Die Rolle der nicht-kodierenden RNAs miR-26 und \(Malat1\) bei der \(in\) \(vitro\) Differenzierung zu Neuronen / The role of the non-coding RNAs miR-26 and \(Malat1\) during \(in\) \(vitro\) neuronal differentiation

Was [geb. Houben], Nina

January 2023

Während der embryonalen Neurogenese spielt die Repression neuraler Gene in nicht neuralen Zellen, sowie in neuralen Vorläuferzellen durch den REST (repressor element silencing transcription factor)-Komplex eine wichtige Rolle. Durch die schrittweise Inaktivierung diese Komplexes im Verlauf der Differenzierung werden neurale Genexpressionsprogramme gesteuert. Zusätzlich kommt bei der Kontrolle der räumlichen und zeitlichen Regulation der Genexpression während der Neurogenese verschiedenen miRNAs eine wichtige Rolle zu. So konnte in vorangegangenen Arbeiten im Zebrafischen gezeigt werden, dass miR-26b die Transkription eines wichtigen Effektorproteins des REST-Komplexes, CTDSP2 (C-terminal domain small phosphatases), während der Neurogenese negativ reguliert. Da darüber hinaus die miR-26 Repression zu einer stark verminderten neuronalen Differenzierung führte, kommt diesem regulatorischen Schaltkreis eine zentrale Rolle bei der Neurogenese im Zebrafisch zu. Die zusammen mit ihren Ctdsp-Wirtsgenen koexprimierte miR-26 Familie liegt in Vertebraten evolutionär hoch konserviert vor. Analog zum Zebrafisch konnte im murinen in vitro ES-Zell Differenzierungssystem gezeigt werden, dass miR-26 die Expression von Ctdsp2 reprimiert. Weiterhin konnte in diesem System gezeigt werden, dass auch Rest ein miR-26 Zielgen ist und dass der Verlust der miR-26 zu einem Arrest der differenzierenden Zellen im neuronalen Vorläuferstadium führt. Zusammengenommen deuten diese vorangegangenen Arbeiten auf eine zentrale Rolle der miR-26 während der Neurogenese hin. Die hier vorgestellte Arbeit zielte zunächst darauf ab die Regulation des REST-Komplexes durch die miR-26 auf molekularer Ebene besser zu verstehen. Der Verlust der miR-26 Bindestelle in der Ctdsp2 mRNA führte zu einer erhöhten Ctdsp2 Expression, beeinflusste aber nicht die terminale Differenzierung zu Neuronen. Im Gegensatz hierzu führte der Verlust der miR-26 Bindestelle in der Rest mRNA zu einem Arrest der Differenzierung im neuralen Vorläuferzellstadium. Zellen in denen die miR-26 Bindestelle in Rest deletiert war, zeigten zudem, genau wie miR-26 knockout (KO) Zellen, eine erhöhte Expression von REST-Komplex Komponenten, sowie eine verringerte Expression von REST-regulierten miRNAs. Zusammengenommen weisen diese Daten daraufhin, dass während der Neurogenese im Säugersystem die Inaktivierung von Rest durch miR-26 für die Maturierung von Neuronen eine zentrale Rolle spielt. Ein weiterer Fokus dieser Arbeit lag auf der Regulation der miR-26 Expression während der Neurogenese. Vorangegangene Arbeiten in nicht-neuronalen Zelltypen identifizierten die lnc (long-non-coding) RNA Malat1 als eine ce (competitive endogenous) RNA der miR-26. Um den Einfluss von Malat1 auf die miR-26 Expression während der Neurogenese zu untersuchen, wurde zunächst mittels CRISPR/Cas9 der vollständige Malat1-Lokus in ESCs deletiert. Der Verlust von Malat1 führte zu einer erhöhten Expression der miR-26 Familienmitglieder sowie deren Ctdsp-Wirtsgene. Weiterhin war die Proliferation von Malat1 KO neuronalen Vorläuferzellen stark vermindert, was mit einer Erhöhung der Frequenz seneszenter Zellen einherging. Durch die Inaktivierung von miR-26 in differenzierenden Malat1 KO ESCs konnte dieser proliferative Phänotyp aufgehoben werden. Darüber hinaus konnte eine verstärkte neuronale Differenzierung dieser Zellen beobachtet werden. Zusammenfassend zeigen diese Daten, dass neben der Regulation des REST-Komplexes durch miR-26 auch die Kontrolle des Zellzyklus über die Malat1-vermittelte Regulation der miR-26 in neuronalen Vorläuferzellen einen kritischen Schritt bei der Differenzierung von neuronalen Vorläuferzellen zu maturen Neuronen darstellt. / During embryonic neurogenesis, repression of neural genes in non-neural cells, as well as in neural progenitor cells by the REST (repressor element silencing transcription factor) complex, plays an important role. The gradual inactivation of this complex during differentiation controls neural gene expression programs. In addition, different miRNAs play important roles in controlling the spatial and temporal regulation of gene expression during neurogenesis. For example, previous work in zebrafish demonstrated that miR-26b negatively regulates the transcription of a key effector protein of the REST complex, CTDSP2 (C-terminal domain small phosphatases), during neurogenesis. Since miR-26 repression also resulted in severely reduced neuronal differentiation, this regulatory circuit plays a central role in zebrafish neurogenesis. The miR-26 family, co-expressed with its Ctdsp host genes, is evolutionarily highly conserved in vertebrates. Analogous to zebrafish, miR-26 was shown to repress Ctdsp2 expression in a murine in vitro ESC differentiation system. Furthermore, in this system, it was shown that Rest is also a miR-26 target and that loss of miR-26 leads to arrest of differentiating cells at the neuronal progenitor stage. Taken together, these previous analyses suggest a central role for miR-26 during neurogenesis. The work presented here first aimed to better understand the regulation of the REST complex by miR-26 at the molecular level. Loss of the miR-26 binding site in Ctdsp2 mRNA increased Ctdsp2 expression but did not affect terminal differentiation into neurons. In contrast, loss of the miR-26 binding site in the Rest mRNA resulted in arrest of differentiation at the neural progenitor cell stage. Cells in which the miR-26 binding site was deleted in Rest also showed increased expression of REST complex components, as well as decreased expression of RESTregulated miRNAs, just like miR-26 knockout (KO) cells. Taken together, these data indicate that during mammalian neurogenesis, inactivation of REST by miR-26 plays a central role in the maturation of mammalian neurons. Another focus of this work was on the regulation of miR-26 expression during neurogenesis. Previous analyses in non-neuronal cell types identified the lnc(long-non-coding)RNA Malat1 as a ce(competitive endogenous)RNA of miR-26. To investigate the effect of Malat1 on miR-26 expression during neurogenesis, the complete Malat1 locus was deleted in ESCs using CRISPR/Cas9. Loss of Malat1 resulted in increased expression of miR-26 family members as well as their Ctdsp host genes. Furthermore, proliferation of Malat1 KO neural progenitor cells was greatly reduced, which was accompanied by an increase in the frequency of senescent cells. Inactivation of miR-26 in differentiating Malat1 KO ESCs abrogated this proliferative phenotype. In addition, increased neuronal differentiation of these cells was observed. In conclusion, these data demonstrate that in addition to regulation of the REST complex by miR-26, cell cycle control via Malat1-mediated regulation of miR-26 in neuronal progenitor cells is a critical step for the differentiation of neuronal progenitor cells into mature neurons.

Neurogenese

Non-coding RNA

embryonale Stammzelle

ddc:570

Endotheliale Stickstoffmonoxidsynthase (NOS-III) reguliert die Proliferation neuraler Stammzellen im adulten Gyrus dentatus / Endothelial nitric oxide synthase (NOS-III) regulates the proliferation of neural stem cells in the adult dentate gyrus

Wycislo, Matthias

January 2007

Die Proliferation von in der Subgranulärzone des Gyrus dentatus ansässigen neuralen Stammzellen ist der erste Schritt der Neuentstehung von Nervenzellen im adulten Organismus, der so genannten adulten Neurogenese, die in bestimmten neurogenen Nischen des ZNS von Säugetieren und des Menschen vorkommt. Die vorliegende Arbeit zeigt, dass das Enzym endotheliale Stickstoffmonoxidsynthase (NOS-III bzw. eNOS) bzw. durch NOS-III gebildetes Stickstoffmonoxid (NO) die Proliferation neuraler Stamm- bzw. Vorläuferzellen im Gyrus dentatus des Hippokampus positiv reguliert, da Mäuse, bei denen das Gen für dieses Enzym deletiert ist, über eine signifikant erniedrigte Stammzellproliferation verfügen. NOS-III-Knockout-Mäuse zeigen außerdem erhöhte Volumina von Substrukturen des Gyrus dentatus. Biometrische Faktoren, wie z. B. Alter, Geschlecht, Körpergewicht, Umgebungsbedingungen, hatten dagegen keinen signifikanten Einfluss auf die adulte Neurogenese. Die Abnahme der adulten Neurogenese bei NOS-III-Knockout-Tieren ist fast vollständig auf die Reduktion der Stammzellproliferation in der Subgranulärzone des Gyrus dentatus zurückzuführen. Ein Netto-Zuwachs an neu gebildeten Neuronen 4 Wochen nach Proliferation kann jedoch durch NOS-III nicht bewirkt werden, was auf eine komplexe Regulation der adulten Neurogenese hinweist. Die Stammzellproliferation im adulten murinen Gyrus dentatus wird jedoch vermutlich unter anderem über im Endothel gebildetes NO (als gasförmiges, parakrines Signalmolekül) vermittelt. / The proliferation of neural stem cells residing in the subgranular layer of the dentate gyrus represents the first step in the formation of new neurons in the adult organism, the so-called adult neurogenesis that occurs in certain neurogenic niches of the mammalian as well as human CNS. The present work shows that endothelial nitric oxide synthase (NOS-III or eNOS) and nitric oxide (NO) formed by NOS-III, respectively, positively regulate the proliferation of neural stem- or precursor cells in the dentate gyrus of the hippocampus since NOS-III knockout mice (NOS III -/-) show significantly reduced stem cell proliferation. Moreover, NOS-III knockout mice exhibit increased volumina of dentate gyrus substructures. In contrast, biometric factors like age, gender, body mass and environmental conditions did not influence adult neurogenesis significantly. Mainly, the decrease of adult neurogenesis in NOS-III knockout animals is attributable to the reduction of stem cell proliferation in the subgranular zone of the dentate gyrus. However, a net increase of new neurons 4 weeks after proliferation cannot be produced by NOS-III pointing to a complex regulation of adult neurogenesis. Yet, stem cell proliferation in the murine dentate gyrus is presumambly mediated inter alia by NO as a gaseous, paracrine molecule produced in the endothelium.

Neurogenese

Stickstoffmonoxid

Stickstoffmonoxid-Synthase

Gyrus dentatus

Hippocampus

ddc:610

Untersuchungen zum in vivo Differenzierungspotenzial muriner und humaner hämatopoetischer sowie muriner neuraler Stammzellen / Analysis of the in vivo differentiation potential of murine and human hematopoietic as well as murine neural stem cells

Harder, Friedrich

January 2002

Zusammenfassung Im Zuge der Säugerentwicklung entsteht aus der totipotenten Eizelle ein Organismus aus mehr als 200 verschiedenen Zelltypen. Dabei wird die Entwicklung und der Erhalt des Tieres von Stammzellen gewährleistet. Während der Embryonalentwicklung gibt es nur transient vorkommende Stammzelltypen, während der adulte Körper die Homoeostase mittels permanent vorhandener somatischer Stammzellen aufrechterhält. Als kennzeichnend für die somatischen Stammzellen galt, dass sie nur die Zellen ihres Gewebes ersetzen können. In der vorliegenden Arbeit wurde untersucht, ob SSZ tatsächlich auf die Bildung von Zellen ihres Stammzellkompartiments beschränkt sind. Dazu wurden drei verschiedene Stammzelltypen, murine hämatopoetische und humane HSZ sowie murine NSZ in murine Präimplantationsblastozysten injiziert. Da dies die Zellen mit einer Umgebung exponiert, von der die Bildung aller Zelltypen des erwachsenen Tieres ausgeht. Es konnte gezeigt werden, dass zur Mitte der Schwangerschaft Nachkommen aller drei injizierten Stammzelltypen sich präferentiell in den fötalen hämatopoetischen Geweben befinden. Für humane hämatopoetische und murine NSZ wurde gezeigt, dass diese hämatopoetische Vorläufer in hämatopoetischen Geweben der Embryonen bilden, sowie dass Nachkommen dieser Zellen ein erythroides Genexpressionsmuster aktivieren. Der Vergleich adulter chimärer Tiere zeigte, dass HSZ zu nahezu gleichen Teilen neurale und hämatopoetische Gewebe besiedelt hatten. Nachkommen neuraler Stammzellen dagegen vor allem in neuralen Geweben adulter Tiere gefunden wurden. Aus diesen Ergebnisssen lässt sich ableiten, dass SSZ durch die Exposition mit der frühen embryonalen Mikroumgebung zur Bildung heterologer Zelltypen angeregt werden können. Außerdem demonstrieren diese Ergebnisse das unterschiedliche Entwicklungspotenzial von HSZ und NSZ und grenzen es gegenüber dem pluripotenten Differenzierungspotenzial von ES-Zellen ab. / Summary During mammalian ontogeny an organism develops from a totipotent zygot that is composed of more than 200 distinct cell types. The development and the maintanance of the organism is dependent on somatic stem cells. Transient stem cell types exist during early embryonic development, but homoestasis of the adult is maintained by resident somatic stem cells. The restriction in committent to the exclusive generation of cells of their own stem cell system was considered as a hallmark of adult stem cells. The objective of the present thesis was to investigate whether somatic stem cells are truly restricted to the generation of cells belonging to their own stem cell system only. To this end three somatic stem cell types, murine hematopoietic, human hematopoietic and murine neural stem cells were injected into murine blastocysts. The blastocysts provides the injected stem cells with a microenvironment permissive for the generation of all cell types of the adult organism. It could be shown using this method that progeny of murine and human hematopoietic and murine neural stem cells preferentially engrafted the hematopoietic tissues of the developing embryo. Furthermore, injection of human hematopoietic and murine neural stem cells gave rise to hematopoietic progenitors cells in fetal hematopoietic tissues, and generated cells with an erythroid gene expression pattern. Comparison of adult chimeric animals revealed that progeny of hematopoietic stem cells had engrafted hematopoietic and neural tissues to a similar extent, whereas progeny of neural stem cells was preferentially detected in neural tissues. This result indicates, that somatic stem cells can generate heterologous cells if exposed to the early embryonic environment. Furthermore, it demonstrates the distinct and different developmental potentials of hematopoietic and neural stem cells and and distinguishes them from the pluripotent differentiation potential of ES-cells.

Maus

Mensch

Stammzelle

Neurogenese

Blutstammzelle

Zelldifferenzierung

ddc:570

CHARACTERISATION OF Y-BOX PROTEIN 3 (MSY3) IN THE DEVELOPING MURINE CENTRAL NERVOUS SYSTEM

Grzyb, Anna Natalia

26 March 2007

Neurons, astrocytes and oligodendrocytes of the central nervous system (CNS) arise from a common pool of multipotent neuroepithelial progenitor cells lining the walls of the neural tube. Initially, neuroepithelial cells undergo symmetric proliferative divisions, thereby expanding the progenitor pool and determining the size of brain compartments. At the onset of neurogenesis, a subset of progenitors switch to asymmetric or terminal symmetric neurogenic divisions. Maintenance of progenitor cell population throughout the period of neurogenesis is essential to generate the full diversity of neuronal cell types and proper histological pattern. However, the mechanisms responsible for the maintenance of progenitor cells proliferation are far from being fully understood. The family of Y-box proteins is involved in control of proliferation and transformation in various normal and pathological cellular systems, and therefore was considered as a candidate to exert such a function. Y-box proteins have a capacity to bind DNA and RNA, thereby controlling gene expression from transcription to translation. This study aimed to examine the expression of mouse Y-box protein 3 (MSY3) in the developing nervous system and elucidate its putative role in regulation of proliferation of progenitor cells. As presented in this work, the MSY3 protein in the embryonic CNS is expressed solely in progenitor cells and not neurons. Moreover, as shown by two independent approaches: morphologically, i.e. using immunofluorescence and confocal microscopy, and biochemically, MSY3 expression is downregulated concomitantly with the spatiotemporal progression of neurogenesis. Interestingly, in preliminary results it was shown that MSY3 is expressed in Dcx-positive transient amplifying precursors in germinal zones of the adult brain, and in EGF-dependent neurospheres. To evaluate whether MSY3 could regulate the neurogenesis, the levels of the MSY3 protein in the progenitors were acutely downregulated or elevated by electroporation of RNAi or MSY3 expression plasmids, respectively. Neither premature reduction of MSY3 in the neuroepithelium (E9.5-E11.5) nor prolonged expression at the developmental stage when this protein is endogenously downregulated (E10.5-14.5) did affect proliferation versus the cell cycle exit of progenitors. Moreover, in Notch1-deficient progenitors in the cerebellar anlage, which exhibit precocious differentiation, MSY3 was not prematurely downregulated, suggesting that MSY3 also is not an early marker of differentiation. Differential centrifugation, immunoprecipitation and polysomal analysis performed in this study revealed that the MSY3 protein in the developing embryo, as well as in Neuro-2A cells, is associated with RNA. On a sucrose density gradient MSY3 co-fractionates with ribosomes and actively translating polysomes, suggesting that it might have a role in regulation of translation. However, downregulation or overexpression of MSY3 in the Neuro-2A cell line did not affect global translation rates. Other researchers suggested that the MSY3 protein has the redundant function with Y-box protein 1 (YB-1). Accordingly, in our system the MSY3 protein could be co-immunoprecipitated with YB-1. Importantly, developmentally regulated expression of MSY3 is not a hallmark of general translation apparatus, as several other proteins involved in translation did not show similar downregulation. To summarise, this work showed that the MSY3 protein is a marker of proliferation of progenitor cells in the embryonic and adult brain, being absent from neurons. Discovery of the molecular mechanism by which MSY3 exerts its role in the cell could provide the link between the translational machinery and proliferation.

Y-box protein

MSY3

neurogenesis

Y-box Protein

MSY3

Neurogenese

ddc:570

rvk:WG 6975

Proteine

Neurogenese

Zentralnervensystem

Maus

Novel in vivo imaging approaches to study embryonic and adult neurogenesis in the mouse

Attardo, Alessio

15 February 2007

Neurogenesis is the process of generation of neurons during embryonic development and adulthood. The focus of this doctoral work is the study of the cell biological aspects of neurogenesis and the mechanisms regulating the switch of neural stem cells from proliferation to differentiation. During embryonic development neurogenic divisions occur at the apical or basal side of the pseudostratified epithelium that forms the wall of the neural tube, the neuroepithelium. Apical asymmetric neurogenic divisions (AP) give rise to a neuron and a progenitor cell, while basal symmetric neurogenic divisions (BP) give rise to two neurons. The first part of this thesis is focused on the study of some cell biological aspects of BPs. We first validated the use of the Tis21-GFP knock in mouse line, previously generated in our laboratory. We found that the totality of neurogenic progenitors is marked by the expression of a nuclear GFP. We calculated the abundance of BPs overtime since the onset of neurogenesis showing that BPs overcome APs over development. We studied the loss of apical contact of the basal dividing cells. We found that both neurogenic and non-neurogenic basally dividing progenitors miss the apical contact; which is lost prior mitosis. We generated and characterized a second mouse line, the Tubb3-GFP line expressing a plasma membrane-localized GFP in neurons. These two lines were crossed to obtain a new line (TisTubb-GFP) allowing detection of neurogenic divisions and tracking daughter cells. Using this model: (i) we imaged symmetric neurogenic divisions of BPs, identifying daughter cells as neurons, during imaging; (ii) we compared the kinetics of betaIII-tubulin-GFP appearance after apical or basal mitosis, showing that daughters of BPs express betaIII-tubulin-GFP faster than daughters coming from apical divisions; (iii) we imaged neuronal migration and localization of the Golgi apparatus. Neurogenesis in the adult is confined to two specific regions in the telencephalon: the sub ependymal zone, lining the ventricle, and dentate gyrus of the hippocampus. The second part of this thesis focuses on the adult neurogenic progenitors lineage. Tis21-GFP expression was found and characterized in the two adult neurogenic regions from early postnatal to adulthood. Using a panel of markers for the adult neurogenic cell lineage and confocal imaging, we characterized Tis21-GFP expression, in the dentate gyrus. Tis21-GFP is first expressed in the neurogenic subpopulation of doublecortin positive cells. Tis21-GFP is inherited by the neurons and eventually degraded. Moreover, our data suggest that mitotic Tis21-GFP cells are an indicator of the levels of neurogenesis more accurate than doublecortin positive cells, in the early postnatal mouse. (Anlage Quick time movies 77,88 MB)

Neurogenesis

adult neurogenesis

imaging

two-photon microscopy

Tis21

transgenic

Neurogenese

Altersneurogenese

Mikroskopie

Tis21

Transgenese

ddc:570

rvk:WG 6975

Neurogenese

Maus

Function analysis of Xenopus NumbL in the context of primary neurogenesis / Fuktionsanalyse von Xenopus NumbL in der primären Neurogenese

Nieber, Frank

06 December 2010

Mitglieder der Numb Protein-Familie in Vertebraten haben vielfältige Funktionen während der frühen Embryogenese, einschließend einer essentiellen Rolle in der Entwicklung des Nervensystems. Numb Proteine interagieren als Gerüst-Proteine mit vielen Interaktionspartnern und können demnach mehrere Funktionen haben, wie zum Beispiel die Inhibition des Notch Signalweges. Die exakte Funktion während der Entwicklung in Vertebraten ist jedoch unklar. Im Gegensatz zu Numb wird NumbL ist ausschließlich im entstehenden Nervensystem von Xenopus exprimiert und wird durch die proneuralen Faktoren der Neurogenin Familie induziert und durch Notch inhibiert. Während die Überexpression von NumbL zu einer leichten Zunahme postmitotischer Neuronen führt, inhibiert ein Knockdown von NumbL alle molekularen Marker stromabwärts von Neurogenin und führt zu einer Zunahme von Vorläufer-Markern. Weiter werden in dieser Arbeit Beweise für die Interaktion von NumbL mit dem endocytotischen AP-2 Komplex erbracht und das diese Interaktion essentiell für die Funktion von NumbL während der primären Neurogenese ist. Interessanterweise scheint die Inhibition der Neurogenese bei einem Knockdown von NumbL nicht auf einer Deregulierung des Notch Signalweges zu beruhen.

570 Biowissenschaften, Biologie

Biology (incl. Psychology)

Numb

NumbL

Notch

Neurogenese

Xenopus

Numb

NumbL

Notch

Neurogenese

Xenopus

42.13 Molekularbiologie

WF 200 Molekularbiologie

Novel in vivo imaging approaches to study embryonic and adult neurogenesis in the mouse

Attardo, Alessio

20 December 2006

Neurogenesis is the process of generation of neurons during embryonic development and adulthood. The focus of this doctoral work is the study of the cell biological aspects of neurogenesis and the mechanisms regulating the switch of neural stem cells from proliferation to differentiation. During embryonic development neurogenic divisions occur at the apical or basal side of the pseudostratified epithelium that forms the wall of the neural tube, the neuroepithelium. Apical asymmetric neurogenic divisions (AP) give rise to a neuron and a progenitor cell, while basal symmetric neurogenic divisions (BP) give rise to two neurons. The first part of this thesis is focused on the study of some cell biological aspects of BPs. We first validated the use of the Tis21-GFP knock in mouse line, previously generated in our laboratory. We found that the totality of neurogenic progenitors is marked by the expression of a nuclear GFP. We calculated the abundance of BPs overtime since the onset of neurogenesis showing that BPs overcome APs over development. We studied the loss of apical contact of the basal dividing cells. We found that both neurogenic and non-neurogenic basally dividing progenitors miss the apical contact; which is lost prior mitosis. We generated and characterized a second mouse line, the Tubb3-GFP line expressing a plasma membrane-localized GFP in neurons. These two lines were crossed to obtain a new line (TisTubb-GFP) allowing detection of neurogenic divisions and tracking daughter cells. Using this model: (i) we imaged symmetric neurogenic divisions of BPs, identifying daughter cells as neurons, during imaging; (ii) we compared the kinetics of betaIII-tubulin-GFP appearance after apical or basal mitosis, showing that daughters of BPs express betaIII-tubulin-GFP faster than daughters coming from apical divisions; (iii) we imaged neuronal migration and localization of the Golgi apparatus. Neurogenesis in the adult is confined to two specific regions in the telencephalon: the sub ependymal zone, lining the ventricle, and dentate gyrus of the hippocampus. The second part of this thesis focuses on the adult neurogenic progenitors lineage. Tis21-GFP expression was found and characterized in the two adult neurogenic regions from early postnatal to adulthood. Using a panel of markers for the adult neurogenic cell lineage and confocal imaging, we characterized Tis21-GFP expression, in the dentate gyrus. Tis21-GFP is first expressed in the neurogenic subpopulation of doublecortin positive cells. Tis21-GFP is inherited by the neurons and eventually degraded. Moreover, our data suggest that mitotic Tis21-GFP cells are an indicator of the levels of neurogenesis more accurate than doublecortin positive cells, in the early postnatal mouse. (Anlage Quick time movies 77,88 MB)

info:eu-repo/classification/ddc/570

ddc:570

Neurogenese; Maus

CHARACTERISATION OF Y-BOX PROTEIN 3 (MSY3) IN THE DEVELOPING MURINE CENTRAL NERVOUS SYSTEM

Grzyb, Anna Natalia

05 February 2007

Neurons, astrocytes and oligodendrocytes of the central nervous system (CNS) arise from a common pool of multipotent neuroepithelial progenitor cells lining the walls of the neural tube. Initially, neuroepithelial cells undergo symmetric proliferative divisions, thereby expanding the progenitor pool and determining the size of brain compartments. At the onset of neurogenesis, a subset of progenitors switch to asymmetric or terminal symmetric neurogenic divisions. Maintenance of progenitor cell population throughout the period of neurogenesis is essential to generate the full diversity of neuronal cell types and proper histological pattern. However, the mechanisms responsible for the maintenance of progenitor cells proliferation are far from being fully understood. The family of Y-box proteins is involved in control of proliferation and transformation in various normal and pathological cellular systems, and therefore was considered as a candidate to exert such a function. Y-box proteins have a capacity to bind DNA and RNA, thereby controlling gene expression from transcription to translation. This study aimed to examine the expression of mouse Y-box protein 3 (MSY3) in the developing nervous system and elucidate its putative role in regulation of proliferation of progenitor cells. As presented in this work, the MSY3 protein in the embryonic CNS is expressed solely in progenitor cells and not neurons. Moreover, as shown by two independent approaches: morphologically, i.e. using immunofluorescence and confocal microscopy, and biochemically, MSY3 expression is downregulated concomitantly with the spatiotemporal progression of neurogenesis. Interestingly, in preliminary results it was shown that MSY3 is expressed in Dcx-positive transient amplifying precursors in germinal zones of the adult brain, and in EGF-dependent neurospheres. To evaluate whether MSY3 could regulate the neurogenesis, the levels of the MSY3 protein in the progenitors were acutely downregulated or elevated by electroporation of RNAi or MSY3 expression plasmids, respectively. Neither premature reduction of MSY3 in the neuroepithelium (E9.5-E11.5) nor prolonged expression at the developmental stage when this protein is endogenously downregulated (E10.5-14.5) did affect proliferation versus the cell cycle exit of progenitors. Moreover, in Notch1-deficient progenitors in the cerebellar anlage, which exhibit precocious differentiation, MSY3 was not prematurely downregulated, suggesting that MSY3 also is not an early marker of differentiation. Differential centrifugation, immunoprecipitation and polysomal analysis performed in this study revealed that the MSY3 protein in the developing embryo, as well as in Neuro-2A cells, is associated with RNA. On a sucrose density gradient MSY3 co-fractionates with ribosomes and actively translating polysomes, suggesting that it might have a role in regulation of translation. However, downregulation or overexpression of MSY3 in the Neuro-2A cell line did not affect global translation rates. Other researchers suggested that the MSY3 protein has the redundant function with Y-box protein 1 (YB-1). Accordingly, in our system the MSY3 protein could be co-immunoprecipitated with YB-1. Importantly, developmentally regulated expression of MSY3 is not a hallmark of general translation apparatus, as several other proteins involved in translation did not show similar downregulation. To summarise, this work showed that the MSY3 protein is a marker of proliferation of progenitor cells in the embryonic and adult brain, being absent from neurons. Discovery of the molecular mechanism by which MSY3 exerts its role in the cell could provide the link between the translational machinery and proliferation.

info:eu-repo/classification/ddc/570

ddc:570

Y-box protein, MSY3, neurogenesis

Y-box Protein, MSY3, Neurogenese

Adulte hippocampale Neurogenese bei psychischen Erkrankungen / Adult hippocampal neurogenesis in psychiatric deseases

Finger, Mathias Johannes

January 2007

Es existiert bereits eine Vielzahl von tierexperimentellen Studien bezüglich Einflussfaktoren auf die adulte Neurogenese. Nachdem die Teilungsfähigkeit von neuralen Stammzellen Ende der 1990er Jahre auch im adulten humanen Gehirn nachgewiesen wurde, war es das Ziel der vorliegenden Arbeit, adulte Neurogenese bei psychischen Erkrankungen zu quantifizieren bzw. den Ein-fluss medikamentöser Therapien auf die adulte Neurogenese zu untersuchen. Diese Studie stellt dabei die bislang einzige Arbeit dar, die sich mit der humanen adulten Neurogenese bei psychischen Erkrankungen beschäftigt. Mittels Doppelfärbungen von Ki67 und BrdU an Mausgewebe wurde zunächst nachgewiesen, dass das Ki67-Antigen ein zuverlässiger Marker für sich teilende Zellen ist, woraufhin die Färbeprozedur problemlos auf Humangewebe übertragen werden konnte. Die Quantifizierung von Ki67 positiven Zellen erfolgte entlang der Körnerzellschicht in einem definierten Abstand in der Einheit Zellen pro Millimeter. Die Ergebnisse der hier vorliegenden Studie widersprechen in mehrfacher Hinsicht den Hypothesen, die sich aus tierexperimentellen Studien ergeben. Während die neurale Stammzellproli-feration bei schizophrenen Psychosen signifikant vermindert ist, findet sich kein Unterschied bei affektiven Erkrankungen im Vergleich zu Kontrollen. Weder wird die „Neurogenese-Hypothese“ der Depression bestätigt, noch zeigte sich ein Effekt antidepressiv oder antipsychotisch wirksamer Pharmaka auf die Rate adulter Neurogenese, da eine pharmakologische Therapie jedweder Art keinen Einfluss auf die Zahl Ki67 positiver Zellen hatte. Deshalb scheint eine Steigerung der adulten Neurogenese kein Wirkmechanismus dieser Medikamente zu sein. Ein überraschendes Ergebnis jedoch ist die signifikant reduzierte Rate adulter Neurogenese bei an Schizophrenie erkrankten Patienten. Aufgrund der sehr begrenzten Anzahl untersuchter Patienten ist die vorliegende Studie in ihrer Aussagekraft jedoch eingeschränkt und muss daher an einem größeren Patientenkollektiv wiederholt werden. Eine Vielzahl von Fragen bzgl. des Stellenwerts der adulten Neurogenese bei psychischen Erkrankungen bleibt darüber hinaus weiter ungeklärt, was die Durchführung weiterer Studien am adulten humanen Gehirn verlangt. / The phenomenon of adult neurogenesis (AN), that is, the generation of functional neurons from neural stem cells in the dentate gyrus of the hippocampus, has attracted remarkable attention, especially as it was shown that this process is also active in the human brain. Based on animal studies, it has been suggested that reduced AN is implicated in the etiopathology of psychiatric disorders, and that stimulation of AN contributes to the mechanism of action of antidepressant therapies. As data from human post-mortem brain are still lacking, we investigated whether the first step of AN, that is, the level of neural stem cell proliferation (NSP; as quantified by Ki-67 immunohistochemistry), is altered in tissue from the Stanley Foundation Neuropathology Consortium comprising brain specimens from patients with bipolar affective disorder, major depression, schizophrenia as well as control subjects (n = 15 in each group). The hypothesis was that stem cell proliferation is reduced in affective disorders, and that antidepressant treatment increases NSP. Neither age, brain weight or pH, brain hemisphere investigated nor duration of storage had an effect on NSP. Only in bipolar disorder, postmortem interval was a significant intervening variable. In disease, onset of the disorder and its duration likewise did not affect NSP. Also, cumulative lifetime dose of fluphenazine was not correlated with NSP, and presence of antidepressant treatment did not result in an increase of NSP. Concerning the different diagnostic entities, reduced amounts of newly formed cells were found in schizophrenia, but not in major depression. Our findings suggest that reduced NSP may contribute to the pathogenesis of schizophrenia, whereas the rate of NSP does not seem to be critical to the etiopathology of affective disorders, nor is it modified by antidepressant drug treatment.

Neurogenese

Depression

Schizophrenie

Hippocampus

Manie

Ki-67

ddc:610

Etude anatomique et fonctionnelle du cerveau des souris KO STOP : modèle animal pour l'étude de la schizophrénie

Jany, Marion

22 October 2010

Mon travail de thèse participe à la caractérisation des bases cellulaires et moléculaires neurodéveloppementales à l'origine de la schizophrénie. A partir d'un modèle animal pour l'étude de la schizophrénie (souris KO STOP), j'ai tenté de déterminer les relations entre la diminution du volume cérébral, la biologie cellulaire des neurones in situ, et les événements cellulaires et moléculaires à l'origine de cette diminution de volume. Ainsi, j'ai démontré, par western blot quantitatif, que la réduction de volume cérébral chez les souris KO STOP était associée à une forte diminution des compartiments myéliniques, axonaux et synaptiques. Une analyse morphométrique a montré ensuite que la surface de plusieurs tracts myélinisés était fortement réduite chez la souris KO STOP. Le résultat majeur de ce travail, confirmé par l'utilisation de traceur lipidique, a été la mise en évidence de l'absence de la partie post-commissurale du fornix, tract reliant l'hippocampe au corps mamillaire et fortement altéré chez les schizophrènes. Le traçage lentiviral de ces axones a montré la désorganisation des fibres du fornix chez les souris KO STOP. J'ai ensuite analysé la neurogenèse adulte hippocampale et démontré que ce processus était spécifiquement et progressivement altéré chez les souris KO STOP. L'architecture dendritique des neurones immatures des souris KO STOP semble anormale, avec un dendrite primaire plus long et un arbre dendritique plus branché. Le traçage rétroviral-GFP des cellules souches neurales de l'hippocampe, a permis de montrer, à 4 semaines post-infection, une réduction du nombre de neurones immatures chez les souris KO STOP suggérant une maturation prématurée des neurones néoformés. Ce travail ouvre des perspectives de recherche sur le développement embryonnaire du fornix et des connectivités neuronales en général. Nous envisageons aussi d'analyser la maturation axonale et synaptique des neurones hippocampaux néoformés, étapes du développement neuronal importantes pour la mise en place des connectivités neuronales.

Schizophrenie

Fornix

Connectivité neuronale

Maturation neuronale

Neurogenese adulte hippocampale