Zeb2 as a regulator of adhesion interplay in the developing mouse neocortex

Der menschliche Neokortex wird als Hauptsitz kognitiver Funktionen höherer Ordnung angesehen. Das Verständnis der neokortikalen Entwicklung anderer Säugetierarten ist von wesentlicher Bedeutung, um die menschliche Gehirnorganisation im Allgemeinen und neurologische Entwicklungsstörungen im Speziellen besser zu verstehen. In dieser Arbeit habe ich die Rolle des mit dem Mowat-Wilson-Syndrom assoziierten Transkriptionsfaktors Zeb2 in der neokortikalen Entwicklung der Maus untersucht. Ich habe nachgewiesen, dass Zeb2 die Adhäsion neugeborener kortikaler Neurone sowohl vor als auch nach der radialen Migration über zwei unabhängige molekulare Wege reguliert. Hierbei konnte ich zeigen, dass die Adhäsion im Vorfeld der radialen Migration über den molekularen Zeb2-Nrp1-Itgβ1- Weg reguliert wird. Zeb2 unterdrückt zell-intrinsisch die neuronale Adhäsion an die extrazelluläre Matrix und kontrolliert dadurch den Beginn der radialen Migration, die Dauer des multipolaren Stadiums sowie die Motilität multipolarer Neurone, ohne die radiale Migration selbst oder das spätere Zellschicksal innerhalb der kortikalen Schichten zu beeinflussen. Hierbei sind die apikalen Dendriten der Neurone normalerweise parallel zueinander und senkrecht zur Hirnhautoberfläche ausgerichtet. Ich habe gezeigt, dass die Ausrichtung der Neurone im Anschluss an ihre Migration von der Adhäsion der Zellen untereinander sowie zur extrazellulären Matrix abhängt und dieser Prozess unabhängig von der radialen Migration erfolgt. Zeb2 koordiniert das gesamt e Repertoire dieser postmigratorischen Adhäsion über den molekularen Zeb2-Cdh6-Itgβ1-Weg. Zusammenfassend zeigt diese Studie die Bedeutung der neuronalen Adhäsion während der neokortikalen Entwicklung auf und entschlüsselt die Regulationsmechanismen für die Initiierung der radialen Migration sowie für die postmigratorische Orientierung der Neurone der oberen kortikalen Schichten.The human brain is a highly sophisticated biological structure and its formation is a highly orchestrated process. The human neocortex, in particular, is the main place of higher-order cognitive functions. Understanding the neocortical development of other mammalian species is essential for understanding brain organisation in common neurodevelopmental disorders in particular. Here I studied the role of Mowat-Wilson syndrome-associated transcription factor Zeb2 in mouse neocortical development. I have shown in this study that Zeb2 regulates adhesion of new born cortical neurons both before and after radial locomotion via two independent molecular pathways. I have shown that adhesion prior to radial locomotion is tightly regulated via Zeb2-Nrp1-Itgβ1 molecular pathway. Zeb2 cell-intrinsically suppresses adhesion of neurons to the extracellular matrix and therefore restricts the initiation of radial locomotion, multipolar stage duration and motility of multipolar neurons without affecting radial locomotion itself and layer cell fate acquisition. Once radial migration is finished neurons have to form apical dendrite and establish contact with the meningeal surface. Normally, apical dendrites of neurons are oriented parallel to each other and perpendicular to the meningeal surface. I have shown that postmigratory orientation of neurons is dependent on cell-to-cell and cell-to-extracellular matrix adhesion and occurs independently from radial migration. Zeb2 orchestrates the whole repertoire of adhesion of neurons completed radial migration via Zeb2-Cdh6-Itgβ1 molecular pathway. I have demonstrated that Cadherin 6 balance is crucial for establishment of postmigratory neuronal orientation under normal conditions. Taken together, this study has revealed the importance of neuronal adhesion during neocortical development and separated the regulation mechanisms for initiation of radial migration and postmigratory orientation of upper layer neurons

Viral vectors for delivering gene material into cells and their application in neurobiology (Review)

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Optogenetic approaches in neurobiology

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Application of the AAV-Syn-BDNF-EGFP virus vector as a neuroprotective agent in modeling hypoxia in vitro

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Phenotypic variations in the behavior of sip1 knockout mice

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Identification of novel mutations controlling cerebral cortex malformations caused by ENU-induced mutagenesis in the mouse

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Srsf1 and Elavl1 act antagonistically on neuronal fate choice in the developing neocortex by controlling TrkC receptor isoform expression

The seat of higher-order cognitive abilities in mammals, the neocortex, is a complex structure, organized in several layers. The different subtypes of principal neurons are distributed in precise ratios and at specific positions in these layers and are generated by the same neural progenitor cells (NPCs), steered by a spatially and temporally specified combination of molecular cues that are incompletely understood. Recently, we discovered that an alternatively spliced isoform of the TrkC receptor lacking the kinase domain, TrkC-T1, is a determinant of the corticofugal projection neuron (CFuPN) fate. Here, we show that the finely tuned balance between TrkC-T1 and the better known, kinase domain-containing isoform, TrkC-TK+, is cell type-specific in the developing cortex and established through the antagonistic actions of two RNA-binding proteins, Srsf1 and Elavl1. Moreover, our data show that Srsf1 promotes the CFuPN fate and Elavl1 promotes the callosal projection neuron (CPN) fate in vivo via regulating the distinct ratios of TrkC-T1 to TrkC-TK+. Taken together, we connect spatio-temporal expression of Srsf1 and Elavl1 in the developing neocortex with the regulation of TrkC alternative splicing and transcript stability and neuronal fate choice, thus adding to the mechanistic and functional understanding of alternative splicing in vivo

Interleukin-10 restores glutamate receptor-mediated Ca(2+)-signaling in brain circuits under loss of Sip1 transcription factor.

peer reviewedOBJECTIVE: This study aimed to investigate the connection between the mutation of the Sip1 transcription factor and impaired Ca(2+)-signaling, which reflects changes in neurotransmission in the cerebral cortex in vitro. METHODS: We used mixed neuroglial cortical cell cultures derived from Sip1 mutant mice. The cells were loaded with a fluorescent ratiometric calcium-sensitive probe Fura-2 AM and epileptiform activity was modeled by excluding magnesium ions from the external media or adding a GABA(A) receptor antagonist, bicuculline. Intracellular calcium dynamics were recorded using fluorescence microscopy. To identify the level of gene expression, the Real-Time PCR method was used. RESULTS: It was found that cortical neurons isolated from homozygous (Sip1(fl/fl)) mice with the Sip1 mutation demonstrate suppressed Ca(2+) signals in models of epileptiform activity in vitro. Wild-type cortical neurons are characterized by synchronous high-frequency and high-amplitude Ca(2+) oscillations occurring in all neurons of the network in response to Mg(2+)-free medium and bicuculline. But cortical Sip1(fl/fl) neurons only single Ca(2+) pulses or attenuated Ca(2+) oscillations are recorded and only in single neurons, while most of the cell network does not respond to these stimuli. This signal deficiency of Sip1(fl/fl) neurons correlates with a suppressed expression level of the genes encoding the subunits of NMDA, AMPA, and KA receptors; protein kinases PKA, JNK, CaMKII; and also the transcription factor Hif1α. These negative effects were partially abolished when Sip1(fl/fl) neurons are grown in media with anti-inflammatory cytokine IL-10. IL-10 increases the expression of the above-mentioned genes but not to the level of expression in wild-type. At the same time, the amplitudes of Ca(2+) signals increase in response to the selective agonists of NMDA, AMPA and KA receptors, and the proportion of neurons responding with Ca(2+) oscillations to a Mg(2+)-free medium and bicuculline increases. CONCLUSION: IL-10 restores neurotransmission in neuronal networks with the Sip1 mutation by regulating the expression of genes encoding signaling proteins

Sip-1 mutations cause disturbances in the activity of NMDA- and AMPA-, but not kainate receptors of neurons in the cerebral cortex

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Mutation in the Sip1 transcription factor leads to a disturbance of the preconditioning of AMPA receptors by episodes of hypoxia in neurons of the cerebral cortex due to changes in their activity and subunit composition. The protective effects of interleukin-10.

peer reviewedThe Sip1 mutation plays the main role in pathogenesis of the Mowat-Wilson syndrome, which is characterized by the pronounced epileptic symptoms. Cortical neurons of homozygous mice with Sip1 mutation are resistant to AMPA receptor activators. Disturbances of the excitatory signaling components are also observed on such a phenomenon of neuroplasticity as hypoxic preconditioning. In this work, the mechanisms of loss of the AMPA receptor's ability to precondition by episodes of short-term hypoxia were investigated on cortical neurons derived from the Sip1 homozygous mice. The preconditioning effect was estimated by the level of suppression of the AMPA receptors activity with hypoxia episodes. Using fluorescence microscopy, we have shown that cortical neurons from the Sip1(fl/fl) mice are characterized by the absence of hypoxic preconditioning effect, whereas the amplitude of Ca(2+)-responses to the application of the AMPA receptor agonist, 5-Fluorowillardiine, in neurons from the Sip1 mice brainstem is suppressed by brief episodes of hypoxia. The mechanism responsible for this process is hypoxia-induced desensitization of the AMPA receptors, which is absent in the cortex neurons possessing the Sip1 mutation. However, the appearance of preconditioning in these neurons can be induced by phosphoinositide-3-kinase activation with a selective activator or an anti-inflammatory cytokine interleukin-10