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Plants must respond to multiple stimuli in a natural environment. Therefore they need the ability to rapidly reorganise and specifically build up appropriate metabolites to adapt to their environment. Abiotic cues, such as ambient solar radiation, influence the next trophic level directly, but also an altered plant composition triggered by these environmental cues can have an effect on the behaviour of herbivores. The aim of this study was to test effects of the important ultraviolet (UV) radiation on plants and on plant-insect interactions using multi-level investigations. The focus was on the conduction of controlled experiments with broccoli plants in highly engineered greenhouses covered with innovative materials, which only differed in their UV-B transmission. For the first time in this controlled environment the plant-mediated UV-B effects on phloem-feeding aphids were studied. Broccoli plants (Brassica oleracea L. convar. botrytis, Brassicaceae) were under filter tents either exposed to (inclusion, +UV) or not exposed to (exclusion, -UV) UV-A / UV-B radiation. In greenhouses covered with new, innovative materials transmitting high (80%), medium (23%) or low (4%) levels of ambient solar UV-B radiation, in particular the influence of UV-B radiation on broccoli was examined. Plants respond highly specific to environmental stimuli such as UV-B radiation and herbivory. UV-B radiation has a strong impact on the plants’ architecture and flavonoid contents, which can in turn influence plant-insect interactions. Phloem-feeding aphids can be negatively affected by UV-B mediated plant changes. However, a direct effect of UV radiation on the behaviour of herbivores is also evident. Mainly the number, composition and quality of herbivorous species as well as an exceeding of a certain infestation threshold determine the mode of plant changes. In conclusion, UV-B radiation has the potential to harden plants against herbivores and simultaneously increases the concentrations of valuable secondary metabolites for human nutrition in important crop species such as broccoli.
Phytohormones are known for their pivotal roles in promoting normal growth and development of the plants and contributing to the mechanism of defense. Although an over simplification, however, they may be categorized as stress specific and growth promoting. SA and JA/Ethylene are implicated in stress responses while auxins, cytokinins and gibberellins are involved in developmental processes. Phytohormones from the above perspective got much attention in the last few decades; however their reciprocal role is currently in focus. It is because of the reason that plant pathogens cause overall hormonal imbalance at host pathogen interface and alter host physiology for the sake of pathogenecity. Despite their importance in growth and development, cytokinins are among the most neglected phytohormones that are usually noticed as consequence rather than a cause of pathogen infection. Results presented in this thesis are based on the hypothesis that elevated levels of CKs embody plants with resistance against hemibiotrophic pathogens. To explore a connection between the spread of P. syringae and its tobacco host, CKs over producing transgenic plants were investigated whereby bacterial IPT gene was expressed under the control of pathogen inducible, tetracycline inducible and developmentally inducible promoters. To further validate the out-come of transgenic plants, various types of cytokinins were exogenously fed to detached tobacco leaves. Mentioned transgenics and exogenous CKs feeding approaches unanimously resulted in, “more cytokinins less disease symptoms” and vice versa. This state of cytokinins mediated resistance was further substantiated with various cellular, signaling, biochemical and microbial approaches wherein levels of SA and JA remained unaffected. Conversely, PR1 gene expression was strongly up-regulated in enhanced cytokinins accumulating samples. Moreover, less accumulation of ROS was observed in IPT expressing sites of the plants as compared to their corresponding controls. Additionally, we neither noticed any direct effect of cytokinins on the growth of P. syringae pv. tabaci nor found presence of anti-microbial peptides in cytokinins enriched extracts. Interestingly, enhanced accumulation of phtyoalexins in elevated CKs status of the plant proved to be a possible gesture in jeopardizing the spread of pathogen. Contrarily, no reduction was observed in the spread of fungal necrotrophic pathogen Sclerotinia sclerotiorum when leaves of elevated CKs were inoculated. Besides host-pathogen interaction in perspective of elevated cytokinins, impact of modulated sugar status of the plant on the spread of pathogen was also investigated. For this purpose, previously generated modulated invertase enzyme tobacco transgenic plants were analyzed. We showed that repression and de-repression of CIN1 gene under the control of tetracycline inducible-promoter did not affect the growth of P. syrinage pv. tabaci in Tet::CIN1 transgenic plants. Moreover, invertase inhibitor tobacco lines expressing NtCIF gene under the control of the same promoter failed to exhibit differential pathogenic responses in induced and non induced status of the plant. Similar was the case of tomato transgenic plants expressing NtCIF gene under the control of invertase gene Lin6 promoter in Lin6:: NtCIF plants for P.syringae pv. tomato DC 3000. Interestingly, when challenged Lin6:: NtCIF tomato plants with Botrytis cinerea, severe disease symptoms were observed on transgenic leaves as compared to control plants. To dissect a potential link between cytokinins and sugar metabolism with its effect on the growth of pathogen, invertase transgenic plants with elevated CKs were probed. When expressed exogenous IPT gene under the control of pathogen inducible promoter (4xJERE::IPT) in transgenic background of Tet::CIN1, we observed localized differences in symptom development for P.syringae pv. tabaci. Similarly, when exogenously fed with kinetin, detached leaves of Tet::CIN1 exhibited retarded growth of P.syringae pv. tabaci as compared to the tetracycline induced leaves. These results led to the conclusion that extracellular invertase may not play an essential role in cytokinins mediated disease resistance against hemibiotrophic pathogens.
Land plants must control the transpiration water stream and balance it with carbon dioxide uptake for optimal photosynthesis. A highly specialized type of plant cell called guard cells have evolutionary appeared which are suited for this complicated purpose. Guard cells are located by pairs on aerated plant surface and form stomata – structural units, which represent highly regulated “watergate” (Roelfsema and Hedrich, 2005). Guard cells sense many environmental and internal plant-derived stimuli and by changing degree of their swelling tightly regulate diffusion of water vapor and other gases. Cell processes taking place in stomata during their movements had been a subject of intensive investigation for more than three decades (Schroeder et al., 2001; Assmann and Shimazaki, 1999). With use of electrophysiological technique the basic processes underlying stomatal movements were described (Thiel et al., 1992; Dietrich et. al., 2001; Roelfsema and Hedrich, 2005). Another set of questions arised between plant biologists is how the signals affecting stomatal aperture are transduced in guard cells starting from perception by receptor structures and ending on the osmodynamic motor components. Introduction of fluorescent microspectroscopy technique allowed to characterize some Ca2+ and H+-based signaling events, taking place in the cytoplasm during stomata function. Most of the processes, taking place in stomata were characterized in guard cell preparations, such as strips of isolated leaf epidermis or guard cell protoplasts, - cells with enzymaticaly digested cell walls. Some experimental observations although point that reactions of guard cells located in their natural environment, leaves of intact plants can differ from those could be registered in preparations. These deviations might be explained by the modulation of guard cell function by apoplastic factors originating from surrounding tissues like mesophyll or leaf epidermis (Roelfsema and Hedrich, 2002). On the other hand registration of physiological responses in prepared tissues may also contain possible artifacts, related to the preparation procedures. The aim of the experimental work presented here was to investigate the cell signaling events, taking place in guard cells upon plant stress hormone abscisic acid (ABA) and some other stimuli action. Abscisic acid is a compound that synthesized in plant roots upon drought and closes stomata in the leaf to prevent the plant organism from excessive water loss. Previous studies on guard cell of isolated epidermis and guard cell protoplasts showed, that ABA induces stomatal closure via activation of plasma membrane anion channels (Grabov et al., 1997; Pei et al, 1997). Anion channels are known to be activated by elevated 2 concentrations of cytoplasmic Ca2+ [Ca2+]cyt (Schroeder and Hagiwara, 1989; Hedrich et al., 1990). Application of Ca2+-sensitive fluorescent probes revealed [Ca2+]cyt increases in guard cells upon ABA action (McAinsh et al., 1990). This observation led to suggestion that [Ca2+]cyt directly participate in the transduction of ABA signal in guard cells. Although no direct evidences for co-occurrence of [Ca2+]cyt rises and following activation of anion channels upon ABA action was not presented until yet. Results of experimental work performed on intact Vicia faba, Commelina communis and Nicotiana plumbagnifolia plants showed that guard cells of intact plant leaves respond with transient activation of plasma membrane anion channels upon perception of ABA. Kinetics of the response is highly reproducible and seemed to be conserved between species. Although despite clear generation of anion current transients, no [Ca2+]cyt increases could be recorded with using fluorescent probe Fura-2 microinjected into the cytoplasm. Together with results of later study on intact Nicotiana tabacum guard cells, reported obligatory [Ca2+]cyt increases which were desynchronized with anion current transients (Marten et al., 2007b) this, may indicate that [Ca2+]cyt increases are not necessary component of ABA signal transduction pathway. Together with absence of the effect of cytoplasm-delivered Ca2+- mobilizing agents IP3, IP6 and NAADP on anion currents these data may suppose that role of [Ca2+]cyt in ABA signaling must be reassessed. Further interest represented characterization of [Ca2+]cyt signaling and homeostasis in intact guard cells comparing with those in prepared cells. Experiments revealed strong deviations in [Ca2+]cyt behavior between different measuring systems. While guard cells of intact plants were able to strictly maintain [Ca2+]cyt level upon experimental shifting of [Ca2+]cyt level in either direction of elevation or decrease, cells of isolated epidermis showed complete absence of such ability. Guard cell protoplasts showed even weaker [Ca2+]cyt regulation ability and were capable of low physiological [Ca2+]cyt levels maintaining only at depolarized membrane potentials. Apart to these differences, prepared guard cells showed also for-time less activation of anion currents by experimentally imposed [Ca2+]cyt increases. These data strongly suggest that registered in guard cell preparations [Ca2+]cyt signals may contain significant part of artifacts and must be carefully used for the building of models of guard cells signaling. Further experimental investigations are strongly required for understanding guard cell functioning, especially with relation of vacuoles participation. The experimental work was done by the author in the period from october 2001 until november 2004 under supervision of Professor Dr. Rainer Hedrich in laboratory of molecular plant physiology and biophysics at Julius-Maximillians University of Würzburg, Würz3 burg, Federal Republic of Germany. Scientific coordinator of the Ph. D. project is Dr. Max Robert Gustaaf Roelfsema, University of Würzburg. Most of experimental results, presented here (chapter III) are also published elsewhere (Roelfsema et al., 2004; Langer et al., 2004; Levchenko et al., 2005, 2008). Chapter I intend to shortly introduce the reader into the field of guard cell research and point out the current level of understanding regarding this branch of plant research. Special attention is given to description of guard cell ion channels, their function and regulation, including the mechanisms of Ca2+-, H+- and phosphorylation-based signaling. This section is preceded by a short history of guard cell research and explains the actuality of presented work. In chapter II experimental techniques, methods and data processing approaches, used in the presented work are described. Technique used for electrophysiological registrations on intact plant leaves were used before and described in more details by Roelfsema et al. (2001). Fluorescent microspectroscopy technique was for the first time applied to intact plant leaves in this work and described in more details including calibration of Fura-2 based measurements. Chapter III presents the major results of the experimental work. In chapter IV the experimental results are discussed and put into context with current knowledge of guard cell function knowledge. Finally, remarks on perspectives of guard cell signaling research are drawn.
Insects have evolved an astonishing array of defences to ward off enemies. Well-known and widespread is the regurgitation of oral secretions (OS), fluids that repel attacking predators. In herbivores, the effectiveness of OS has been ascribed so far to the presence of deterrent secondary metabolites sequestered from the host plant. This notion implies, however, that generalists experience less protection on plants with low amounts of secondary metabolites or with compounds ineffective against potential enemies. Resolving the dilemma, we describe a novel defence mechanism that is independent of deterrents as it relies on the OS’ intrinsic detergent properties. The OS of Spodoptera exigua (and other species) was found to be highly amphiphilic and well capable of wetting the hydrophobic cuticle of predatory ants. As a result, affected ants stopped attacking and engaged in extensive cleansing. The presence of surfactants was sufficient to explain the defensive character of herbivore OS. We hypothesize that detergency is a common but unrecognised mode of defence which provides a base level of protection that may or may not be further enhanced by plant-derived deterrents. Our study also proves that insects ‘invented’ the use of defensive surfactants long before modern agriculture had started applying them as insecticides.
An der pflanzlichen Plasmamembran geschieht die erste Wahrnehmung von mikrobiellen Molekülen, die MAMPs genannt werden. MAMP/PAMP Rezeptoren leiten frühe Abwehrantworten, wie die Produktion von reaktiven Sauerstoffspezies (ROS), externe Alkalisierung oder Ethylen, ein. Die Arabidopsis FLS2 rezeptorartige Kinase (RLK) stellt einen plasmamembran-lokalisierten MAMP Rezeptor dar, der über die Detektion des Flagellum von Pseudomonas species, eine basale Immunität in Arabidopsis thaliana vermittelt. Flg22, der kürzeste aktive Teil des bakteriellen Flagellins besteht aus 22 Aminosäuren und ist der bestuntersuchte bakterielle Elizitor. In der vorliegenden Arbeit zeigen wir eine starke Beteiligung von Ionenflüssen in der Initiationsphase der basalen Immunität. Unsere Messungen an intakten Arabidopsis Pflanzen und Pflanzengeweben sind in höchstem Masse reproduzierbar und öffnen eine neue Sicht, über die Natur von Ionentransporten in der Pflanzen - Mikroben Interaktion. Als Antwort auf die Applikation von flg22, haben wir nach einer Verzögerungsphase von etwa 2 Minuten eine transiente, dosis-abhängige Depolarisation (EC50=0,2 nM) in Mesophyll- und Wurzelhaarzellen von A. thaliana messen können. Das um 2 Aminsäuren kürzere Peptid flg22 Δ2 oder das Flagellin anderer Bakterien (Agrobacterium or Azospirillum) führten zu keiner Membrandepolarisation. Ebenso konnten keine Membranspannungsänderungen in dem Arabidopsis Ökotypen Ws-0, dem der funktionelle FLS2 Rezeptor fehlt, detektiert werden. Die Komplementation von Ws-0 Pflanzen mit dem intakten FLS2 Rezeptorgen rief eine Resensibilisierung für flg22 hervor. Mit dem EF-Tu Elizitor Peptid aus E.coli, welches durch den Arabidopsis MAMP Rezeptor EFR detektiert wird, wurden ähnliche Ergebnisse erzielt. Auf der Basis von Aequorin wurden Kalzium-induzierte Lumineszenzmessungen durchgeführt, in denen ein transienter Anstieg der zytosolischen Kalziumkonzentration als Antwort auf die Applikation von flg22 gemessen werden konnte. Dosis-Abhängigkeitsmessungen von flg22 und [Ca2+]cyt wiesen zwei unterschiedliche EC50 Werte, von 43 ± 2 pM und 67 ± 42 nM, auf. Möglicherweise wird auf zwei verschiedene Kalziumpools zugegriffen oder es werden zwei verschiedene Kalziumleitfähigkeiten aktiviert. Die Ionenkanalaktivierung und folgende Depolarisation benötigt die aktive Rezeptorkinase. In bak1-4 Arabidopsis Pflanzen, in denen die FLS2 Untereinheit BAK1 – eine weitverbreitete RLK, die auch mit dem Brassinosteroid Rezeptor assoziiert ist – fehlt, konnte keine Depolarisation als Antwort auf flg22 gemessen werden. Arabidopsis Mesophyllzellen zeigten die typische Alkalisierung des Apoplasten als Antwort auf flg22. Nicht-invasive MIFETM Experimente mit Ionen-selektiven Elektroden ergaben, dass der pH-Anstieg durch einen Einstrom von Protonen hervorgerufen wurde. Zusätzlich wurde ein Ausstrom von Chlorid und Kalium aufgezeichnet. Ähnlich wie das Kalziumsignal waren alle detektierten Ionenströme von transienter Natur. Im zweiten Ansatz wurden Membranpotential-Messungen durchgeführt, während in der externen Lösung die Konzentrationen von Protonen, Kalzium, Kalium oder Anionen variiert wurden. Nur eine Änderung des Anionengradienten hatte einen entscheidenden Einfluss auf die flg22-induzierte Depolarisation, was die Wichtigkeit der Anionenkanalaktivierung unterstreicht. Exudat Analysen ergaben, dass Nitrat das bevorzugt transportierte Ion ist. Unter zahlreichen getesteten Ionenkanalblockern erwies sich lediglich Lanthan als effektiver Blocker des flg22-induzierten zytosolichen Kalziumanstiegs, des Protoneneinstroms und der Membrandepolarisation. Da Lanthan bekanntlich unspezifische Kationenkanäle blockt, kann man an diesem Punkt davon ausgehen, dass Kalzium-aktivierte Anionenkanäle die Membrandepolarisation vermitteln und darauf eine Aktivierung von auswärtsgerichteten Kaliumkanälen folgt. Zukünftige Studien mit Doppelläufigen-Mikroelektroden Spannungsklemmexperimenten oder externen ionenselektiven Elektroden an intakten Schliesszellen werden helfen weitere Informationen über die Natur der Ionenkanäle in der basalen Immunität oder generell in der Pflanzen-Mikroben Interaktion zu erhalten. Über die elektrophysiologische Charakterisierung der multiplen Ionenströme in der basalen Immunität hinaus, ist natürlich der nächste wichtige Schritt das oder die Gene zu finden, die für die Ionenkanäle oder Transporter kodieren, die durch nicht nekrotisierende Elizitoren wie flg22 in der basalen Immunantwort in Pflanzen aktiviert werden.
Wirkspektrum und Signaltransduktionsmechanismus von oxidierten Lipiden in Arabidopsis thaliana
(2009)
Die endogen in Pflanzen radikalisch gebildeten Phytoprostane regulieren in Arabidopsis thaliana eine Reihe von Genen, die an den Prozessen der Detoxifizierung und Zellproliferation beteiligt sind, während die externe Applikation dieser Oxylipine in vitro eine Akkumulation von sekundären Metaboliten, sogenannten Phytoalexinen, nach sich zieht. Ferner war aus vorherigen Arbeiten des Lehrstuhls für Pharmazeutische Biologie bekannt, dass die Vorbehandlung mit Phytoprostanen in Arabidopsis thaliana eine Schutzwirkung gegen nachfolgenden oxidativen Stress vermittelt. Neben nicht-enzymatisch gebildeten Oxylipinen akkumulieren in höheren Pflanzen als Antwort auf einen oxidativen Stress auch enzymatisch gebildete Oxylipine wie 12-Oxophytodiensäure (OPDA) und Jasmonsäure (JA). Als Ausgangspunkt zur systematischen Analyse der von einzelnen Phytoprostanen vermittelten Wirkspektren diente in der vorliegenden Arbeit eine Transkriptionsanalyse unter Verwendung einer mixotrophen Arabidopsis thaliana Zellkultur nach Phytoprostan-A1 (PPA1)-Behandlung. In weiterführenden Experimenten wurde das durch PPA1-vermittelte Genexpressionsprofil mit dem Profil von weiteren, nicht-enzymatischen sowie dem durch die enzymatisch gebildeten Oxylipine OPDA bzw. JA hervorgerufenen Genexpressionsprofil verglichen. Die Vergleiche zeigten signifikante Übereinstimmungen, aber auch deutliche Unterschiede im Wirkprofil einzelner enzymatischer bzw. nicht-enzymatischer Oxylipine. Das Wirkungsspektrum der radikalisch gebildeten PPA1 überschneidet sich zu 40 Prozent mit dem der enzymatisch gebildeten OPDA, jedoch nur zu sieben Prozent mit dem Wirkspektrum der ebenfalls enzymatisch gebildeten JA. Diese Beobachtung ließ einen über strukturelle Merkmale vermittelten Signalmechanismus vermuten, da die chemischen Strukturen von PPA1 und OPDA, nicht jedoch PPA1 und JA, verwandt sind. Zur Überprüfung der vorstehenden Hypothese wurden die Promotorbereiche der durch PPA1 mehr als dreifach induzierten Gene bioinformatisch auf häufig vorhandene Sequenzmotive untersucht. Es zeigte sich, dass etwa die Hälfte der Promotorbereiche der durch PPA1 induzierten Gene ein Bindungsmotiv für TGA-Transkriptionsfaktoren enthält. Nachfolgende Transkriptomanalysen in der TGA-Dreifach knockout Arabidopsis thaliana Mutante tga2tga5tga6 zeigten, dass 60 Prozent der PPA1- bzw. 30 Prozent der ODPA-vermittelten Genexpression durch die TGA-Transkriptionsfaktoren TGA2, TGA5 und TGA6 vermittelt werden. Neben übereinstimmenden Wirkungen von PPA1 und OPDA in der Genexpression sind in der Literatur überschneidende Wirkungen von OPDA und JA bezüglich einer Wurzelwachstumshemmung in Arabidopsis thaliana beschrieben. In Experimenten zur Untersuchung des Wurzelwachstums resultierte die exogene Applikation von JA bzw. OPDA auf Arabidopsis thaliana Samen in einer Hemmung des Wurzelwachstums um 63 bzw. 72 Prozent. Dagegen vermittelte PPA1 nur eine Hemmung um 50 Prozent. Die vorstehend beschriebenen Wirkungen verschiedener Phytoprostane belegen ein umfassendes Wirkspektrum dieser heterogenen Substanzklasse. Neben den in vorliegender Arbeit im Vordergrund stehenden Phytoprostan-vermittelten Stressreaktionen sind eine Reihe physiologischer Prozesse, darunter das Wurzelwachstum, zumindest teilweise durch Phytoprostane reguliert. Ferner konnte in der der vorliegenden Arbeit erstmalig gezeigt werden, dass mindestens zwei der durch Phytoprostane induzierten Gene Proteine kodieren, die effizient die Metabolisierung von Phytoprostanen fordern, um oxidativen Schäden vorzubeugen. Vermittelt werden die Phytoprostan- Wirkungen unter anderem durch die TGA-Transkriptionsfaktoren TGA2, TGA5 und TGA6, welche zur Expression von Detoxifizierungs- und Stressgenen führen.
Die Lamina ist ein Netzwerk aus Lamin-Proteinen und befindet sich unterhalb der inneren Kernmembran. Die Lamine A/C, die zu den Typ V Intermediärfilamenten gehören, spielen eine wichtige Rolle bei der Aufrechterhaltung der strukturellen Integrität des Zellkernes sowie der Chromatinorganisation, der Transkription, der DNA-Replikation, der Differenzierung und der Genomstabilität. In den letzten Jahren wurden über 200 verschiedene Mutationen im Lamin A/C kodierenden LMNA Gen gefunden, die mehr als 10 unterschiedliche Krankheiten, die so genannten Laminopathien, auslösen können. Zu diesen Laminopathien zählen unter anderem die Emery-Dreifuss-Muskeldystrophie (EDMD) und das Progerie-Syndrom. Die Mutation LMNA S143F In dieser Arbeit wurde zunächst die Punktmutation LMNA S143F, die in der N-terminalen Domäne des Lamin A/C lokalisiert ist, näher untersucht. Diese Mutation ist der Auslöser von einzigartigen phänotypischen Merkmalen einer frühen Myopathie sowie einer Progerie. Strukturelle Analysen mit dem Elektronenmikroskop ergaben, dass die primären dermalen Fibroblasten der Laminopathie-Patientin morphologisch veränderte Zellkerne hatten. In Abhängigkeit von S143F Lamin A/C konnte in den Patientenfibroblasten eine abnormale Lokalisation der Kernproteine Nesprin2 Giant und den kürzeren Nesprin2-Isoformen nachgewiesen werden. Darüber hinaus konnten wir beobachten, dass eine reduzierte Expression von Nesprin2 Giant eine Rolle bei der Ausprägung der morphologischen Kerndeformationen spielte. Patientenzellen, die Nesprin2 Giant in hohem Maße exprimierten, zeigten keine Deformationen des Zellkerns und eine normale Verteilung verschiedener Kernproteine. FRAP-Analysen in vivo und biochemische Proteinextraktionsstudien des S143F-Lamin A/Cs in vitro zeigten eine verringerte Mobilität und Dynamik, sowie eine reduzierte Löslichkeit von S143F Lamin A/C gegenüber wildtypischem Lamin A/C. Die Mutation LMNA S143F liegt im Außenbereich der coiled-coil-Struktur des Lamins. Dadurch führt der Austausch der neutralen AS Serin durch die große hydrophobe AS Phenylalanin nicht zu einer Störung in der Dimer-bildung, sondern zu einer Beeinflussung der Formierung zu Protofilamenten bzw. höheren Strukturen. Dies konnte durch in vitro Untersuchungen von rekonstituierten Parakristallen aus S143F Lamin A/C dargestellt werden, die eine Veränderung des transversalen Bänderungs-musters aufwiesen. Zusammengenommen zeigen die Resultate, dass die Mutation LMNA S143F die Lamin-A-Polymerisation beeinflusst und dadurch die Dynamik und Mobilität der Typ A-Lamine beeinträchtigt. Außerdem konnte erstmals nachgewiesen werden, dass das Nesprin2 Giant Protein eine essentielle Rolle in der Pathogenese von Laminopathien einnimmt, indem es die Struktur des Zellkerns verstärkt und als struktureller „Gegenspieler“ zu Lamin A/C fungiert. Die Mutation LMNA R545C Die Punktmutation LMNA R545C, die in der C-terminalen Domäne des Lamin A/C lokalisiert, ist Auslöser eines sehr gravierenden Phänotyps der autosomal dominanten Form der Emery- Dreifuss-Muskeldystrophie (AD-EDMD). Strukturelle Analysen ergaben, dass die primären Myoblasten des EDMD-Patienten morphologisch veränderte Zellkerne haben. Ein Vergleich von deformierten Kernen aus Zellen mit verschiedenen Laminopathie-auslösenden Mutationen wie LMNA R545C, LMNA S143F und LMNA R377H zeigten allerdings, dass die untersuchten Mutationen nicht immer zu gleichen abnormalen Phänotypen der Kernmorphologie, sondern zu divergenten Ausprägungen der morphologischen Kernveränderungen in Patientenzellen führten. Immunfluoreszenzanalysen ergaben, dass auch die Proteine Lamin A/C und Emerin in den Patientenzellen eine fehlerhafte Verteilung aufwiesen und „Honigwabenmuster“ ausbildeten. Interessanterweise konnte auch eine vom Alter der Zellen abhängige Akkumulation der 20S-Untereinheit des Proteasoms in kleine nukleäre Foci beobachtet werden. Diese Foci kolokalisierten weitgehend mit den promyelotischen Leukämie-Körperchen (PML). In den Patientenmyoblasten war der CDK-Inhibitor p21 stark angereichert, was ein Hinweis auf eine Beeinträchtigung der proteasomalen Funktion ist. Nach Kultivierung der Patientenmyoblasten in Minimalmedium zeigten diese eine eingeschränkte Fähigkeit zur ex-vivo Differenzierung zu Myotuben. Dementsprechend war die Expression des Myogenese-spezifischen Transkriptionsfaktors Myogenin, sowie des Proliferationmarkers hypophosphoryliertes Retinoblastoma-Protein in Patientenmyoblasten nicht korrekt induziert. Zusammengenommen weisen diese Daten darauf hin, dass auch die Mutation LMNA R545C Einfluss auf die Kernarchitektur und -Proteinverteilung, die Chromatinorganisation, Gen-expression und Funktion des Proteasoms einnimmt. Darüber hinaus beeinträchtigte die Mutation LMNA R545C die Fähigkeit zur korrekten Proliferation und Differenzierung der Myoblasten, welches eine potentielle Rolle in der Pathogenese von Laminopathien einnimmt.
Activation of mitogen-activated protein (MAP) kinases is a common reaction of plant cells in defense-related signal transduction pathways. Since the downstream events after the activation of MAP kinases are largely unknown in plants, the role of MAP kinases in the co-ordinate regulation of defense reactions and primary carbon metabolism by stress related stimuli has been analyzed in tomato. Thus, the relationship between mitogen activated protein kinases (LpMPK2 and LpMPK3) and extracellular invertases Lin6, as the key enzyme of an apoplasmic phloem unloading pathway, has been analyzed. The results showed that the mRNAs of LpMPK3 and Lin6 are sequentially induced by the same set of stress related stimuli (E-Fol, PGA,wounding, and KCl). The induction of the Lin6 promotor, as revealed by an increase in β-glucuronidase activity after 2 hours, was dependent both on the expression and activation of LpMPK3. These data suggest that the induction of extracellular invertase Lin6 by stress related stimuli requires LpMPK3. Glucose, metabolic molecule, was shown to result in the simultaneous induction of AtMPK4 and AtMPK6 activities that could be separated by anion-exchange chromatography, and characterized by differential cross-reaction with MAP kinase antibodies. Taken together, these data suggest that the activation of MAP inases play central roles in the regulation of sugar signaling. Stomatal movement is controlled by environmental signals including light intensity,humidity and atmospheric CO2 level. In Arabidopsis, a complete MAP kinase signaling cascade regulates stomatal development and patterning. However, the movement of stomata mediated by CO2 induced signaling pathways is not fully studied in higher plants. Here, we show that elevated levels of CO2 induce rapid and transient activation of SIPK and NtMPK4. The activation of both MAP kinases may regulate the anion channel activation for stomatal movement by the elevated level CO2. Up to now, the non-antioxidant function of tocopherol is not clear in higher plant,whereas the ability of tocopherol to modulate the stress tolerance mediated by function of antioxidant has been described in numerous studies. Thus, the function of α-tocopherol in stimuli-induced signal transduction pathways mediated by MAP kinase has been analyzed in tobacco. It has been shown that the activation of MAP kinase was induced by treatment of fungal elicitor and α-tocopherol phosphate but not α-tocopherol. Interestingly, α-tocopherol showed the transient inhibitory effect on the activation of stimuli-induced MAP Kinases in BY2 cells and tobacco plants, whereas ascorbate did not inhibit the activation of MAP kinases. The inhibitory activity test indicated that current application may indirectly affect the activity of MAP kinases. These results suggest that α-tocopherol can negatively regulate stimuliinduced signal transduction pathways via inactivation of MAP kinases. The purine-analogues have been tested and reported to be specific inhibitors of protein kinases mediated by structural-based selectivity in mammalian. Here, we tested C2, N6, N9-trisubstituted purines to determine basic relationship between their chemical structure and inhibitory activity using a particular plant MAP kinase. The modification of substitution in position C2 and N9 caused the increased inhibitory activity of 6-(benzylamino) purine analogue. In addition, 6-(isopentenylamino) purine analogues suggested that addition of a methyl group to position N9 caused at least 2-fold increased inhibitory activity compared with the addition of isopropyl group.Taken together, our study suggests that the selectivity and potency of inhibitors can be improved by structure modification. In addition, we have characterized the physiological function of Arabidopsis thaliana PLAT domain protein 1 (AtPDP1) in modulating the interaction of defense pathways mediated by biotic and abiotic factors. Interestingly, overexpression of AtPDP1 resulted in increasing susceptibility of virulent pathogens and necrotrophic fungus, and developing necrosis induced by unknown biotic factors. However, these overexperssion lines showed the significantly delayed senescence and higher level of phosystem II quantum yield compared with control plants against high salt stress. Our results strongly indicate that AtPDP1 positively regulate with salt tolerance, and enhances the sensitivity to biotic stresses. We propose that the AtPDP1 might be regulated with the complex pathways of interplay among various signaling during stress adaptation.
The genus Borrelia belongs to the spirochete phylum, an ancient evolutionary branch of the domain bacteria that is only afar related to Gram-negative bacteria. Borreliae can be subdivided into the agents of the two borrelian-caused human diseases, Lyme disease and relapsing fever. Both disease patterns are closely related to the peculiar biology of Borrelia species and exhibit a wide spectrum of diverse clinical manifestations. Due to the small 0.91 Mb chromosome, borreliae have a lack of biosynthetic capacity. Thus, all Borrelia species are highly dependent on nutrients provided by their hosts. The transport of nutrients and other molecules across the outer membrane is enabled by pore-forming proteins, so-called porins. Porins are water-filled channels and can be subdivided into two different classes, general diffusion pores and substrate-specific porins. In terms of the Lyme disease agent Borrelia burgdorferi, three putative porins were characterized in previous studies: P13, Oms28 and P66. In contrast to Lyme disease species, the porin knowledge of relapsing fever Borrelia is low, which means that not any porin has actually been described for representatives of these agents. Thus, the general aim of this thesis was to provide insight into the porin content of both, Lyme disease and relapsing fever spirochetes. This aim could be achieved by isolating and identifying porins from Borrelia outer membranes and by biophysically characterizing them in artificial lipid membranes. In one chapter of this study, the first identification and characterization of a relapsing fever porin is presented. The pore-forming protein was isolated from outer membranes of Borrelia duttonii, Borrelia hermsii and Borrelia recurrentis and designated Oms38, for “outer membrane-spanning protein of 38 kDa”. Biophysical characterization of Oms38 was achieved by using the black lipid bilayer method and demonstrated that Oms38 forms small, water-filled channels with a single-channel conductance of 80 pS in 1 M KCl. The Oms38 channel did not exhibit voltage-dependent closure and is slightly selective for anions with a permeability ratio of cations over anions of 0.41 in KCl. Subsequently, a protein homologous to Oms38 was identified in the Lyme disease agents Borrelia burgdorferi, Borrelia garinii and Borrelia afzelii. The pore-forming protein of these species exhibits high sequence homology to Oms38 and similar biophysical properties, i.e. it forms pores of 50 pS in 1 M KCl. Interestingly, titration experiments revealed that this pore could be partly blocked by dicarboxylic anions, which means that this protein does not form a general diffusion pore but a channel with a binding-site specific for those compounds. Consequently, this porin was termed DipA, for “dicarboxylate-specific porin A”. In another set of experiments, it was shown that the porin P66 is present in both Lyme disease and relapsing fever species. Therefor, the outer membranes of the Lyme disease species Borrelia burgdorferi, Borrelia afzelii, Borrelia garinii and the relapsing fever species Borrelia duttonii, Borrelia recurrentis and Borrelia hermsii were closer investigated. Except of the P66 homologue of Borrelia hermsii P66 of all species was highly active in artificial lipid membranes, forming pores with huge single-channel conductances between 9 and 11 nS in 1 M KCl. Moreover, the channel diameter and the constitution of Borrelia burgdorferi P66 were investigated in detail. Therefor, the P66 single-channel conductance in the presence of different nonelectrolytes with known hydrodynamic radii was analyzed in black lipid bilayers. The effective diameter of the P66 channel lumen was determined to be ~1.9 nm. Furthermore, as derived from multi-channel experiments the P66-induced membrane conductance could be blocked by certain nonelectrolytes, such as PEG 400, PEG 600 and maltohexaose. Additional blocking experiments on the single-channel level revealed seven subconducting states and indicated a heptameric constitution of the P66 channel. This indication could be confirmed by Blue native PAGE analysis which demonstrated that P66 units form a complex with a corresponding mass of approximately 440 kDa. Taking together, this thesis describes detailed biochemical and biophysical investigations of both Lyme disease and relapsing fever Borrelia porins and represents an important step forward in understanding the outer membrane pathways for nutrient uptake of these strictly host-dependent, pathogenic spirochetes. Furthermore, it provides some knowledge of the outer-membrane protein composition of Borrelia spirochetes. A profound knowledge of surface-exposed proteins, such as porins, is one precondition for the production of a successful vaccine and the drug design against the two borrelian-caused diseases.