47 research outputs found

    Imaging and Recording Subventricular Zone Progenitor Cells in Live Tissue of Postnatal Mice

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    The subventricular zone (SVZ) is one of two regions where neurogenesis persists in the postnatal brain. The SVZ, located along the lateral ventricle, is the largest neurogenic zone in the brain that contains multiple cell populations including astrocyte-like cells and neuroblasts. Neuroblasts migrate in chains to the olfactory bulb where they differentiate into interneurons. Here, we discuss the experimental approaches to record the electrophysiology of these cells and image their migration and calcium activity in acute slices. Although these techniques were in place for studying glial cells and neurons in mature networks, the SVZ raises new challenges due to the unique properties of SVZ cells, the cellular diversity, and the architecture of the region. We emphasize different methods, such as the use of transgenic mice and in vivo electroporation that permit identification of the different SVZ cell populations for patch clamp recording or imaging. Electroporation also permits genetic labeling of cells using fluorescent reporter mice and modification of the system using either RNA interference technology or floxed mice. In this review, we aim to provide conceptual and technical details of the approaches to perform electrophysiological and imaging studies of SVZ cells

    Intrinsic Neuronal Activity during Migration Controls the Recruitment of Specific Interneuron Subtypes in the Postnatal Mouse Olfactory Bulb

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    Neuronal activity has been identified as a key regulator of neuronal network development, but the impact of activity on migration and terminal positioning of interneuron subtypes is poorly understood. The absence of early subpopulation markers and the presence of intermingled migratory and postmigratory neurons make the developing cerebral cortex a difficult model to answer these questions. Postnatal neurogenesis in the subventricular zone (SVZ) offers a more accessible and compartmentalized model. Neural stem cells regionalized along the border of the lateral ventricle produce two main subtypes of neural progenitors, granule cells and periglomerular neurons that migrate tangentially in the rostral migratory stream (RMS) before migrating radially in the olfactory bulb (OB) layers. Here, we used targeted postnatal electroporation to compare the migration of these two populations in male and female mice. We do not observe any obvious differences regarding the mode of tangential or radial migration between these two subtypes. However, we find a striking increase of intrinsic calcium activity in granule cell precursors (GC-Ps) when they switch from tangential to radial migration. By decreasing neuronal excitability in GC-Ps, we find that neuronal activity has little effect on migration but is required for normal positioning and survival of GC-Ps in the OB layers. Strikingly, decreasing activity of periglomerular neuron precursors (PGN-Ps) did not impact their positioning or survival. Altogether these findings suggest that neuronal excitability plays a subtype specific role during the late stage of migration of postnatally born OB interneurons

    GABAA Increases Calcium in Subventricular Zone Astrocyte-Like Cells Through L- and T-Type Voltage-Gated Calcium Channels

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    In the adult neurogenic subventricular zone (SVZ), the behavior of astrocyte-like cells and some of their functions depend on changes in intracellular Ca2+ levels and tonic GABAA receptor activation. However, it is unknown whether, and if so how, GABAA receptor activity regulates intracellular Ca2+ dynamics in SVZ astrocytes. To monitor Ca2+ activity selectively in astrocyte-like cells, we used two lines of transgenic mice expressing either GFP fused to a Gq-coupled receptor or DsRed under the human glial fibrillary acidic protein (hGFAP) promoter. GABAA receptor activation induced Ca2+ increases in 40–50% of SVZ astrocytes. GABAA-induced Ca2+ increases were prevented with nifedipine and mibefradil, blockers of L- and T-type voltage-gated calcium channels (VGCC). The L-type Ca2+ channel activator BayK 8644 increased the percentage of GABAA-responding astrocyte-like cells to 75%, suggesting that the majority of SVZ astrocytes express functional VGCCs. SVZ astrocytes also displayed spontaneous Ca2+ activity, the frequency of which was regulated by tonic GABAA receptor activation. These data support a role for ambient GABA in tonically regulating intracellular Ca2+ dynamics through GABAA receptors and VGCC in a subpopulation of astrocyte-like cells in the postnatal SVZ

    : Maurocalcine transduction into cells

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    International audienceMaurocalcine (MCa) is a 33-amino-acid residue peptide toxin isolated from the scorpion Scorpio maurus palmatus. External application of MCa to cultured myotubes is known to produce Ca2+ release from intracellular stores. MCa binds directly to the skeletal muscle isoform of the ryanodine receptor, an intracellular channel target of the endoplasmic reticulum, and induces long lasting channel openings in a mode of smaller conductance. Here we investigated the way MCa proceeds to cross biological membranes to reach its target. A biotinylated derivative of MCa was produced (MCa(b)) and complexed with a fluorescent indicator (streptavidine-cyanine 3) to follow the cell penetration of the toxin. The toxin complex efficiently penetrated into various cell types without requiring metabolic energy (low temperature) or implicating an endocytosis mechanism. MCa appeared to share the same features as the so-called cell-penetrating peptides. Our results provide evidence that MCa has the ability to act as a molecular carrier and to cross cell membranes in a rapid manner (1-2 min), making this toxin the first demonstrated example of a scorpion toxin that translocates into cells

    Specific In Vivo Staining of Astrocytes in the Whole Brain after Intravenous Injection of Sulforhodamine Dyes

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    Fluorescent staining of astrocytes without damaging or interfering with normal brain functions is essential for intravital microscopy studies. Current methods involved either transgenic mice or local intracerebral injection of sulforhodamine 101. Transgenic rat models rarely exist, and in mice, a backcross with GFAP transgenic mice may be difficult. Local injections of fluorescent dyes are invasive. Here, we propose a non-invasive, specific and ubiquitous method to stain astrocytes in vivo. This method is based on iv injection of sulforhodamine dyes and is applicable on rats and mice from postnatal age to adulthood. The astrocytes staining obtained after iv injection was maintained for nearly half a day and showed no adverse reaction on astrocytic calcium signals or electroencephalographic recordings in vivo. The high contrast of the staining facilitates the image processing and allows to quantify 3D morphological parameters of the astrocytes and to characterize their network. Our method may become a reference for in vivo staining of the whole astrocytes population in animal models of neurological disorders

    Activité calcique et communication paracrine avant synaptogenèse dans le développement du néocortex murin

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    In mouse neocortex, precursor cell divisions occur as soon as E11 and give rise to the first pioneers neurons, including Cajal-Retzius cells. Spontaneous electrical activity, supported by ion channels, is a key factor in central nervous system development. In the present work, the main goal was to understand how ion channels and calcium signalling are implicated in early neurogenesis. First, we found an inward sodium current in 55% of neuronal cells, including all Cajal-Retzius cells. At the same stage, we observed spontaneous calcium activity in proliferative and neuronal cells of cortical slices. We developed an imaging software statistically analyze calcium activity and to identify ions channels imvolved. While synapses were not yet formed, we observed the presence of synchronous calcium activity and early paracrine communication between cells. We demonstrated the existence of a signalling cascade: glycine receptors depolarization activate sodium channels expressed in neuronal cells, which in turn lead to cytoplasmic calcium increases via Na+/Ca2+ exchangers. The subsequent glutamate exocytosis paracrine release activate neocortical cells lacking sodium channels. The use of organotypic brain slice culture showed a major physiological implication of this original pathway in corticogenesis.Dans le néocortex murin, la division des cellules précurseurs a lieu dès le stade E11 et donne naissance aux premiers neurones pionniers dont les cellules de Cajal-Retzius. L'activité électrique spontanée, portée par les canaux ioniques, joue un rôle prépondérant dans le développement du système nerveux central. Comprendre la place des canaux ioniques et de la signalisation calcique dans les phases précoces de le neurogenèse était l'objectif principal de mon projet. Nous avons montré l'apparition précoce de canaux sodiques dépendants du voltage dans 55% des cellules neuronales à E13, dont les cellules de Cajal-Retzius. En parallèle, nous avons observé des activités calciques spontanées dans les cellules proliférantes et neuronales au même stade. La conception d'un logiciel d'imagerie nous a permis d'analyser statistiquement ces activités et d'identifier les canaux ioniques impliqués. Alors que les synapses ne sont pas encore formées, nous avons observé la mise en place d'activités synchrones au sein du néocortex et démontré l'existence de communications paracrines entre les cellules. De plus, nous avons identifié l'existence d'une cascade de signalisation où la dépolarisation des récepteurs glycinergiques active les canaux sodiques présents sur les neurones pionniers. Dans ces neurones, l'influx sodique entraîne une augmentation de calcium cytoplasmique via un échangeur Na+/Ca2+ puis une exocytose glutamatergique dont le libération paracrine induit l'activation d'autres cellules néocorticales. L'utilisation de la culture organotypique de cerveau nous a laissé entrevoir une implication physiologique majeure de cette cascade de signalisation dans la corticogenèse

    Activité calcique et communication paracrine avant synaptogenèse dans le développement du néocortex murin

    No full text
    Dans le néocortex murin, la division des cellules précurseurs a lieu dès le stade E11 et donne naissance aux premiers neurones pionniers dont les cellules de Cajal-Retzius. L'activité électrique spontanée, portée par les canaux ioniques, joue un rôle prépondérant dans le développement du système nerveux central. Comprendre la place des canaux ioniques et de la signalisation calcique dans les phases précoces de le neurogenèse était l'objectif principal de mon projet. Nous avons montré l'apparition précoce de canaux sodiques dépendants du voltage dans 55% des cellules neuronales à E13, dont les cellules de Cajal-Retzius. En parallèle, nous avons observé des activités calciques spontanées dans les cellules proliférantes et neuronales au même stade. La conception d'un logiciel d'imagerie nous a permis d'analyser statistiquement ces activités et d'identifier les canaux ioniques impliqués. Alors que les synapses ne sont pas encore formées, nous avons observé la mise en place d'activités synchrones au sein du néocortex et démontré l'existence de communications paracrines entre les cellules. De plus, nous avons identifié l'existence d'une cascade de signalisation où la dépolarisation des récepteurs glycinergiques active les canaux sodiques présents sur les neurones pionniers. Dans ces neurones, l'influx sodique entraîne une augmentation de calcium cytoplasmique via un échangeur Na+/Ca2+ puis une exocytose glutamatergique dont le libération paracrine induit l'activation d'autres cellules néocorticales. L'utilisation de la culture organotypique de cerveau nous a laissé entrevoir une implication physiologique majeure de cette cascade de signalisation dans la corticogenèse.GRENOBLE1-BU Sciences (384212103) / SudocSudocFranceF

    Characterization of perinatally born glutamatergic neurons of the mouse olfactory bulb based on NeuroD6 expression reveals their resistance to sensory deprivation

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    International audienceDuring postnatal olfactory bulb (OB) neurogenesis, predetermined stem cells residing in the ventricular-subventricular zone continuously generate progenitors that migrate in the rostral migratory stream and integrate into the OB. Although the vast majority of these postnatally generated interneurons are inhibitory, a sub-fraction represents glutamatergic neurons that integrate into the superficial glomerular layer. In the present work, we demonstrate that the bHLH transcription factor NeuroD6 is specifically and transitorily expressed in the dorsal neurogenic lineage that generates glutamatergic juxtaglomerular cells (JGCs) for the OB. Using lineage tracing combined with whole brain clearing, we provide new insight into timing of generation, morphology , and connectivity of glutamatergic JGCs. Specifically, we show that all glutamatergic JGCs send complex axons with varying projection patterns into different layers of the OB. Moreover, we find that, contrary to GABAergic OB interneurons, glutamatergic JGCs survive under sensory deprivation, indicating that inhibitory and excitatory populations are differentially susceptible to environmental stimulation
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