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海胆卵和胚胎中sec1/munc18成员的选择性表达。

Selective expression of a sec1/munc18 member in sea urchin eggs and embryos.

作者信息

Leguia Mariana, Wessel Gary M

机构信息

Department of Molecular Biology, Cell Biology and Biochemistry, Brown University, 69 Brown Street, Providence, RI 02912, USA.

出版信息

Gene Expr Patterns. 2004 Oct;4(6):645-57. doi: 10.1016/j.modgep.2004.04.009.

Abstract

Regulated secretion is mediated by SNAREs (soluble NSF attachment receptors) and their regulators and effectors, which include the SM (sec1/munc18) family of proteins. Homologs of the SNAREs have been identified in sea urchins, associated with cortical granule exocytosis at fertilization, with membranes of the cleavage furrow, and in secretory cells later in development. To contribute to the understanding of regulated secretion in sea urchins we have cloned the single SM protein homolog from two species of sea urchin, Lytechinus variegatus and Strongylocentrotus purpuratus. In oocytes and eggs, we find that it localizes to the plasma membrane and the cortical region of the egg, consistent with a role in one of the steps leading to cortical granule exocytosis. The protein is also expressed throughout development, enriched in membranes of the cleavage furrow in early embryos, and in cells of the gut in advanced embryos. Furthermore, we find that sec1/munc18 co-localizes with its cognate binding partner syntaxin. Finally, our biochemical analysis shows that the protein associates with rab3 in high molecular weight complexes, suggesting that the exocytotic machinery functions as a multi-protein subunit to mediate regulated secretion in sea urchins. These results will be instrumental in the future to functionally test the SNARE regulators associated with multiple membrane fusion events.

摘要

调节性分泌由SNAREs(可溶性NSF附着受体)及其调节因子和效应器介导,其中包括SM(sec1/munc18)蛋白家族。在海胆中已鉴定出SNAREs的同源物,它们与受精时的皮质颗粒胞吐作用、分裂沟的膜以及发育后期的分泌细胞相关。为了有助于理解海胆中的调节性分泌,我们从两种海胆——多棘刺海胆和紫球海胆中克隆了单一的SM蛋白同源物。在卵母细胞和卵子中,我们发现它定位于质膜和卵子的皮质区域,这与它在导致皮质颗粒胞吐作用的步骤之一中所起的作用一致。该蛋白在整个发育过程中也有表达,在早期胚胎的分裂沟膜中富集,在晚期胚胎的肠道细胞中也有富集。此外,我们发现sec1/munc18与其同源结合伴侣 syntaxin共定位。最后,我们的生化分析表明,该蛋白与rab3在高分子量复合物中结合,这表明胞吐机制作为一个多蛋白亚基发挥作用,以介导海胆中的调节性分泌。这些结果将有助于未来对与多种膜融合事件相关的SNARE调节因子进行功能测试。

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