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  • Generation of subtype-specific neurons from postnatal astroglia of the mouse cerebral cortex.

Generation of subtype-specific neurons from postnatal astroglia of the mouse cerebral cortex.

Nature protocols (2011-02-05)
Christophe Heinrich, Sergio Gascón, Giacomo Masserdotti, Alexandra Lepier, Rodrigo Sanchez, Tatiana Simon-Ebert, Timm Schroeder, Magdalena Götz, Benedikt Berninger
摘要

Instructing glial cells to generate neurons may prove to be a strategy to replace neurons that have degenerated. Here, we describe a robust protocol for the efficient in vitro conversion of postnatal astroglia from the mouse cerebral cortex into functional, synapse-forming neurons. This protocol involves two steps: (i) expansion of astroglial cells (7 d) and (ii) astroglia-to-neuron conversion induced by persistent and strong retroviral expression of Neurog2 (encoding neurogenin-2) or Mash1 (also referred to as achaete-scute complex homolog 1 or Ascl1) and/or distal-less homeobox 2 (Dlx2) for generation of glutamatergic or GABAergic neurons, respectively (7-21 d for different degrees of maturity). Our protocol of astroglia-to-neuron conversion by a single neurogenic transcription factor provides a stringent experimental system to study the specification of a selective neuronal subtype, thus offering an alternative to the use of embryonic or neural stem cells. Moreover, it can be a useful model for studies of lineage conversion from non-neuronal cells, with potential for brain regenerative medicine.

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Sigma-Aldrich
HEPES, ≥99.5% (titration)
Sigma-Aldrich
透明质酸酶 来源于牛睾丸, Type IV-S, lyophilized powder (essentially salt-free), 750-3000 units/mg solid
Sigma-Aldrich
胰蛋白酶 来源于牛胰腺, powder, ≥7,500 BAEE units/mg solid
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单克隆抗 β-微管蛋白 III 小鼠抗, clone SDL.3D10, ascites fluid
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单克隆抗-MAP2 小鼠抗, ascites fluid, clone HM-2
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Brain Derived Neurotrophic Factor, Human, Recombinant, E. coli