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首页> 外文期刊>The Journal of Neuroscience: The Official Journal of the Society for Neuroscience >Genetic analysis of soluble N-ethylmaleimide-sensitive factor attachment protein function in Drosophila reveals positive and negative secretory roles.
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Genetic analysis of soluble N-ethylmaleimide-sensitive factor attachment protein function in Drosophila reveals positive and negative secretory roles.

机译:果蝇中可溶性N-乙基马来酰亚胺敏感因子附着蛋白功能的遗传分析揭示了正负分泌作用。

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The N-ethylmaleimide-sensitive factor (NSF) and soluble NSF attachment protein (SNAP) are cytosolic factors that promote vesicle fusion with a target membrane in both the constitutive and regulated secretory pathways. NSF and SNAP are thought to function by catalyzing the disassembly of a SNAP receptor (SNARE) complex consisting of membrane proteins of the secretory vesicle and target membrane. Although studies of NSF function have provided strong support for this model, the precise biochemical role of SNAP remains controversial. To further explore the function of SNAP, we have used mutational and transgenic approaches in Drosophila to investigate the effect of altered SNAP dosage on neurotransmitter release and SNARE complex metabolism. Our results indicate that reduced SNAP activity results in diminished neurotransmitter release and accumulation of a neural SNARE complex. Increased SNAP dosage results in defective synapse formation and a variety of tissue morphological defects without detectably altering the abundance of neural SNARE complexes. The SNAP overexpression phenotypes are enhanced by mutations in other secretory components and are at least partially overcome by co-overexpression of NSF, suggesting that these phenotypes derive from a specific perturbation of the secretory pathway. Our results indicate that SNAP promotes neurotransmitter release and SNARE complex disassembly but inhibits secretion when present at high abundance relative to NSF.
机译:N-乙基马来酰亚胺敏感因子(NSF)和可溶性NSF附着蛋白(SNAP)是在组成型和调节型分泌途径中均能促进囊泡与靶膜融合的胞质因子。 NSF和SNAP被认为通过催化由分泌囊泡和靶膜的膜蛋白组成的SNAP受体(SNARE)复合物的分解而发挥功能。尽管对NSF功能的研究为该模型提供了有力的支持,但SNAP的确切生化作用仍存在争议。为了进一步探索SNAP的功能,我们在果蝇中使用了突变和转基因方法来研究改变SNAP剂量对神经递质释放和SNARE复合物代谢的影响。我们的结果表明,SNAP活性降低导致神经递质释放和神经SNARE复合物积累减少。 SNAP剂量增加会导致缺陷的突触形成和多种组织形态学缺陷,而不会检测到神经SNARE复合物的丰度。 SNAP过表达表型通过其他分泌成分的突变而增强,并且至少部分通过NSF的共过表达而克服,表明这些表型源自分泌途径的特定扰动。我们的结果表明,SNAP促进神经递质的释放和SNARE复合物的分解,但是当相对于NSF含量很高时,会抑制分泌。

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