TY - JOUR A1 - Li, Shan A1 - Li, Xin A1 - Link, Roman A1 - Li, Ren A1 - Deng, Liping A1 - Schuldt, Bernhard A1 - Jiang, Xiaomei A1 - Zhao, Rongjun A1 - Zheng, Jingming A1 - Li, Shuang A1 - Yin, Yafang T1 - Influence of cambial age and axial height on the spatial patterns of xylem traits in Catalpa bungei, a ring-porous tree species native to China JF - Forests N2 - Studying how cambial age and axial height affects wood anatomical traits may improve our understanding of xylem hydraulics, heartwood formation and axial growth. Radial strips were collected from six different heights (0–11.3 m) along the main trunk of three Manchurian catalpa (Catalpa bungei) trees, yielding 88 samples. In total, thirteen wood anatomical vessel and fiber traits were observed usinglight microscopy (LM) and scanning electron microscopy (SEM), and linear models were used to analyse the combined effect of axial height, cambial age and their interaction. Vessel diameter differed by about one order of magnitude between early- and latewood, and increased significantly with both cambial age and axial height in latewood, while it was positively affected by cambial age and independent of height in earlywood. Vertical position further had a positive effect on earlywood vessel density, and negative effects on fibre wall thickness, wall thickness to diameter ratio and length. Cambial age had positive effects on the pit membrane diameter and vessel element length, while the annual diameter growth decreased with both cambial age and axial position. In contrast, early- and latewood fiber diameter were unaffected by both cambial age and axial height. We further observed an increasing amount of tyloses from sapwood to heartwood, accompanied by an increase of warty layers and amorphous deposits on cell walls, bordered pit membranes and pit apertures. This study highlights the significant effects of cambial age and vertical position on xylem anatomical traits, and confirms earlier work that cautions to take into account xylem spatial position when interpreting wood anatomical structures, and thus, xylem hydraulic functioning. KW - wood anatomy KW - vertical and radial variation KW - earlywood KW - latewood KW - growth ring width KW - tyloses KW - pit membrane diameter KW - vessel lumen diameter KW - fibre length Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-196297 SN - 1999-4907 VL - 10 IS - 8 ER - TY - THES A1 - Fröschel, Christian T1 - Genomweite Analyse der zellschichtspezifischen Expression in der Arabidopsis-Wurzel nach Inokulation mit pathogenen und mutualistischen Mikroorganismen T1 - Genome-wide analysis of cell-type specific expressed genes in the Arabidopsis-root after inoculation with pathogenic and mutualistic microorganisms N2 - Obwohl Pflanzenwurzeln mit einer Vielzahl von Pathogenen in Kontakt kommen, sind induzierbare Abwehrreaktionen der Wurzel bisher kaum beschrieben. Aufgrund der konzentrischen Zellschicht-Organisation der Wurzel wird angenommen, dass bei einer Immunantwort in jeder Zellschicht ein spezifisches genetisches Programm aktiviert wird. Eine Überprüfung dieser Hypothese war bisher wegen methodischen Limitierungen nicht möglich. Die zellschichtspezifische Expression Epitop-markierter ribosomaler Proteine erlaubt eine Affinitätsaufreinigung von Ribosomen und der assoziierten mRNA. Diese Methodik, als TRAP (Translating Ribosome Affinity Purification) bezeichnet, ermöglicht die Analyse des Translatoms und wurde dahingehend optimiert, pflanzliche Antworten auf Befall durch bodenbürtige Mikroorganismen in Rhizodermis, Cortex, Endodermis sowie Zentralzylinder spezifisch zu lokalisieren. Die Genexpression in der Arabidopsis-Wurzel nach Inokulation mit drei Bodenorganismen mit unterschiedlichen Lebensweisen wurde vergleichend betrachtet: Piriformospora indica kann als mutualistischer Pilz pflanzliches Wachstum und Erträge positiv beeinflussen, wohingegen der vaskuläre Pilz Verticillium longisporum für erhebliche Verluste im Rapsanbau verantwortlich ist und der hemibiotrophe Oomycet Phytophthora parasitica ein breites Spektrum an Kulturpflanzen befällt und Ernten zerstört. Für die Interaktionsstudien zwischen Arabidopsis und den Mikroorganismen während ihrer biotrophen Lebensphase wurden sterile in vitro-Infektionssysteme etabliert und mittels TRAP und anschließender RNA-Sequenzierung eine zellschichtspezifische, genomweite Translatomanalyse durchgeführt (Inf-TRAP-Seq). Dabei zeigten sich massive Unterschiede in der differentiellen Genexpression zwischen den Zellschichten, was die Hypothese der zellschichtspezifischen Antworten unterstützt. Die Antworten nach Inokulation mit pathogenen bzw. mutualistischen Mikroorganismen unterschieden sich ebenfalls deutlich, was durch die ungleichen Lebensweisen begründbar ist. Durch die Inf-TRAP-Seq Methodik konnte z.B. im Zentralzylinder der Pathogen-infizierten Wurzeln eine expressionelle Repression von positiven Regulatoren des Zellzyklus nachgewiesen werden, dagegen in den mit P. indica besiedelten Wurzeln nicht. Dies korrelierte mit einer Pathogen-induzierten Inhibition des Wurzelwachstums, welche nicht nach Inokulation mit P. indica zu beobachten war. Obwohl keines der drei Mikroorganismen in der Lage ist, den Zentralzylinder direkt zu penetrieren, konnte hier eine differentielle Genexpression detektiert werden. Demzufolge ist ein Signalaustausch zu postulieren, über den äußere und innere Zellschichten miteinander kommunizieren. In der Endodermis konnten Genexpressionsmuster identifiziert werden, die zu einer Verstärkung der Barriere-Funktionen dieser Zellschicht führen. So könnte etwa durch Lignifizierungsprozesse die Ausbreitung der Mikroorganismen begrenzt werden. Alle drei Mikroorganismen lösten besonders im Cortex die Induktion von Genen für die Biosynthese Trp-abhängiger, antimikrobieller Sekundärmetaboliten aus. Die biologische Relevanz dieser Verteilungen kann nun geklärt werden. Zusammenfassend konnten in dieser Dissertation erstmals die durch Mikroorganismen hervorgerufenen zellschichtspezifischen Antworten der pflanzlichen Wurzel aufgelöst werden. Vergleichende bioinformatische Analyse dieses umfangreichen Datensatzes ermöglicht nun, gezielt testbare Hypothesen zu generieren. Ein Verständnis der zellschichtspezifischen Abwehrmaßnahmen der Wurzel ist essentiell für die Entwicklung neuer Strategien zur Ertragssteigerung und zum Schutz von Nutzpflanzen gegen Pathogene in der Landwirtschaft. N2 - Although plant roots are surrounded by a plethora of microorganisms, their interactions are poorly characterized on a molecular level. Due to the concentric organization of the root cell-layers, it is anticipated that these layers contribute to pathogen defense by providing specific genetically defined programs, which build up barriers to restrict infection. Because of methodical limitations, this theory was not confirmed, yet. Immunoprecipitation of cell-layer specific expressed epitope-tagged ribosomes allows an isolation of ribosome/mRNA complexes that subsequently can be analyzed. This approach is called “Translating Ribosome Affinity Purification” (TRAP). It was optimized to identify cell-layer specific induced defenses and to be combined with a system to inoculate plant roots directly with soil-born microorganisms. Hence, this method enables molecular dissection of infected Arabidopsis-roots to unravel expression patterns found in rhizodermis, cortex, endodermis and central cylinder, respectively. Comparative studies were performed with three species of microorganisms having different life-styles: On the one hand the beneficial fungus Piriformospora indica, that can promote plant growth and crop yield and on the other hand two pathogens with the vascular fungus Verticillium longisporum, causing damage in oilseed rape production and the hemibiotrophic Oomycet Phytophthora parasitica, which causes plant damage on many crop plants. After performing TRAP with infected roots, the cell-type specific mRNA was analyzed via RNA-Sequencing resulting in a genome-wide impression of differentially expressed genes (Inf-TRAP-Seq). Massive differences occurred among the cell-layers approving the theory of cell-type specific immune responses. Moreover the defense responses varied according to inoculation with pathogenic or beneficial microorganisms probably due to their life-style. For example by using the newly established Inf-TRAP-Seq approach it was shown that positive regulators of cell proliferation were expressionally repressed in central cylinder of pathogen-infected roots but not in P. indica colonized roots. This correlates with the observation that root growth is suppressed after inoculation with pathogens but not after inoculation with P. indica. Although none of the three microorganisms is able to penetrate the central cylinder, differentially expressed genes were detected in this layer suggesting an exchange of signals to enable communication between inner and outer layers. Expression patterns were identified in the endodermis, that could lead to reinforcement of barrier functions of this cell-layer for example by lignification-processes. By this means the propagation of the microorganisms is restricted. All three microorganisms elicited induction of genes involved in biosynthesis of Trp-derived secondary metabolites, especially in the cortex. Now the biological relevance of these distributions can be investigated additionally. Hence, within this thesis for the first time a cell-type specific resolution was obtained regarding defense responses in the Arabidopsis-root triggered by microorganisms. A huge dataset was generated. This can be analyzed extensively by bioinformatics and its applications to set up new hypotheses, which can be tested by further approaches. An understanding of cell-type defined root defense responses is essential to facilitate new strategies for protecting crop plants against pathogens and to increase crop yield in agriculture. KW - Schmalwand KW - Wurzel KW - Phytophthora KW - Piriformospora indica KW - Verticillium KW - Wurzelzellschichten KW - Zellschichtspezifische Expression KW - Zentralzylinder KW - Cortex KW - Rhizodermis KW - Endodermis KW - cell-type specific KW - Inf-TRAP-Seq Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146439 ER - TY - THES A1 - Glenz, René T1 - Die Rolle von Sphingobasen in der pflanzlichen Zelltodreaktion T1 - The role of sphingobases in plant cell death reaction N2 - Sphingobasen bilden das Grundgerüst und die Ausgangsbausteine für die Biosynthese von Sphingolipiden. Während komplexere Sphingolipide einen wichtigen Bestandteil von eukaryotischen Membranen bilden, sind Sphingobasen, die auch als long-chain bases (LCBs) bezeichnet werden, als Signalmoleküle bei zellulären Prozessen in Eukaryoten bekannt. Im tierischen System wurden antagonistische Effekte von nicht-phosphorylierten Sphingobasen (LCBs) und ihren phosphorylierten Gegenstücken (LCB-Ps) bei vielen Zellfunktionen, insbesondere der Apoptose, nachgewiesen und die zugrundeliegenden Signalwege umfassend aufgeklärt. Im Gegensatz dazu sind in Pflanzen weniger Belege für einen antagonistischen Effekt und mögliche Signaltransduktionsmechanismen bekannt. Für eine regulatorische Funktion von Sphingobasen beim programmierten Zelltod (PCD) in Pflanzen existieren mehrere Hinweise: (I) Mutationen in Genen, die den Sphingobasen-Metabolismus betreffen, führen zum Teil zu spontanem PCD und veränderten Zelltodreaktionen. (II) Die Gehalte von LCBs sind bei verschiedenen Zelltod-auslösenden Bedingungen erhöht. (III) Nekrotrophe Pathogene produzieren Toxine, wie Fumonisin B1 (FB1), die mit dem Sphingolipid-Metabolismus der Wirtspflanze interferieren, was wiederum die Ursache für den dadurch ausgelösten PCD darstellt. (IV) Die Behandlung von Pflanzen mit LCBs, nicht aber mit LCB-Ps, führt zu Zelltod. In dieser Arbeit wurde die Rolle von Sphingobasen in der pflanzlichen Zelltodreaktion untersucht, wobei der Fokus auf der Überprüfung der Hypothese eines antagonistischen, Zelltod-hemmenden Effekts von LCB-Ps lag. Anhand von Leitfähigkeit-basierten Messungen bei Blattscheiben von Arabidopsis thaliana wurde der durch Behandlung mit LCBs und separater oder gleichzeitiger Zugabe von LCB-Ps auftretende Zelltod bestimmt. Mit dieser Art der Quantifizierung wurde der an anderer Stelle publizierte inhibierende Effekt von LCB-Ps auf den LCB-induzierten Zelltod nachgewiesen. Durch parallele Messung der Spiegel der applizierten Sphingobasen im Gewebe mittels HPLC-MS/MS konnte dieser Antagonismus allerdings auf eine reduzierte Aufnahme der LCB bei Anwesenheit der LCB-P zurückgeführt werden, was auch durch eine zeitlich getrennte Behandlung mit den Sphingobasen bestätigt wurde. Darüber hinaus wurde der Einfluss einer exogenen Zugabe von LCBs und LCB-Ps auf den durch Pseudomonas syringae induzierten Zelltod von A. thaliana untersucht. Für LCB-Ps wurde dabei kein Zelltod-hemmender Effekt beobachtet, ebenso wenig wie ein Einfluss von LCB-Ps auf den PCD, der durch rekombinante Expression und Erkennung eines Avirulenzproteins in Arabidopsis ausgelöst wurde. Für LCBs wurde dagegen eine direkte antibakterielle Wirkung im Zuge der Experimente mit P. syringae gezeigt, die den in einer anderen Publikation beschriebenen inhibierenden Effekt von LCBs auf den Pathogen-induzierten Zelltod in Pflanzen relativiert. In weiteren Ansätzen wurden Arabidopsis-Mutanten von Enzymen des Sphingobasen-Metabolismus (LCB-Kinase, LCB-P-Phosphatase, LCB-P-Lyase) hinsichtlich veränderter in-situ-Spiegel von LCBs/LCB-Ps funktionell charakterisiert. Der Phänotyp der Mutanten gegenüber Fumonisin B1 wurde zum einen anhand eines Wachstumstests mit Keimlingen und zum anderen anhand des Zelltods von Blattscheiben bestimmt und die dabei akkumulierenden Sphingobasen quantifiziert. Die Sensitivität der verschiedenen Linien gegenüber FB1 korrelierte eng mit den Spiegeln der LCBs, während hohe Gehalte von LCB-Ps alleine nicht in der Lage waren den Zelltod zu verringern. In einzelnen Mutanten konnte sogar eine Korrelation von stark erhöhten LCB-P-Spiegeln mit einer besonderen Sensitivität gegenüber FB1 festgestellt werden. Die Ergebnisse der vorliegenden Arbeit stellen die Hypothese eines antagonistischen Effekts von phosphorylierten Sphingobasen beim pflanzlichen Zelltod in Frage. Stattdessen konnte in detaillierten Analysen der Sphingobasen-Spiegel die positive Korrelation der Gehalte von LCBs mit dem Zelltod gezeigt werden. Die hier durchgeführten Experimente liefern damit nicht nur weitere Belege für die Zelltod-fördernde Wirkung von nicht-phosphorylierten Sphingobasen, sondern tragen zum Verständnis der Sphingobasen-Homöostase und des Sphingobasen-induzierten PCD in Pflanzen bei. N2 - Sphingobases are the building blocks for the biosynthesis of sphingolipids. While complex sphingolipids form a major part of eukaryotic membranes, sphingobases, which are also called long-chain bases (LCBs), are well-known signaling molecules of cellular processes in eukaryotes. In the animal system, antagonistic effects of nonphosphorylated sphingobases (LCBs) and their phosphorylated counterparts (LCB-Ps) have been reported in many cell functions, with a particular focus on apoptosis, and the underlying signaling pathways have been elucidated in detail. In contrast, few records of an antagonistic effect and the potential signal transduction mechanisms have been established in plants. Several lines of evidence point to a regulatory function of sphingobases in plant programmed cell death (PCD): (i) Mutations in genes related to sphingobase metabolism may cause spontaneous PCD and altered cell death reactions. (ii) Levels of LCBs are increased under different cell death conditions. (iii) Necrotrophic pathogens produce toxins, like fumonisin B1 (FB1), interfering with sphingolipid metabolism of the host plant and, thus, causing PCD. (iv) Treatment of plants with LCBs, but not LCB-Ps, induces cell death. In the present study the role of sphingobases in plant cell death reactions, with a focus on the examination of the hypothesis of an antagonistic cell death-inhibitory effect of LCB-Ps, has been investigated. Using conductivity-based measurements of Arabidopsis thaliana leaf discs, cell death induced by treatment with LCBs and separated or combined feeding of LCB-Ps was determined. That kind of quantification allowed the verification of an inhibitory effect of LCB-Ps on LCB-induced cell death, which was published elsewhere. However, by simultaneous measurement of the applied sphingobase levels in the tissue with HPLC-MS/MS, this antagonism could be explained by a reduced uptake of the LCB in the presence of the LCB-P, which was also confirmed by a separated treatment with the sphingobases. In addition to that an impact of exogenous applied LCBs and LCB-Ps on cell death in A. thaliana induced by Pseudomonas syringae has been investigated. For LCB-Ps no cell death inhibitory effect was observed. Similarly, there was no impact for LCB-Ps on the cell death induced by recombinant expression of an avirulence protein in Arabidopsis. For LCBs, a direct antibacterial effect against P. syringae was shown in this work. This puts previous findings of an inhibitory effect of LCBs on pathogen-induced cell death in plants into a new perspective. In further approaches, Arabidopsis mutants of enzymes of the sphingobase metabolism (LCB kinase, LCB-P phosphatase, LCB-P lyase) were functionally characterized with regard to altered in situ levels of LCBs/LCB-Ps. The phenotype of the mutants in response to fumonisin B1 was determined in a growth assay with seedlings, and by cell death measurements in leaf discs, which were accompanied by quantification of sphingobase levels. The sensitivity of different lines to FB1 was closely correlated with the levels of LCBs, while high contents of LCB-Ps alone were not able to reduce cell death. Some mutants even showed a correlation of highly enhanced LCB-P levels with a pronounced sensitivity to FB1. The results of the present study challenge the hypothesis of an antagonistic effect of phosphorylated sphingobases on plant cell death. Instead, a detailed analysis of sphingobase levels revealed a positive correlation of LCB contents with cell death. The conducted experiments not only provide further evidence for a cell death-promoting effect of nonphosphorylated sphingobases, but also contribute to the comprehension of sphingobase homeostasis, as well as of the sphingobase-induced PCD in plants. KW - Sphingolipide KW - Phytosphingosine KW - Ackerschmalwand KW - Pseudomonas syringae KW - Zelltod KW - Sphingobasen (LCB, LCB-P) KW - Ackerschmalwand KW - programmierter Zelltod KW - Sphingobases KW - Arabidopsis KW - programmed cell death Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-187903 ER - TY - JOUR A1 - Elmaidomy, Abeer H. A1 - Mohammed, Rabab A1 - Hassan, Hossam M. A1 - Owis, Asmaa I. A1 - Rateb, Mostafa E. A1 - Khanfar, Mohammad A. A1 - Krischke, Markus A1 - Mueller, Martin J. A1 - Abdelmohsen, Usama Ramadan T1 - Metabolomic profiling and cytotoxic tetrahydrofurofuran lignans investigations from Premna odorata Blanco JF - Metabolites N2 - Metabolomic profiling of different Premna odorata Blanco (Lamiaceae) organs, bark, wood, young stems, flowers, and fruits dereplicated 20, 20, 10, 20, and 20 compounds, respectively, using LC–HRESIMS. The identified metabolites (1–34) belonged to different chemical classes, including iridoids, flavones, phenyl ethanoids, and lignans. A phytochemical investigation of P. odorata bark afforded one new tetrahydrofurofuran lignan, 4β-hydroxyasarinin 35, along with fourteen known compounds. The structure of the new compound was confirmed using extensive 1D and 2D NMR, and HRESIMS analyses. A cytotoxic investigation of compounds 35–38 against the HL-60, HT-29, and MCF-7 cancer cell lines, using the MTT assay showed that compound 35 had cytotoxic effects against HL-60 and MCF-7 with IC50 values of 2.7 and 4.2 µg/mL, respectively. A pharmacophore map of compounds 35 showed two hydrogen bond acceptor (HBA) aligning the phenoxy oxygen atoms of benzodioxole moieties, two aromatic ring features vectored on the two phenyl rings, one hydrogen bond donor (HBD) feature aligning the central hydroxyl group and thirteen exclusion spheres which limit the boundaries of sterically inaccessible regions of the target’s active site. KW - Premna KW - lignan KW - metabolomic KW - cytotoxic KW - pharmacophore map Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-193187 SN - 2218-1989 VL - 9 IS - 10 ER - TY - JOUR A1 - Duan, Xiaodong A1 - Nagel, Georg A1 - Gao, Shiqiang T1 - Mutated channelrhodopsins with increased sodium and calcium permeability JF - Applied Sciences N2 - (1) Background: After the discovery and application of Chlamydomonas reinhardtii channelrhodopsins, the optogenetic toolbox has been greatly expanded with engineered and newly discovered natural channelrhodopsins. However, channelrhodopsins of higher Ca\(^{2+}\) conductance or more specific ion permeability are in demand. (2) Methods: In this study, we mutated the conserved aspartate of the transmembrane helix 4 (TM4) within Chronos and PsChR and compared them with published ChR2 aspartate mutants. (3) Results: We found that the ChR2 D156H mutant (XXM) showed enhanced Na\(^+\) and Ca\(^{2+}\) conductance, which was not noticed before, while the D156C mutation (XXL) influenced the Na\(^+\) and Ca\(^{2+}\) conductance only slightly. The aspartate to histidine and cysteine mutations of Chronos and PsChR also influenced their photocurrent, ion permeability, kinetics, and light sensitivity. Most interestingly, PsChR D139H showed a much-improved photocurrent, compared to wild type, and even higher Na+ selectivity to H\(^+\) than XXM. PsChR D139H also showed a strongly enhanced Ca\(^{2+}\) conductance, more than two-fold that of the CatCh. (4) Conclusions: We found that mutating the aspartate of the TM4 influences the ion selectivity of channelrhodopsins. With the large photocurrent and enhanced Na\(^+\) selectivity and Ca\(^{2+}\) conductance, XXM and PsChR D139H are promising powerful optogenetic tools, especially for Ca\(^{2+}\) manipulation. KW - optogenetics KW - channelrhodopsins KW - sodium KW - calcium KW - DC gate Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-197435 SN - 2076-3417 VL - 9 IS - 4 ER - TY - THES A1 - Beck, Sebastian T1 - Using optogenetics to influence the circadian clock of \(Drosophila\) \(melanogaster\) T1 - Die Verwendung der Optogenetik zur Beeinflussung der circadianen Uhr von \(Drosophila\) \(melanogaster\) N2 - Almost all life forms on earth have adapted to the most impactful and most predictable recurring change in environmental condition, the cycle of day and night, caused by the axial rotation of the planet. As a result many animals have evolved intricate endogenous clocks, which adapt and synchronize the organisms’ physiology, metabolism and behaviour to the daily change in environmental conditions. The scientific field researching these endogenous clocks is called chronobiology and has steadily grown in size, scope and relevance since the works of the earliest pioneers in the 1960s. The number one model organism for the research of circadian clocks is the fruit fly, Drosophila melanogaster, whose clock serves as the entry point to understanding the basic inner workings of such an intricately constructed endogenous timekeeping system. In this thesis it was attempted to combine the research on the circadian clock with the techniques of optogenetics, a fairly new scientific field, launched by the discovery of Channelrhodopsin 2 just over 15 years ago. Channelrhodopsin 2 is a light-gated ion channel found in the green alga Chlamydomonas reinhardtii. In optogenetics, researches use these light-gated ion channels like Channelrhodopsin 2 by heterologously expressing them in cells and tissues of other organisms, which can then be stimulated by the application of light. This is most useful when studying neurons, as these channels provide an almost non-invasive tool to depolarize the neuronal plasma membranes at will. The goal of this thesis was to develop an optogenetic tool, which would be able to influence and phase shift the circadian clock of Drosophila melanogaster upon illumination. A phase shift is the adaptive response of the circadian clock to an outside stimulus that signals a change in the environmental light cycle. An optogenetic tool, able to influence and phase shift the circadian clock predictably and reliably, would open up many new ways and methods of researching the neuronal network of the clock and which neurons communicate to what extent, ultimately synchronizing the network. The first optogenetic tool to be tested in the circadian clock of Drosophila melanogaster was ChR2-XXL, a channelrhodopsin variant with dramatically increased expression levels and photocurrents combined with a prolonged open state. The specific expression of ChR2-XXL and of later constructs was facilitated by deploying the three different clock-specific GAL4-driver lines, clk856-gal4, pdf-gal4 and mai179-gal4. Although ChR2-XXL was shown to be highly effective at depolarizing neurons, these stimulations proved to be unable to significantly phase shift the circadian clock of Drosophila. The second series of experiments was conducted with the conceptually novel optogenetic tools Olf-bPAC and SthK-bPAC, which respectively combine a cyclic nucleotide-gated ion channel (Olf and SthK) with the light-activated adenylyl-cyclase bPAC. These tools proved to be quite useful when expressed in the motor neurons of instar-3 larvae of Drosophila, paralyzing the larvae upon illumination, as well as affecting body length. This way, these new tools could be precisely characterized, spawning a successfully published research paper, centered around their electrophysiological characterization and their applicability in model organisms like Drosophila. In the circadian clock however, these tools caused substantial damage, producing severe arrhythmicity and anomalies in neuronal development. Using a temperature-sensitive GAL80-line to delay the expression until after the flies had eclosed, yielded no positive results either. The last series of experiments saw the use of another new series of optogenetic tools, modelled after the Olf-bPAC, with bPAC swapped out for CyclOp, a membrane-bound guanylyl-cyclase, coupled with less potent versions of the Olf. This final attempt however also ended up being unsuccessful. While these tools could efficiently depolarize neuronal membranes upon illumination, they were ultimately unable to stimulate the circadian clock in way that would cause it to phase shift. Taken together, these mostly negative results indicate that an optogenetic manipulation of the circadian clock of Drosophila melanogaster is an extremely challenging subject. As light already constitutes the most impactful environmental factor on the circadian clock, the combination of chronobiology with optogenetics demands the parameters of the conducted experiments to be tuned with an extremely high degree of precision, if one hopes to receive positive results from these types of experiments at all. N2 - Nahezu alle Lebewesen der Erde haben sich an den Tag-Nacht-Zyklus angepasst, die einflussreichste und verlässlichste wiederkehrende Veränderung der Umwelt-bedingungen, verursacht durch die axiale Rotation des Planeten. Daraus resultierend haben viele Tiere komplizierte innere Uhren entwickelt, welche ihre Physiologie, ihren Stoffwechsel und ihr Verhalten an die tägliche Veränderung der natürlichen Bedingungen anpassen. Das Wissenschaftsfeld, das sich der Erforschung dieser inneren Uhren widmet, wird Chronobiologie genannt und hat seit der Arbeit der ersten Pioniere ab 1960 stetig an Größe und Relevanz gewonnen. Der prominenteste Modellorganismus für die Erforschung der circadianen Uhr ist Drosophila melanogaster, deren Uhr als Ansatzpunkt dient, die grundlegenden Vorgänge eines derart komplexen, endogenen Taktsystems zu verstehen. In dieser Thesis wurde versucht die Forschung an der circadianen Uhr mit den Techniken der Optogenetik zu kombinieren, eines jungen Forschungsfeldes, welches durch die Entdeckung von Channelrhodpsin 2 vor über 15 Jahren eröffnet wurde. Channelrhodopsin 2 ist ein Licht-gesteuerter Ionenkanal, der in der Grünalge Chlamydomonas reinhardtii entdeckt wurde. In der Optogenetik nutzen Forscher diese Licht-gesteuerten Ionenkanäle, indem sie sie in den Zellen anderer Organismen exprimieren, welche dann durch Licht stimuliert werden können. Dies ist besonders nützlich bei der Untersuchung von Neuronen, da diese Kanäle ein nahezu nicht-invasives Werkzeug zur Depolarisation neuronaler Membranen bieten. Das Ziel dieser Thesis war es, ein optogenetisches Werkzeug zu entwickeln, welches die circadiane Uhr von Drosophila melanogaster durch Licht manipulieren und deren Phase verschieben kann. Eine Phasenverschiebung ist die adaptive Antwort der circadianen Uhr auf einen äußeren Reiz, welcher eine Veränderung des natürlichen Lichtzyklus signalisiert. Ein optogenetisches Werkzeug, das die Phase der inneren Uhr verlässlich verschieben kann, würde viele neue Möglichkeiten zur Erforschung des neuronalen Uhrnetzwerks eröffnen und wie die Neuronen miteinander kommunizieren um das Netzwerk zu synchronisieren. Das erste optogenetische Werkzeug das in der circadianen Uhr von Drosophila melanogaster getestet wurde war „ChR2-XXL“, eine Channelrhodopsin-Variante mit erhöhter Expression und Photoströmen, gepaart mit einem verlängerten geöffneten Zustand. Die spezifische Expression von ChR2-XXL und auch die späterer Konstrukte wurde durch die Verwendung der drei Uhr-spezifischen GAL4-Treiberlinien clk856-gal4, pdf-gal4 und mai179-gal4 bewerkstelligt. Obwohl bereits gezeigt wurde, dass ChR2-XXL höchst effektiv die Depolarisierung von Neuronen bewirkt, waren diese Stimulationen jedoch nicht in der Lage die Phase der circadianen Uhr von Drosophila signifikant zu verschieben. Die zweite Serie an Versuchen wurde mit den konzeptionell neuartigen optogenetischen Werkzeugen Olf-bPAC und SthK-bPAC durchgeführt, welche jeweils einen durch zyklische Nukleotide gesteuerten Ionenkanal (Olf und SthK) mit der Licht-gesteuerten Adenylatcyclase bPAC kombinieren. Diese Werkzeuge erwiesen sich als äußert nützlich, solange sie in den Motoneuronen von Drosophila-Larven im dritten Larvenstadium exprimiert wurden, wo sie bei Beleuchtung die Larven sowohl paralysierten, als auch deren Körperlänge beeinflussten. Auf diese Weise konnten diese neuen Werkzeuge präzise charakterisiert werden, was in der erfolgreichen Veröffentlichung eines Forschungsartikels mündete, welcher hauptsächlich von der elektrophysiologischen Charakterisierung der Werkzeuge handelte und von deren Anwendungsmöglichkeiten in Modellorganismen wie Drosophila. In der circadianen Uhr verursachten diese Werkzeuge jedoch substantielle Schäden und produzierten schwere Arrhythmie und Anomalien in der neuronalen Entwicklung. Die Verwendung einer temperatur-sensitiven GAL80-Linie um die Expression zu verzögern, erzeugte ebenfalls keinerlei positive Ergebnisse. Für die letzte Serie an Experimenten wurde eine weitere Reihe neuer optogenetischer Werkzeuge verwendet, orientiert an Olf-bPAC und SthK-bPAC, wobei bPAC durch die membrangebundene Guanylatcyclase „CyclOp“ ausgetauscht wurde, welche wiederrum mit weniger wirkstarken Olf-Varianten kombiniert wurde. Dieser letzte Ansatz scheiterte jedoch ebenfalls. Obwohl diese neuen Werkzeuge in der Lage waren die Neuronenmembran bei Beleuchtung effektiv zu depolarisieren, vermochten sie es letztendlich nicht eine Phasenverschiebung zu bewirken. Zusammengenommen zeigen diese überwiegend negativen Ergebnisse, dass die optogenetische Manipulation der circadianen Uhr von Drosophila melanogaster ein extrem anspruchsvolles Thema ist. Da Licht bereits ohnehin den einflussreichsten Umweltfaktor für die circadiane Uhr darstellt, verlangt die Kombination von Chronobiologie und Optogenetik eine extrem präzise Feinabstimmung der Versuchsparameter, um überhaupt darauf hoffen zu dürfen, positive Ergebnisse mit derlei Versuchen zu erzeugen. KW - Chronobiologie KW - Optogenetik KW - Taufliege KW - Optogenetics KW - Chronobiology KW - Channelrhodopsin KW - Drosophila melanogaster Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-184952 ER - TY - JOUR A1 - Liu, Yi A1 - Maierhofer, Tobias A1 - Rybak, Katarzyna A1 - Sklenar, Jan A1 - Breakspear, Andy A1 - Johnston, Matthew G. A1 - Fliegmann, Judith A1 - Huang, Shouguang A1 - Roelfsema, M. Rob G. A1 - Felix, Georg A1 - Faulkner, Christine A1 - Menke, Frank L.H. A1 - Geiger, Dietmar A1 - Hedrich, Rainer A1 - Robatzek, Silke T1 - Anion channel SLAH3 is a regulatory target of chitin receptor-associated kinase PBL27 in microbial stomatal closure JF - eLife N2 - In plants, antimicrobial immune responses involve the cellular release of anions and are responsible for the closure of stomatal pores. Detection of microbe-associated molecular patterns (MAMPs) by pattern recognition receptors (PRRs) induces currents mediated via slow-type (S-type) anion channels by a yet not understood mechanism. Here, we show that stomatal closure to fungal chitin is conferred by the major PRRs for chitin recognition, LYK5 and CERK1, the receptor-like cytoplasmic kinase PBL27, and the SLAH3 anion channel. PBL27 has the capacity to phosphorylate SLAH3, of which S127 and S189 are required to activate SLAH3. Full activation of the channel entails CERK1, depending on PBL27. Importantly, both S127 and S189 residues of SLAH3 are required for chitin-induced stomatal closure and anti-fungal immunity at the whole leaf level. Our results demonstrate a short signal transduction module from MAMP recognition to anion channel activation, and independent of ABA-induced SLAH3 activation. KW - plants Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-202631 VL - 8 ER - TY - JOUR A1 - Jaślan, Dawid A1 - Dreyer, Ingo A1 - Lu, Jinping A1 - O'Malley, Ronan A1 - Dindas, Julian A1 - Marten, Irene A1 - Hedrich, Rainer T1 - Voltage-dependent gating of SV channel TPC1 confers vacuole excitability JF - Nature Communications N2 - In contrast to the plasma membrane, the vacuole membrane has not yet been associated with electrical excitation of plants. Here, we show that mesophyll vacuoles from Arabidopsis sense and control the membrane potential essentially via the K\(^+\)-permeable TPC1 and TPK channels. Electrical stimuli elicit transient depolarization of the vacuole membrane that can last for seconds. Electrical excitability is suppressed by increased vacuolar Ca\(^{2+}\) levels. In comparison to wild type, vacuoles from the fou2 mutant, harboring TPC1 channels insensitive to luminal Ca\(^{2+}\), can be excited fully by even weak electrical stimuli. The TPC1-loss-of-function mutant tpc1-2 does not respond to electrical stimulation at all, and the loss of TPK1/TPK3-mediated K\(^{+}\) transport affects the duration of TPC1-dependent membrane depolarization. In combination with mathematical modeling, these results show that the vacuolar K\(^+\)-conducting TPC1 and TPK1/TPK3 channels act in concert to provide for Ca\(^{2+}\)- and voltage-induced electrical excitability to the central organelle of plant cells. KW - Biophysics KW - Plant signalling Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-202029 VL - 10 ER - TY - JOUR A1 - Raheem, Dotsha J. A1 - Tawfike, Ahmed F. A1 - Abdelmohsen, Usama R. A1 - Edrada-Ebel, RuAngelie A1 - Fitzsimmons-Thoss, Vera T1 - Application of metabolomics and molecular networking in investigating the chemical profile and antitrypanosomal activity of British bluebells (\(Hyacinthoides\) \(non-scripta\)) JF - Scientific Reports N2 - Bulb, leaf, scape and flower samples of British bluebells (Hyacinthoides non-scripta) were collected regularly for one growth period. Methanolic extracts of freeze-dried and ground samples showed antitrypanosomal activity, giving more than 50% inhibition, for 20 out of 41 samples. High-resolution mass spectrometry was used in the dereplication of the methanolic extracts of the different plant parts. The results revealed differences in the chemical profile with bulb samples being distinctly different from all aerial parts. High molecular weight metabolites were more abundant in the flowers, shoots and leaves compared to smaller molecular weight ones in the bulbs. The anti-trypanosomal activity of the extracts was linked to the accumulation of high molecular weight compounds, which were matched with saponin glycosides, while triterpenoids and steroids occurred in the inactive extracts. Dereplication studies were employed to identify the significant metabolites via chemotaxonomic filtration and considering their previously reported bioactivities. Molecular networking was implemented to look for similarities in fragmentation patterns between the isolated saponin glycoside at m/z 1445.64 [M + formic-H](-) equivalent to C64H104O33 and the putatively found active metabolite at m/z 1283.58 [M + formic-H](-) corresponding to scillanoside L-1. A combination of metabolomics and bioactivity-guided approaches resulted in the isolation of a norlanostane-type saponin glycoside with antitrypanosoma I activity of 98.9% inhibition at 20 mu M. KW - Drug discovery KW - Metabolomics Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-224935 VL - 9 ER - TY - JOUR A1 - Hupp, Sabrina A1 - Rosenkranz, Maaria A1 - Bonfig, Katharina A1 - Pandey, Chandana A1 - Roitsch, Thomas T1 - Noninvasive Phenotyping of Plant–Pathogen Interaction: Consecutive In Situ Imaging of Fluorescing Pseudomonas syringae, Plant Phenolic Fluorescence, and Chlorophyll Fluorescence in Arabidopsis Leaves JF - Frontiers in Plant Science N2 - Plant–pathogen interactions have been widely studied, but mostly from the site of the plant secondary defense. Less is known about the effects of pathogen infection on plant primary metabolism. The possibility to transform a fluorescing protein into prokaryotes is a promising phenotyping tool to follow a bacterial infection in plants in a noninvasive manner. In the present study, virulent and avirulent Pseudomonas syringae strains were transformed with green fluorescent protein (GFP) to follow the spread of bacteria in vivo by imaging Pulse-Amplitude-Modulation (PAM) fluorescence and conventional binocular microscopy. The combination of various wavelengths and filters allowed simultaneous detection of GFP-transformed bacteria, PAM chlorophyll fluorescence, and phenolic fluorescence from pathogen-infected plant leaves. The results show that fluorescence imaging allows spatiotemporal monitoring of pathogen spread as well as phenolic and chlorophyll fluorescence in situ, thus providing a novel means to study complex plant–pathogen interactions and relate the responses of primary and secondary metabolism to pathogen spread and multiplication. The study establishes a deeper understanding of imaging data and their implementation into disease screening. KW - green fluorescence protein (GFP) KW - plant–pathogen interaction KW - imaging PAM KW - chlorophyll fluorescence imaging KW - phenolic compounds Y1 - 2019 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189425 SN - 1664-462X VL - 10 IS - 1239 ER -