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首页> 外文期刊>Molecular biology of the cell >Identification of the Neuroblastoma-amplified Gene Product as a Component of the Syntaxin 18 Complex Implicated in Golgi-to-Endoplasmic Reticulum Retrograde Transport
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Identification of the Neuroblastoma-amplified Gene Product as a Component of the Syntaxin 18 Complex Implicated in Golgi-to-Endoplasmic Reticulum Retrograde Transport

机译:神经母细胞瘤扩增的基因产物作为Syntaxin 18复杂的高尔基体-内质网逆行运输牵连的组成部分的鉴定。

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摘要

Syntaxin 18, a soluble N -ethylmaleimide-sensitive factor (NSF) attachment protein receptor (SNARE) protein implicated in endoplasmic reticulum (ER) membrane fusion, forms a complex with other SNAREs (BNIP1, p31, and Sec22b) and several peripheral membrane components (Sly1, ZW10, and RINT-1). In the present study, we showed that a peripheral membrane protein encoded by the neuroblastoma-amplified gene ( NAG ) is a subunit of the syntaxin 18 complex. NAG encodes a protein of 2371 amino acids, which exhibits weak similarity to yeast Dsl3p/Sec39p, an 82-kDa component of the complex containing the yeast syntaxin 18 orthologue Ufe1p. Under conditions favoring SNARE complex disassembly, NAG was released from syntaxin 18 but remained in a p31-ZW10-RINT-1 subcomplex. Binding studies showed that the extreme N-terminal region of p31 is responsible for the interaction with NAG and that the N- and the C-terminal regions of NAG interact with p31 and ZW10-RINT-1, respectively. Knockdown of NAG resulted in a reduction in the expression of p31, confirming their intimate relationship. NAG depletion did not substantially affect Golgi morphology and protein export from the ER, but it caused redistribution of Golgi recycling proteins accompanied by a defect in protein glycosylation. These results together suggest that NAG links between p31 and ZW10-RINT-1 and is involved in Golgi-to-ER transport.
机译:Syntaxin 18是一种与内质网(ER)膜融合有关的可溶性N-乙基马来酰亚胺敏感因子(NSF)附着蛋白受体(SNARE)蛋白,与其他SNARE(BNIP1,p31和Sec22b)和一些外周膜成分形成复合体(Sly1,ZW10和RINT-1)。在本研究中,我们显示了由神经母细胞瘤扩增基因(NAG)编码的外周膜蛋白是语法18复合体的亚基。 NAG编码2371个氨基酸的蛋白质,与酵母Dsl3p / Sec39p(包含酵母语法18直向同源物Ufe1p的复合物的82-kDa成分)的相似性较弱。在支持SNARE复杂分解的条件下,NAG从语法18中释放出来,但仍保留在p31-ZW10-RINT-1子复合物中。结合研究表明,p31的极端N末端区域负责与NAG的相互作用,而NAG的N末端和C末端区域分别与p31和ZW10-RINT-1相互作用。剔除NAG导致p31表达减少,证实了它们的亲密关系。 NAG的消耗并没有实质性地影响高尔基体的形态和蛋白从ER的输出,但它导致了高尔基体回收蛋白的重新分布,并伴有蛋白糖基化缺陷。这些结果共同表明,p31和ZW10-RINT-1之间的NAG链接与高尔基体到ER的运输有关。

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