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Synaptophysin I controls the targeting of VAMP2/synaptobrevin II to synaptic vesicles

机译:突触素I控制VAMP2 /突触素II对突触小泡的靶向

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Synaptic vesicle (SV) proteins are synthesized at the level of the cell body and transported down the axon in membrane precursors of SVs. To investigate the mechanisms underlying sorting of proteins to SVs, fluorescent chimeras of vesicle-associated membrane protein (VAMP) 2, its highly homologous isoform VAMP1 and synaptotagmin I (SytI) were expressed in hippocampal neurons in culture. Interestingly, the proteins displayed a diffuse component of distribution along the axon. In addition, VAMP2 was found to travel in vesicles that constitutively fuse with the plasma membrane. Coexpression of VAMP2 with synaptophysin I (SypI), a major resident of SVs, restored the correct sorting of VAMP2 to SVs. The effect of SypI on VAMP2 sorting was dose dependent, being reversed by increasing VAMP2 expression levels, and highly specific, because the sorting of the SV proteins VAMP1 and SytI was not affected by SypI. The cytoplasmic domain of VAMP2 was found to be necessary for both the formation of VAMP2-SypI hetero-dimers and for VAMP2 sorting to SVs. These data support a role for SypI in directing the correct sorting of VAMP2 in neurons and demonstrate that a direct interaction between the two proteins is required for SypI in order to exert its effect. [References: 42]
机译:突触小泡(SV)蛋白在细胞体水平上合成,并沿SVs膜前体的轴突向下运输。为了研究将蛋白质分类为SV的基本机制,在培养的海马神经元中表达了囊泡相关膜蛋白(VAMP)2的荧光嵌合体,其高度同源的同种型VAMP1和突触小分子蛋白I(SytI)。有趣的是,蛋白质沿轴突显示出弥散性分布。另外,发现VAMP2在与质膜组成性融合的囊泡中传播。 VAMP2与突触素I(SypI)(SV的主要成员)的共表达恢复了VAMP2对SV的正确分类。由于SV蛋白VAMP1和SytI的分选不受SypI的影响,SypI对VAMP2的分选具有剂量依赖性,可以通过增加VAMP2表达水平来逆转,并且具有高度特异性。发现VAMP2的胞质结构域对于形成VAMP2-SypI异二聚体和将VAMP2分选至SV都是必需的。这些数据支持SypI在指导神经元中VAMP2正确排序方面的作用,并证明SypI需要两种蛋白质之间的直接相互作用才能发挥其作用。 [参考:42]

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