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内分泌β细胞中突触结合蛋白异构体的表达与定位:它们在胰岛素胞吐作用中的功能

Expression and localisation of synaptotagmin isoforms in endocrine beta-cells: their function in insulin exocytosis.

作者信息

Gut A, Kiraly C E, Fukuda M, Mikoshiba K, Wollheim C B, Lang J

机构信息

Division de Biochimie Clinique, Département de Médecine, Université de Genève, CH-1211 Genève 4, Switzerland.

出版信息

J Cell Sci. 2001 May;114(Pt 9):1709-16. doi: 10.1242/jcs.114.9.1709.

DOI:10.1242/jcs.114.9.1709
PMID:11309201
Abstract

Exocytosis of insulin containing Large Dense Core Vesicles (LDCVs) from pancreatic beta-cells and derived cell lines is mainly controlled by Ca(2+). Several lines of evidence have demonstrated a role of the Ca(2+)- and phospholipid-binding protein synaptotagmin (syt) in this event. Synaptotagmins form a large protein family with distinct affinities for Ca(2+) determined by their two C(2) domains (C(2)A/B). Except for the well-characterized isoforms I and II, their role is still unclear. We have used here insulin-secreting cells as a model system for LDCV exocytosis to gain insight into the function of synaptotagmins. Immunocytochemical analysis revealed that of the candidate Ca(2+) sensors in LDCV exocytosis, syt III was not expressed in primary beta-cells, whereas syt IV was only found adjacent to the TGN. However, syt V-VIII isoforms were expressed at different levels in various insulin-secreting cells and in pancreatic islet preparations. In streptolysin-O permeabilized primary beta-cells the introduction of recombinant peptides (100 nM) corresponding to the C(2) domains of syt V, VII and VIII, but not of syt III, IV or VI, inhibited Ca(2+)-evoked insulin exocytosis by 30% without altering GTP gamma S-induced release. Our observations demonstrate that syt III and IV are not involved in the exocytosis of LDCVs from primary beta-cells whereas V, VII and VIII may mediate Ca(2+)-regulation of exocytosis.

摘要

胰腺β细胞及衍生细胞系中含大致密核心囊泡(LDCV)的胰岛素胞吐作用主要受Ca(2+)调控。多条证据表明Ca(2+)与磷脂结合蛋白突触结合蛋白(syt)在此过程中发挥作用。突触结合蛋白形成一个大的蛋白家族,其两个C(2)结构域(C(2)A/B)决定了它们对Ca(2+)具有不同的亲和力。除了特征明确的I型和II型异构体,它们的作用仍不清楚。我们在此使用胰岛素分泌细胞作为LDCV胞吐作用的模型系统,以深入了解突触结合蛋白的功能。免疫细胞化学分析显示,在LDCV胞吐作用的候选Ca(2+)传感器中,syt III在原代β细胞中不表达,而syt IV仅在高尔基体反面网状结构(TGN)附近发现。然而,syt V - VIII异构体在各种胰岛素分泌细胞和胰岛制剂中以不同水平表达。在经链球菌溶血素 - O通透处理的原代β细胞中,引入对应于syt V、VII和VIII的C(2)结构域的重组肽(100 nM),而不是syt III、IV或VI的重组肽,可抑制Ca(2+)诱发的胰岛素胞吐作用30%,而不改变GTPγS诱导的释放。我们的观察结果表明,syt III和IV不参与原代β细胞中LDCV的胞吐作用,而V、VII和VIII可能介导Ca(2+)对胞吐作用的调节。

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