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Rab33a 介导囊泡顺行转运,促进膜胞吐和轴突生长。

Rab33a mediates anterograde vesicular transport for membrane exocytosis and axon outgrowth.

机构信息

Laboratorie of Neuronal Cell Morphogenesis, Nara Institute of Science and Technology, Ikoma, Nara 630-0192, Japan.

出版信息

J Neurosci. 2012 Sep 12;32(37):12712-25. doi: 10.1523/JNEUROSCI.0989-12.2012.

Abstract

Axon outgrowth requires plasma membrane expansion, which results from post-Golgi vesicular transport and fusion. However, the molecular mechanisms regulating post-Golgi vesicular trafficking for membrane expansion and axon outgrowth remain unclear. Here, we show that Rab33a expression became upregulated during axon outgrowth of cultured rat hippocampal neurons. Rab33a was preferentially localized to the Golgi apparatus and to synaptophysin-positive vesicles that are transported along the growing axon. Previous studies showed that synaptophysin is localized to post-Golgi vesicles transported by fast axonal transport in developing neurons. Reduction of Rab33a expression by RNAi (RNA interference) inhibited the anterograde transport of synaptophysin-positive vesicles, leading to their decrease in axonal tips. Furthermore, this treatment reduced membrane fusion of synaptophysin-positive vesicles at the growth cones and inhibited axon outgrowth. Overexpression of Rab33a, on the other hand, induced excessive accumulation of synaptophysin-positive vesicles and concurrent formation of surplus axons. These data suggest that Rab33a participates in axon outgrowth by mediating anterograde axonal transport of synaptophysin-positive vesicles and their concomitant fusion at the growth cones.

摘要

轴突生长需要质膜的扩展,这是通过高尔基体后期囊泡运输和融合实现的。然而,调节质膜扩展和轴突生长的高尔基体后期囊泡运输的分子机制仍不清楚。在这里,我们发现 Rab33a 在培养的大鼠海马神经元的轴突生长过程中表达上调。Rab33a 优先定位于高尔基体和突触小体阳性囊泡,这些囊泡沿着生长的轴突运输。先前的研究表明,突触小体是定位于发育神经元中快速轴突运输的高尔基体后期囊泡。通过 RNAi(RNA 干扰)降低 Rab33a 的表达抑制了突触小体阳性囊泡的顺行运输,导致它们在轴突末端减少。此外,这种处理减少了生长锥处突触小体阳性囊泡的膜融合,并抑制了轴突生长。另一方面,Rab33a 的过表达诱导了突触小体阳性囊泡的过度积累,并伴随着多余轴突的形成。这些数据表明,Rab33a 通过介导突触小体阳性囊泡的顺行轴突运输及其在生长锥处的伴随融合,参与轴突生长。

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