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Introduction
Neurotransmitter release at presynaptic active zones (AZs) requires concerted protein interactions within a dense 3D nano-hemisphere. Among the complex protein meshwork the (M)unc-13 family member Unc-13 of Drosophila melanogaster is essential for docking of synaptic vesicles and transmitter release.
Methods
We employ minos-mediated integration cassette (MiMIC)-based gene editing using GFSTF (EGFP-FlAsH-StrepII-TEV-3xFlag) to endogenously tag all annotated Drosophila Unc-13 isoforms enabling visualization of endogenous Unc-13 expression within the central and peripheral nervous system.
Results and discussion
Electrophysiological characterization using two-electrode voltage clamp (TEVC) reveals that evoked and spontaneous synaptic transmission remain unaffected in unc-13\(^{GFSTF}\) 3rd instar larvae and acute presynaptic homeostatic potentiation (PHP) can be induced at control levels. Furthermore, multi-color structured-illumination shows precise co-localization of Unc-13\(^{GFSTF}\), Bruchpilot, and GluRIIA-receptor subunits within the synaptic mesoscale. Localization microscopy in combination with HDBSCAN algorithms detect Unc-13\(^{GFSTF}\) subclusters that move toward the AZ center during PHP with unaltered Unc-13\(^{GFSTF}\) protein levels.
Accurate information transfer between neurons governs proper brain function. At chemical synapses, communication is mediated via neurotransmitter release from specialized presynaptic intercellular contact sites, so called active zones. Their molecular composition constitutes a precisely arranged framework that sets the stage for synaptic communication.
Active zones contain a variety of proteins that deliver the speed, accuracy and plasticity inherent to neurotransmission. Though, how the molecular arrangement of these proteins influences active zone output is still ambiguous. Elucidating the nanoscopic organization of AZs has been hindered by the diffraction-limited resolution of conventional light microscopy, which is insufficient to resolve the active zone architecture on the nanometer scale. Recently, super-resolution techniques entered the field of neuroscience, which yield the capacity to bridge the gap in resolution between light and electron microscopy without losing molecular specificity. Here, localization microscopy methods are of special interest, as they can potentially deliver quantitative information about molecular distributions, even giving absolute numbers of proteins present within cellular nanodomains.
This thesis puts forward an approach based on conventional immunohistochemistry to quantify endogenous protein organizations in situ by employing direct stochastic optical reconstruction microscopy (dSTORM). Focussing on Bruchpilot (Brp) as a major component of Drosophila active zones, the results show that the cytomatrix at the active zone is composed of units, which comprise on average ~137 Brp molecules, most of which are arranged in approximately 15 heptameric clusters. To test for a quantitative relationship between active zone ultrastructure and synaptic output, Drosophila mutants and electrophysiology were employed. The findings indicate that the precise spatial arrangement of Brp reflects properties of short-term plasticity and distinguishes distinct mechanistic causes of synaptic depression. Moreover, functional diversification could be connected to a heretofore unrecognized ultrastructural gradient along a Drosophila motor neuron.
Brain function relies on accurate information transfer at chemical synapses. At the presynaptic active zone (AZ) a variety of specialized proteins are assembled to complex architectures, which set the basis for speed, precision and plasticity of synaptic transmission. Calcium channels are pivotal for the initiation of excitation-secretion coupling and, correspondingly, capture a central position at the AZ. Combining quantitative functional studies with modeling approaches has provided predictions of channel properties, numbers and even positions on the nanometer scale. However, elucidating the nanoscopic organization of the surrounding protein network requires direct ultrastructural access. Without this information, knowledge of molecular synaptic structure-function relationships remains incomplete. Recently, super-resolution microscopy (SRM) techniques have begun to enter the neurosciences. These approaches combine high spatial resolution with the molecular specificity of fluorescence microscopy. Here, we discuss how SRM can be used to obtain information on the organization of AZ proteins
The majority of rapid cell-to-cell communication mechanisms and information processing within the nervous system makes use of chemical synapses. Fast neurotransmission on these sites not only requires very close apposition of pre- and postsynaptic partners, but also depends on an effective structural arrangement of cellular components on both sides of the synaptic cleft. Synaptic vesicles fuse at active zones (AZs), characterized by an electron-dense protein mesh of insufficiently characterized composition and function. EM analysis of synapses identified electron dense structures thought (but not proven) to play an important role for vesicle release efficacy. The molecular organization of presynaptic AZs during Ca2+ influx–triggered neurotransmitter release is currently a focus of intense investigation. Due to its appearance in electron micrographs, dense bodies at Drosophila synapses were named T-bars. Together with the lab of Erich Buchner, we recently showed that Bruchpilot (BRP) of the Drosophila melanogaster, homologous to the mammalian CAST/ERC family in its N-terminal half, is essential for the T-bar assembly at AZs and efficient neurotransmitter release respectively. The question, in which way BRP contributes to functional and structural organization of the AZ, was a major focus of this thesis. First, stimulated emission depletion microscopy (STED), featuring significantly increased optical resolution, was used to achieve first insights into ‘cytoarchitecture’ of the AZ compartment. In addition, in vivo live imaging experiments following identified populations of synapses over extended periods were preformed to address the trafficking of protein at forming synapses and thereby providing a temporal sequence for the AZ assembly process. Apart from BRP, two additional AZ proteins, DLiprin-α and DSyd-1, were included into the analysis, which were both shown to contribute to efficient AZ assembly. Drosophila Syd-1 (DSyd-1) and Drosophila Liprin-α (DLiprin-α) clusters initiated AZ assembly, finally forming discrete ‘quanta’ at the AZ edge. ELKS-related Bruchpilot, in contrast, accumulated late from diffuse pools in the AZ center, where it contributed to the electron dense specialization by adopting an extended conformation vertical to the AZ membrane. We show that DSyd-1 and DLiprin-α are important for efficient AZ formation. The results of this thesis describe AZ assembly as a sequential protracted process, with matured AZs characterized by sub-compartments and likely quantal building blocks. This step-wise, in parts reversible path leading to mature AZ structure and function offers new control possibilities in the development and plasticity of synaptic circuits.
The presynaptic active zone (AZ) of chemical synapses is a highly dynamic compartment where synaptic vesicle fusion and neurotransmitter release take place. During evolution the AZ was optimized for speed, accuracy, and reliability of chemical synaptic transmission in combination with miniaturization and plasticity. Single-molecule localization microscopy (SMLM) offers nanometer spatial resolution as well as information about copy number, localization, and orientation of proteins of interest in AZs. This type of imaging allows quantifications of activity dependent AZ reorganizations, e.g., in the context of presynaptic homeostatic potentiation. In combination with high-pressure freezing and optogenetic or electrical stimulation AZs can be imaged with millisecond temporal resolution during synaptic activity. Therefore SMLM allows the determination of key parameters in the complex spatial environment of AZs, necessary for next generation simulations of chemical synapses with realistic protein arrangements.
Synapsen als Stellen der Kommunikation zwischen Neuronen besitzen spezialisierte Bereiche – Aktive Zonen (AZs) genannt –, die aus einem hoch komplexen Netzwerk von Proteinen aufgebaut sind und die Maschinerie für den Prozess der Neurotransmitter-Ausschüttung und das Vesikel-Recycling beinhalten. In Drosophila ist das Protein Bruchpilot (BRP) ein wichtiger Baustein für die T-förmigen Bänder („T-Bars“) der präsynaptischen Aktiven Zonen. BRP ist notwendig für eine intakte Struktur der Aktiven Zone und eine normale Exocytose von Neurotransmitter-Vesikeln. Auf der Suche nach Mutationen, welche die Verteilung von Bruchpilot im Gewebe beeinträchtigen, wurde eine P-Element-Insertion im Gen CG11489 an der Position 79D identifiziert, welches eine Kinase kodiert, die einen hohen Grad an Homologie zur Familie der SR Proteinkinasen (SRPKs) von Säugern aufweist. Die Mitglieder dieser Familie zeichnen sich durch eine evolutionär hoch konservierte zweigeteilte Kinasedomäne aus, die durch eine nicht konservierte Spacer-Sequenz unterbrochen ist. SRPKs phosphorylieren SR-Proteine, die zu einer evolutionär hoch konservierten Familie Serin/Arginin-reicher Spleißfaktoren gehören und konstitutive sowie alternative Spleißprozesse steuern und damit auf post-transkriptioneller Ebene die Genexpression regulieren. Mutation des Srpk79D-Gens durch die P-Element-Insertion (Srpk79DP1) oder eine Deletion im Gen (Srpk79DVN Nullmutante) führt zu auffälligen BRP-Akkumulationen in larvalen und adulten Nerven. In der vorliegenden Arbeit wird gezeigt, dass diese BRP-Akkumulationen auf Ultrastruktur-Ebene ausgedehnten axonalen Agglomeraten elektronendichter Bänder entsprechen und von klaren Vesikeln umgeben sind. Charakterisierung durch Immuno-Elektronenmikroskopie ergab, dass diese Strukturen BRP-immunoreaktiv sind. Um die Bildung BRP-enthaltender Agglomerate in Axonen zu verhindern und damit eine intakte Gehirnfunktion zu gewährleisten, scheint die SRPK79D nur auf niedrigem Niveau exprimiert zu werden, da die endogene Kinase mit verschiedenen Antikörpern nicht nachweisbar war. Wie in anderen Arbeiten gezeigt werden konnte, ist die Expression der PB-, PC- oder PF-Isoform der vier möglichen SRPK79D-Varianten, die durch alternativen Transkriptionsstart in Exon eins beziehungsweise drei und alternatives Spleißen von Exon sieben zustande kommen, zur Rettung des Phänotyps der BRP-Akkumulation im Srpk79DVN Nullmutanten-Hintergrund ausreichend. Zur Charakterisierung der Rescue-Eigenschaften der SRPK79D-PE-Isoform wurde mit der Klonierung der cDNA in einen UAS-Vektor begonnen. Offenbar beruht die Bildung der axonalen BRP-Agglomerate nicht auf einer Überexpression von BRP in den betroffenen Neuronen, denn auch bei reduzierter Expression des BRP-Proteins im Srpk79DVN Nullmutanten-Hintergrund entstehen die BRP-Agglomerate. In Köpfen der Srpk79DVN Nullmutante ist die Gesamtmenge an Bruchpilot-Protein im Vergleich zum Wildtyp nicht deutlich verändert. Auch die auf Protein-Ebene untersuchte Expression der verschiedenen Isoformen der präsynaptischen Proteine Synapsin, Sap47 und CSP weicht in der Srpk79DVN Nullmutante nicht wesentlich von der Wildtyp-Situation ab, sodass sich keine Hinweise auf verändertes Spleißen der entsprechenden prä-mRNAs ergeben. Jedes der sieben bekannten SR-Proteine von Drosophila ist ein potentielles Zielprotein der SRPK79D. Knock-down-Experimente für die drei hier untersuchten SR-Proteine SC35, X16/9G8 und B52/SRp55 im gesamten Nervensystem durch RNA-Interferenz zeigten allerdings keinen Effekt auf die Verteilung von BRP im Gewebe. Hinsichtlich der Flugfähigkeit der Tiere hat die Srpk79DVN Nullmutation keinen additiven Effekt zum Knock-down des BRP-Proteins, denn die Doppelmutanten zeigten bei der Bestimmung des Anteils an flugunfähigen Tieren vergleichbare Werte wie die Einzelmutanten, die entweder die Nullmutation im Srpk79D-Gen trugen, oder BRP reduziert exprimierten. Vermutlich sind Bruchpilot und die SR Proteinkinase 79D somit Teil desselben Signalwegs. Durch Doppelfärbungen mit Antikörpern gegen BRP und CAPA-Peptide wurde abschließend entdeckt, dass Bruchpilot auch im Median- und Transvers-Nervensystem (MeN/TVN) von Drosophila zu finden ist, welche die Neurohämal-Organe beherbergen. Aufgabe dieser Organe ist die Speicherung und Ausschüttung von Neuropeptid-Hormonen. Daher ist zu vermuten, dass das BRP-Protein neben Funktionen bei der Neurotransmitter-Exocytose möglicherweise eine Rolle bei der Ausschüttung von Neuropeptiden spielt. Anders als in den Axonen der larvalen Segmental- und Intersegmentalnerven der Srpk79DVN Nullmutante, die charakteristische BRP-Agglomerate aufweisen, hat die Mutation des Srpk79D-Gens in den Axonen der Va-Neurone, die das MeN/TVN-System bilden, keinen sichtbaren Effekt auf die Verteilung von Brp, denn das Muster bei Färbung gegen BRP weist keine deutlichen Veränderungen zum Wildtyp auf.
Spatial relationships between Cav channels and release sensors at active zones (AZs) are a major determinant of synaptic fidelity. They are regulated developmentally, but the underlying molecular mechanisms are largely unclear. Here, we show that Munc13-3 regulates the density of Cav2.1 and Cav2.2 channels, alters the localization of Cav2.1, and is required for the development of tight, nanodomain coupling at parallel-fiber AZs. We combined EGTA application and Ca2+-channel pharmacology in electrophysiological and two-photon Ca2+ imaging experiments with quantitative freeze-fracture immunoelectron microscopy and mathematical modeling. We found that a normally occurring developmental shift from release being dominated by Ca2+ influx through Cav2.1 and Cav2.2 channels with domain overlap and loose coupling (microdomains) to a nanodomain Cav2.1 to sensor coupling is impaired in Munc13-3-deficient synapses. Thus, at AZs lacking Munc13-3, release remained triggered by Cav2.1 and Cav2.2 microdomains, suggesting a critical role of Munc13-3 in the formation of release sites with calcium channel nanodomains.
In Nervensystemen bedürfen Informationsweitergabe und Gedächtnisformation eines präzisen Zusammenspiels von Synapsen in Zeit und Raum. Synaptische Transmission basiert strukturell auf mesoskopischen cytosolischen Kompartimenten an der präsynaptischen Membran, sogenannten Aktiven Zonen (AZ). Ihre Cytomatrix, bestehend aus zentralen Gerüstproteinen wie Rab3 interacting molecule (RIM), ermöglicht eine schnelle Freisetzung synaptischer Vesikel. Die Defizienz der lokal häufigsten Isoform RIM1α resultiert an einer komplexen zentralen Säugersynapse, die des hippocampalen Moosfaserboutons (MFB) zu im Cornu ammonis (CA)3 befindlichen Pyramidalzellen, in einer dezimierten Langzeitplastizität. Auf Verhaltensebene zeigen diese Mäuse eine reduzierte Lernfähigkeit.
Die vorliegende Dissertation widmet sich grundlegend der bisher unbekannten dreidimensionalen (3D) AZ-Ultrastruktur des MFB in akuten Hippocampusschnitten der adulten Wildtyp- und RIM1α-Knock-Out-Maus (RIM1α\(^{-/-}\)). In einer methodischen Entwicklungsphase wurde ein neuartiges, anspruchsvolles Protokoll der nahezu artefaktfreien (near to native) Synapsenpräparation am MFB mittels Hochdruckgefrierung und Gefriersubstitution sowie der 3D-Modellierung mittels Elektronentomographie etabliert. In einer zweiten Experimentier- und Analysephase ermöglichte die hochwertige synaptische Gewebeerhaltung in beiden Genotypen eine standardisierte, auf Programmierskripten basierte Quantifizierung der AZ-Ultrastruktur bis auf die Ebene eines individuell gedockten synaptischen Vesikels.
Dieser Dissertation gelingt der Nachweis, dass eine Defizienz von RIM1α zu einer multidimensionalen ultrastrukturellen Veränderung der AZ und ihres Vesikelpools am MFB führt. Neben einer Reduktion, Dezentralisierung und strukturellen Veränderung (eng) gedockter Vesikel – der ultrastrukturellen Messgrößen von unmittelbar freisetzungsfähigen Vesikeln – verdichtet sich der distaler lokalisierte Vesikelpool auf zugleich größeren, heterogenen AZ-Flächen mit erweitertem synaptischem Spalt. Vorliegende Untersuchungen tragen zum Verständnisgewinn über eine zentrale Rolle von RIM1α für das Docking und die Organisation von Vesikeln der AZ im MFB bei. Darüber hinaus stellen die präzisen ultrastrukturellen Analysen eine morphologische Grundlage für weiterführende Studien mit Hilfe modernster Techniken dar, beispielsweise über die Auswirkungen der geänderten RIM1α\(^{-/-}\) AZ-Ultrastruktur auf die präsynaptische Plastizität sowie in Korrelation zum Gedächtnis und Lernen der Tiere.
Ultrastructural analysis of wild-type and RIM1α knockout active zones in a large cortical synapse
(2022)
Rab3A-interacting molecule (RIM) is crucial for fast Ca\(^{2+}\)-triggered synaptic vesicle (SV) release in presynaptic active zones (AZs). We investigated hippocampal giant mossy fiber bouton (MFB) AZ architecture in 3D using electron tomography of rapid cryo-immobilized acute brain slices in RIM1α\(^{−/−}\) and wild-type mice. In RIM1α\(^{−/−}\), AZs are larger with increased synaptic cleft widths and a 3-fold reduced number of tightly docked SVs (0–2 nm). The distance of tightly docked SVs to the AZ center is increased from 110 to 195 nm, and the width of their electron-dense material between outer SV membrane and AZ membrane is reduced. Furthermore, the SV pool in RIM1α\(^{−/−}\) is more heterogeneous. Thus, RIM1α, besides its role in tight SV docking, is crucial for synaptic architecture and vesicle pool organization in MFBs.
The second messenger cyclic AMP (cAMP) plays an important role in synaptic plasticity. Although there is evidence for local control of synaptic transmission and plasticity, it is less clear whether a similar spatial confinement of cAMP signaling exists. Here, we suggest a possible biophysical basis for the site-specific regulation of synaptic plasticity by cAMP, a highly diffusible small molecule that transforms the physiology of synapses in a local and specific manner. By exploiting the octopaminergic system of Drosophila, which mediates structural synaptic plasticity via a cAMP-dependent pathway, we demonstrate the existence of local cAMP signaling compartments of micrometer dimensions within single motor neurons. In addition, we provide evidence that heterogeneous octopamine receptor localization, coupled with local differences in phosphodiesterase activity, underlies the observed differences in cAMP signaling in the axon, cell body, and boutons.
Single-molecule localization microscopy (SMLM) greatly advances structural studies of diverse biological tissues. For example, presynaptic active zone (AZ) nanotopology is resolved in increasing detail. Immunofluorescence imaging of AZ proteins usually relies on epitope preservation using aldehyde-based immunocompetent fixation. Cryofixation techniques, such as high-pressure freezing (HPF) and freeze substitution (FS), are widely used for ultrastructural studies of presynaptic architecture in electron microscopy (EM). HPF/FS demonstrated nearer-to-native preservation of AZ ultrastructure, e.g., by facilitating single filamentous structures. Here, we present a protocol combining the advantages of HPF/FS and direct stochastic optical reconstruction microscopy (dSTORM) to quantify nanotopology of the AZ scaffold protein Bruchpilot (Brp) at neuromuscular junctions (NMJs) of Drosophila melanogaster. Using this standardized model, we tested for preservation of Brp clusters in different FS protocols compared to classical aldehyde fixation. In HPF/FS samples, presynaptic boutons were structurally well preserved with ~22% smaller Brp clusters that allowed quantification of subcluster topology. In summary, we established a standardized near-to-native preparation and immunohistochemistry protocol for SMLM analyses of AZ protein clusters in a defined model synapse. Our protocol could be adapted to study protein arrangements at single-molecule resolution in other intact tissue preparations.
Neurotransmitter release is stabilized by homeostatic plasticity. Presynaptic homeostatic potentiation (PHP) operates on timescales ranging from minute- to life-long adaptations and likely involves reorganization of presynaptic active zones (AZs). At Drosophila melanogaster neuromuscular junctions, earlier work ascribed AZ enlargement by incorporating more Bruchpilot (Brp) scaffold protein a role in PHP. We use localization microscopy (direct stochastic optical reconstruction microscopy [dSTORM]) and hierarchical density-based spatial clustering of applications with noise (HDBSCAN) to study AZ plasticity during PHP at the synaptic mesoscale. We find compaction of individual AZs in acute philanthotoxin-induced and chronic genetically induced PHP but unchanged copy numbers of AZ proteins. Compaction even occurs at the level of Brp subclusters, which move toward AZ centers, and in Rab3 interacting molecule (RIM)-binding protein (RBP) subclusters. Furthermore, correlative confocal and dSTORM imaging reveals how AZ compaction in PHP translates into apparent increases in AZ area and Brp protein content, as implied earlier.
The active zone (AZ) protein Bruchpilot (Brp) is essential for rapid glutamate release at Drosophila melanogaster neuromuscular junctions (NMJs). Quantal time course and measurements of action potential-waveform suggest that presynaptic fusion mechanisms are altered in brp null mutants (brp\(^{69}\)). This could account for their increased evoked excitatory postsynaptic current (EPSC) delay and rise time (by about 1 ms). To test the mechanism of release protraction at brp\(^{69}\) AZs, we performed knock-down of Synaptotagmin-1 (Syt) via RNAi (syt\(^{KD}\)) in wildtype (wt), brp\(^{69}\) and rab3 null mutants (rab3\(^{rup}\)), where Brp is concentrated at a small number of AZs. At wt and rab3\(^{rup}\) synapses, syt\(^{KD}\) lowered EPSC amplitude while increasing rise time and delay, consistent with the role of Syt as a release sensor. In contrast, syt\(^{KD}\) did not alter EPSC amplitude at brp\(^{69}\) synapses, but shortened delay and rise time. In fact, following syt\(^{KD}\), these kinetic properties were strikingly similar in wt and brp\(^{69}\), which supports the notion that Syt protracts release at brp\(^{69}\) synapses. To gain insight into this surprising role of Syt at brp\(^{69}\) AZs, we analyzed the structural and functional differentiation of synaptic boutons at the NMJ. At tonic type Ib motor neurons, distal boutons contain more AZs, more Brp proteins per AZ and show elevated and accelerated glutamate release compared to proximal boutons. The functional differentiation between proximal and distal boutons is Brp-dependent and reduced after syt\(^{KD}\). Notably, syt\(^{KD}\) boutons are smaller, contain fewer Brp positive AZs and these are of similar number in proximal and distal boutons. In addition, super-resolution imaging via dSTORM revealed that syt\(^{KD}\) increases the number and alters the spatial distribution of Brp molecules at AZs, while the gradient of Brp proteins per AZ is diminished. In summary, these data demonstrate that normal structural and functional differentiation of Drosophila AZs requires concerted action of Brp and Syt.
Aktive Zonen (AZs) sind hoch spezialisierte, subzelluläre Kompartimente von Neuronen, die der synaptischen Übertragung dienen. Sie enthalten Gerüstproteine wie RIM (Rab3 interacting molecule) sowie elektronendichte Projektionen bestehend aus Bruchpilot bei Drosophila melanogaster oder Bassoon im Säuger, welche Schlüsselkomponenten des Vesikelverkehrs darstellen. Bei der Fliege sind Anzahl und Verteilung von Bruchpilot-Molekülen in AZs relevant für die funktionelle Differenzierung. Ihre Anordnung wird im Abstand von weniger als einem Mikrometer innerhalb einer präsynaptischen Endigung reguliert.
Im Rahmen der vorliegenden Arbeit wurden elektrophysiologische Ableitungen und konfokale sowie höchstauflösende, immunhistochemische Bildgebung mit dem dSTORM (direct Stochastic Optical Reconstruction Microscopy) Verfahren an larvalen, neuromuskulären Synapsen von Drosophila durchgeführt. Dabei wurde das genetische Potenzial des Modellorganismus genutzt, um relevante Proteinfunktionen und -interaktionen zu analysieren.
RIM als zentrale Komponente Aktiver Zonen ist relevant für synaptische Plastizität. Eine als CORD7 (cone-rod dystrophy type 7) bezeichnete Punktmutation (Arginin zu Histidin) innerhalb der 310 Helix der C2A-Domäne von RIM wurde mit erhöhten kognitiven Fähigkeiten einer Patientengruppe in Verbindung gebracht. Weil die Drosophila C2A-Domäne eine hohe Homologie zur Säugerdomäne aufweist, konnte der Einfluss dieser Mutation auf Struktur und Funktion von Synapsen untersucht werden. Es zeigte sich, dass der Aminosäureaustausch der CORD7-Position und des benachbarten Arginin-Restes die synaptische Organisation und Transmission beeinflussen.
In einer Reihe weiterer Experimente wurde das Zusammenspiel von Bruchpilot und Synaptotagmin, dem Calciumsensor der evozierten Transmitterfreisetzung, analysiert. Während AZs ohne Bruchpilot auch ohne Synaptotagmin funktionieren, führt dessen Reduktion zu einer Umverteilung von Bruchpilot-Molekülen innerhalb von AZs und zu dramatischen Änderungen in ihrer Anzahl. Abschließend wurde so ein Beitrag zum Verständnis der molekularen Organisation synaptischer Informationsverarbeitung und Plastizität geleistet, wobei zu klären bleibt, wie die zuverlässige Speicherung von Informationen an AZs erreicht werden kann.
Ziel dieser Arbeit war es, strukturelle Veränderungen präsynaptischer Aktiver Zonen als mögliches Korrelat synaptischer Plastizität zu detektieren. Damit soll die Hypothese getestet werden, dass strukturelle Plastizität Aktiver Zonen eine zentrale Rolle bei der Informationsverarbeitung im Gehirn und bei Lern- und Gedächtnisprozessen spielt. Dazu war es notwendig Methoden zu etablieren, die die strukturelle Analyse Aktiver Zonen und deren Veränderung in vitalem Gewebe ermöglichen. Um die Untersuchungen in einem Gewebe mit plastischen Eigenschaften durchzuführen, wurden Methoden zur Herstellung organotypischer hippocampaler Hirnschnittkulturen etabliert, da hippokampale Moosfasersynapsen ausgeprägte präsynaptische Plastizität aufweisen (Bliss und Collingridge, 1993). Durch Einzelzellelektroporation wurde es möglich, individuelle Neurone mit Transgenen zur Markierung der gesamten Zelle (DsRed) und synaptischer Substrukturen wie Aktive Zonen (z.B.: GFP-CAST, einem Fluorophor-markierten AZ-Protein) zu transfizieren. Mit konfokaler Bildgebung transfizierter Zellen konnten strukturierte Anreicherungen von GFP-CAST in Moosfaserboutons dargestellt werden. Konfokale Bildgebung von Doppelimmunfluoreszenzfärbungen zur detaillierten Analyse der Proteinlokalisation zeigte ein diffraktionsbedingtes Auflösungsdefizit, das auch durch die Anwendung von STED-Mikroskopie nicht zufriedenstellend gelöst werden konnte. Um eine präzise Karte synaptischer Proteine zu erstellen, wurde hochauflösende Mikroskopie (dSTORM) mit einer lateralen räumlichen Auflösung von 20 nm etabliert. Dabei erwiesen sich die ausgeprägte Plastizität, die hohe Dichte an Aktiven Zonen und die variable Gestalt der Boutons im hippokampalen Präparat als problematisch. Aus diesem Grund wurde die elektronenmikroskopisch gut charakterisierte neuromuskuläre Endplatte mit ihrer symmetrischen molekularen Struktur als Präparat für dSTORM verwendet. An der Endplatte konnte die molekulare Organisation der Aktiven-Zonen-Proteine Piccolo und Bassoon dargestellt werden. Zudem konnten erstmals die Mündungen postsynaptischer Falten lichtmikroskopisch aufgelöst werden. So gelang es Werkzeuge zu etablieren, die mit lichtmikroskopischen Methoden die Darstellung der Architektur Aktiver Zonen mit molekularer Auflösung ermöglichen. Die Herausforderung wird es sein, diese neue Dimension in funktionellem Kontext zu nutzen. Die experimentellen Grundlagen dazu wurden durch eine spezielle Badkammer und die Etablierung von Rollertubekulturen bereits gelegt. Dabei ermöglicht dSTORM die Adressierung quantitativer Fragestellungen bis hin zur Bestimmung der Molekülanzahl.
Revealing the molecular organization of anatomically precisely defined brain regions is necessary for refined understanding of synaptic plasticity. Although three-dimensional (3D) single-molecule localization microscopy can provide the required resolution, imaging more than a few micrometers deep into tissue remains challenging. To quantify presynaptic active zones (AZ) of entire, large, conditional detonator hippocampal mossy fiber (MF) boutons with diameters as large as 10 mu m, we developed a method for targeted volumetric direct stochastic optical reconstruction microscopy (dSTORM). An optimized protocol for fast repeated axial scanning and efficient sequential labeling of the AZ scaffold Bassoon and membrane bound GFP with Alexa Fluor 647 enabled 3D-dSTORM imaging of 25 mu m thick mouse brain sections and assignment of AZs to specific neuronal substructures. Quantitative data analysis revealed large differences in Bassoon cluster size and density for distinct hippocampal regions with largest clusters in MF boutons. Pauli et al. develop targeted volumetric dSTORM in order to image large hippocampal mossy fiber boutons (MFBs) in brain slices. They can identify synaptic targets of individual MFBs and measured size and density of Bassoon clusters within individual untruncated MFBs at nanoscopic resolution.
During my PhD I studied two principal biological aspects employing Drosophila melanogaster. Therefore, this study is divided into Part I and II.
Part I: Bruchpilot and Complexin interact to regulate synaptic vesicle tethering to the
active zone cytomatrix
At the presynaptic active zone (AZ) synaptic vesicles (SVs) are often physically linked to an electron-dense cytomatrix – a process referred to as “SV tethering”. This process serves to concentrate SVs in close proximity to their release sites before contacting the SNARE complex for subsequent fusion (Hallermann and Silver, 2013). In Drosophila, the AZ protein Bruchpilot (BRP) is part of the proteinous cytomatrix at which SVs accumulate (Kittel et al., 2006b; Wagh et al., 2006; Fouquet et al., 2009). Intriguingly, truncation of only 1% of the C-terminal region of BRP results in a severe defect in SV tethering to this AZ scaffold (hence named brpnude; Hallermann et al., 2010b).
Consistent with these findings, cell-specific overexpression of a C-terminal BRP fragment, named mBRPC-tip (corresponds to 1% absent in brpnude; m = mobile) phenocopied the brpnude mutant in behavioral and functional experiments. These data indicate that mBRPC-tip suffices to saturate putative SV binding sites, which induced a functional tethering deficit at motoneuronal AZs. However, the molecular identity of the BRP complement to tether SVs to the presynaptic AZ scaffold remains unknown. Moreover, within larval motoneurons membrane-attached C-terminal portions of BRP were sufficient to tether SVs to sites outside of the AZ. Based on this finding a genetic screen was designed to identify BRP interactors in vivo. This screen identified Complexin (CPX), which is known to inhibit spontaneous SV fusion and to enhance stimulus evoked SV release (Huntwork and Littleton, 2007; Cho et al., 2010; Martin et al., 2011). However, so far CPX has not been associated with a function upstream of priming/docking and release of SVs. This work provides morphological and functional evidence, which suggests that CPX promotes recruitment of SVs to the AZ and thereby curtails synaptic short-term depression. Together, the presented findings indicate a functional interaction between BRP and CPX at Drosophila AZs.
Part II: The Adhesion-GPCR Latrophilin/CIRL shapes mechanosensation
The calcium independent receptor of α-latrotoxin (CIRL), also named Latrophilin, represents a prototypic Adhesion class G-protein coupled-receptor (aGPCR). Initially, Latrophilin was identified based on its capacity to bind the α-component of latrotoxin (α-LTX; Davletov et al., 1996; Krasnoperov et al., 1996), which triggers massive exocytotic activity from neurons of the peripheral nervous system (Scheer et al., 1984; Umbach et al., 1998; Orlova et al., 2000). As a result Latrophilin is considered to play a role in synaptic transmission. Later on, Latrophilins have been associated with other biological processes including tissue polarity (Langenhan et al., 2009), fertility (Prömel et al., 2012) and synaptogenesis (Silva et al., 2011). However, thus far its subcellular localization and the identity of endogenous ligands, two aspects crucial for the comprehension of Latrophilin’s in vivo function, remain enigmatic.
Drosophila contains only one latrophilin homolog, named dCirl, whose function has not been investigated thus far.
This study demonstrates abundant dCirl expression throughout the nervous system of Drosophila larvae. dCirlKO animals are viable and display no defects in development and neuronal differentiation. However, dCirl appears to influence the dimension of the postsynaptic sub-synaptic reticulum (SSR), which was accompanied by an increase in the postsynaptic Discs-large abundance (DLG). In contrast, morphological and functional properties of presynaptic motoneurons were not compromised by the removal of dCirl. Instead, dCirl is required for the perception of mechanical challenges (acoustic-, tactile- and proprioceptive stimuli) through specialized mechanosensory devices, chordotonal organs (Eberl, 1999). The data indicate that dCirl modulates the sensitivity of chordotonal neurons towards mechanical stimulation and thereby adjusts their input-output relation. Genetic interaction analyses suggest that adaption of the molecular mechanotransduction machinery by dCirl may underlie this process. Together, these results uncover an unexpected function of Latrophilin/dCIRL in mechanosensation and imply general modulatory roles of aGPCR in mechanoception.
Chemical synapses are a physically and functionally varied type of cell-cell contact specialized in conducting communication between neurons. They are the smallest "computational" unit of the brain and are often classified as electrical and chemical, and they can be distinguished based on their transmission mechanism. These categories could be further broken into many kinds, each having a specific structure-function repertoire that is hypothesized to provide neural networks with distinct computational capabilities. Heterogeneity refers to the variety of structures and functions present in a particular category of synapses. Contributing factors for this heterogeneity may be the synaptic vesicles, the active zone (AZ), the synaptic cleft, the postsynaptic density, and the glial processes associated with the synaptic contacts. Each of these five structural modules has its own set of functions, and their combination determines the spectrum of functional heterogeneity at mammalian excitatory synapses. This work focused on the changes in AZ protein expression after chemical induction of plasticity with forskolin in synaptic contacts of the hippocampal mossy fibers. With the nanoscopic resolution provided by dSTORM, along with the multicolor SIM imaging capabilities, changes in expression of key presynaptic AZ components were analyzed. Using SIM imaging along with a standardized stimulation protocol in acute brain slices from male 16-week old Thy1-mEGFP (Lsi1) mice, the changes of the key AZ proteins Bassoon, Munc 13-1 and Tomosyn were investigated 30 min after stimulation with forskolin (50 μM for 30 min). Forskolin induced changes in these proteins largely in small synaptic contacts whereas no clear changes were detected in large mossy fiber boutons. However, due to the high variability it cannot be ruled out that forskolin may differentially modify AZ protein composition depending on experimental circumstances such as age and gender of mice or the time point and duration of forskolin stimulation. The dSTORM data demonstrated feasibility to perform single molecule 3D imaging of hippocampal presynaptic AZs and allowed quantitative mapping of molecular changes in AZ proteins after induction of plasticity. The findings suggest high heterogeneity in mossy fiber synaptic contacts that may have an impact on the function of neural networks. These imaging approaches may now be used to identify potential differences in functional molecular rearrangements of synaptic proteins in healthy and diseased brain (e.g. after induction of traumatic brain injury).