siderophore schizokinen, but its transport system has remained unidentified. For Anabaena sp. PCC 7120 22 genes were identified as putative TBDTs covering almost all known TBDT subclasses. This is a high number of TBDTs compared to other cyanobacteria. The expression of the 22 putative TBDTs individually depends on the presence of iron, copper or nitrogen. The atypical dependence of TBDT gene expression on different nutrition points to a yet unknown regulatory mechanism. In addition, the hypothesis of the absence of TonB in Anabaena sp. PCC 7120 was clarified by the identification of an according sequence, all5036. Inspection of the genome of Anabaena sp. PCC 7120 shows that only one gene encoding a putative TonB-dependent iron transporter, namely alr0397, is positioned close to genes encoding enzymes involved in the biosynthesis of a hydroxamate siderophore. The expression of alr0397 was elevated under iron-limited conditions. Inactivation of this gene caused a moderate phenotype of iron starvation in the mutant cells. The characterization of the mutant strain showed that Alr0397 is a TonB-dependent schizokinen transporter (SchT) of the outer membrane and that alr0397 expression and schizokinen production are regulated by the iron homeostasis of the cell. Additional two genes of Anabaena sp. PCC 7120 involved in this process were identified. SchE encoded by all4025 is a putative cytoplasmic membrane-localized transporter involved in TolC-dependent siderophore secretion. The mutation of schE resulted in an enhanced sensitivity to high metal concentrations and in drastically reduction of secretion of hydroxamate-type siderophores. IacT coded by all4026 is a predicted outer membrane-localized TonB-dependent iron transporter. Inactivation of iacT resulted in reduced sensitivity to elevated iron and copper levels, whereas decoupling the expression from putative regulation by exchange of the promoter resulted in sensitization against tested metals. Further analysis showed that iron and copper effects are synergistic because decrease of iron induced a significant decrease of copper levels in the iacT insertion mutant but an increase of those levels in Anabaena sp. PCC 7120 where expression of all4026 is under the trc-promoter. In consequence, the results unravel a link between iron and copper homeostasis.
Brain development is a complex and highly organized process that relies on the coordinated interaction between neurons and vessels. These cell systems form a neurovascular link that involves the exchange of oxygen, ions, and other physiological components necessary for proper neuronal and vascular function. This physiologically coupled process is executed through analogous structural and molecular signaling mechanisms shared by both cell types. At the neurovascular interface, the cellular crosstalk via these shared signaling mechanisms allows for the synchronized expansion and integration of neurons and vessels into complex cellular networks. This study investigated the role of VEGFR2, a receptor for vascular endothelial growth factor (VEGF), during postnatal neuronal development in the mouse hippocampus. Prior studies have revealed physiological roles of VEGF, a pro-angiogenic morphogen, in nervous system development. However, it was unclear if VEGF signaling had a direct effect on neuronal physiology and function through neuronal-expressing receptors. In this investigative work, we identified a previously unknown function of VEGFR2, whereby VEGF-induced signaling coordinates the development and circuitry integration of CA3 pyramidal neurons in the early postnatal mouse hippocampus. Mechanistically, we found that VEGFR2 signaling requires receptor endocytosis, a process mediated by ephrinB2. We also found that VEGF-induced cooperative signaling between VEGFR2 and ephrinB2 is functionally required for the dendritic arborization and spine maturation of developing CA3 neurons during the first few postnatal weeks. Moreover, in a collaborative effort with the research group of Carmen Ruiz de Almodovar, formerly at the University of Heidelberg, we simultaneously studied VEGF-induced VEGFR2 signaling in CA3 axonal development. Together, we aimed to gain a comprehensive understanding of the complex interplay between VEGF and VEGFR2 signaling during the early postnatal development of CA3 neurons. Ruiz de Almodovar’s research group found that, unlike the branch and spine development of CA3 dendrites, VEGF-VEGFR2 signaling promotes axonal development through mechanisms that are independent of ephrinB2 function. Our findings on CA3 dendritic development are reported in the published manuscript, Harde et al. (2019), and the complementary work on CA3 axonal development from Ruiz de Almodovar's group is presented in the co-published manuscript, Luck et al. (2019). Although the totality of Ruiz de Almodovar's group's work on CA3 axons is not fully discussed here, it is referenced where noted to provide biological context for our findings on CA3 dendritic development.
VEGFR2 signaling within neurovascular niches is known to play a role in the neurogenesis of neural progenitor cells during embryonic development and within the adult brain. However, the precise localization of neuronal VEGFR2 expression and functional role within the nervous system during postnatal brain development was unknown. To investigate this, we used immunohistochemistry to identify the spatial expression of VEGFR2 within the mouse hippocampus during the first few weeks after birth. Our results showed that VEGFR2 was predominantly expressed within the hippocampal vasculature, consistent with prior studies. However, we also observed localized VEGFR2 expression in pyramidal cell neurons of the hippocampal CA3 region by postnatal day 10 (P10). This spatially restricted postnatal expression of VEGFR2 in CA3 neurons suggested a potential role in the development of these neurons during this developmental stage.
The first two weeks after birth in the mouse hippocampus is a critical period for the development of neuronal circuits, as neurons undergo extensive dendritic arborization and spine formation. To explore the role of VEGFR2 in the postnatal nervous system, we used a Nes-cre VEGFR2lox/- mouse line to target the deletion of VEGFR2 expression within the nervous system while preserving normal receptor expression in all other cell types. We also generated corresponding control mice that were negative for Nes-cre. By breeding these mice with Thy1-GFP reporter mice, we could analyze the functional consequences of VEGFR2 by assessing the morphologies of CA3 dendritic trees and spine density and maturation at P10 and P15, respectively. Our analysis showed that CA3 neurons in Nes-cre VEGFR2lox/- mice had less complex dendritic arbors compared to control mice. There were significant reductions in total length and branch points, particularly in areas located 100-250 μm from the cell soma within the stratum radiatum layer. Additionally, Nes-cre VEGFR2lox/- mice exhibited a significant decrease in spine density accompanied by an increased proportion of immature spines. These findings suggest that VEGFR2 plays a crucial role in the proper development of CA3 dendrites and spines during the early postnatal weeks.
Lipopolysaccharide (LPS) is a major glycolipid component in the outer leaflet of the outer membrane of Gram-negative bacteria and known as endotoxin exhibited by the lipid A moiety, which serves as a membrane anchor. The effective permeability barrier properties of the outer membrane contributed by the presence of LPS in the extracellular layer of the outer membrane confer Gram-negative bacteria a high resistance against hydrophobic compounds such as antibiotics, bile salts and detergents to survive in harsh environments. The biogenesis of LPS is well studied in Escherichia coli (herewith E. coli) and the LPS transport (Lpt) is carried out by a transenvelope complex composed of seven essential proteins (LptABCDEFG), which are located in the three compartments of the cell such as the outer membrane, the inner membrane and the periplasm. The Lpt system also exists in Anabaena sp. PCC 7120 (herewith Anabaena sp.), however, homologues of LptC and LptE are still missing. BLAST search failed to identify a homologue of LptC, in contrast, the secondary structure analysis using the Pfam database based on the existing ecLptC secondary structure identified one open reading frame All0231 as the putative Anabaena sp. homologue of LptC, which is designated anaLptC. Despite the low sequence similarity, the secondary structure alignment between anaLptC and ecLptC using the HHpred server showed that both proteins share high secondary structural similarities. The genotypic analysis of the insertion mutant anaLptC did not identify a fully segregated genome and its phenotypic analysis revealed that it was sensitive against chemicals, suggesting that the analptC gene is essential for the growth of Anabaena sp. and involved in the outer membrane biogenesis. This is further supported by the observation of the small cell phenotype in the anaLptC mutant via transmission electron microscopy. Moreover, physical interactions between the anaLptC periplasmic domain with anaLptA as well as with anaLptF were established, indicating that the anaLptC periplasmic domain is correctly folded and alone functional and that the transmembrane helix is not required for the interaction with anaLptA and anaLptF. Furthermore, the reduction of the O-antigen containing LPS was observed in the insertion mutant anaLptC and the dissociation constant Kd of the anaLptC periplasmic domain for ecLPS was determined.The three-dimensional structure of the periplasmic domain of anaLptC was solved by X-ray crystallography with a resolution of 2.8 Å. The structural superposition between the ecLptC crystal structure (PDB number 3my2) and the crystal structure of anaLptC periplasmic domain obtained by this study showed the similarity in the folding of the two proteins with a Cα r.m.s.d value of about 1 Å and confirmed that the length of anaLptC is more than two times longer than that of ecLptC. The structural comparison also revealed that both structures share the typical β-jellyroll fold and conserved amino acids, which were shown in ecLptC to bind to LPS in vivo and found in anaLptC. Overall, these data strongly suggest that anaLptC is involved in the transport of LPS and support the model whereby the bridge spanning the inner membrane and the outer membrane would be assembled via interactions of the structurally conserved β-jellyroll domains shared by five (LptACDFG) out of seven Lpt proteins.