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在单个胞吐事件中对胰岛素囊泡膜和货物进行同步倏逝波成像。

Simultaneous evanescent wave imaging of insulin vesicle membrane and cargo during a single exocytotic event.

作者信息

Tsuboi T, Zhao C, Terakawa S, Rutter G A

机构信息

Photon Medical Research Center, Hamamatsu University School of Medicine, Japan.

出版信息

Curr Biol. 2000 Oct 19;10(20):1307-10. doi: 10.1016/s0960-9822(00)00756-9.

DOI:10.1016/s0960-9822(00)00756-9
PMID:11069115
Abstract

The classical model of secretory vesicle recycling after exocytosis involves the retrieval of membrane (the omega figure) at a different site. An alternative model involves secretory vesicles transiently fusing with the plasma membrane (the 'kiss and run' mechanism) [1,2]. No continuous observation of the fate of a single secretory vesicle after exocytosis has been made to date. To study the dynamics of fusion immediately following exocytosis of insulin-containing vesicles, enhanced green fluorescent protein (EGFP) fused to the vesicle membrane protein phogrin [3] was delivered to the secretory vesicle membrane of INS-1 beta-cells using an adenoviral vector. The behaviour of the vesicle membrane during single exocytotic events was then examined using evanescent wave microscopy [4-6]. In unstimulated cells, secretory vesicles showed only slow Brownian movement. After a depolarizing pulse, most vesicles showed a small decrease in phogrin-EGFP fluorescence, and some moved laterally over the plasma membrane for approximately 1 microm. In contrast, secretory vesicles loaded with acridine orange all showed a transient (33-100 ms) increase in fluorescence intensity followed by rapid disappearance. Simultaneous observations of phogrin-EGFP and acridine orange indicated that the decrease in EGFP fluorescence occurred at the time of the acridine orange release, and that the lateral movement of EGFP-expressing vesicles occurred after this. Post-exocytotic retrieval of the vesicle membrane in INS-1 cells is thus slow, and can involve the movement of empty vesicles under the plasma membrane ('kiss and glide').

摘要

胞吐作用后分泌囊泡回收的经典模型涉及在不同位点回收膜(Ω形结构)。另一种模型涉及分泌囊泡与质膜瞬时融合(“亲吻并跑”机制)[1,2]。迄今为止,尚未对单个分泌囊泡在胞吐作用后的命运进行连续观察。为了研究含胰岛素囊泡胞吐作用后立即发生的融合动态,使用腺病毒载体将与囊泡膜蛋白嗜铬粒蛋白融合的增强型绿色荧光蛋白(EGFP)[3]递送至INS-1β细胞的分泌囊泡膜。然后使用倏逝波显微镜[4-6]检查单个胞吐事件期间囊泡膜的行为。在未受刺激的细胞中,分泌囊泡仅表现出缓慢的布朗运动。去极化脉冲后,大多数囊泡的嗜铬粒蛋白-EGFP荧光略有下降,一些囊泡在质膜上横向移动约1微米。相比之下,装载吖啶橙的分泌囊泡均显示荧光强度瞬时增加(33-100毫秒),随后迅速消失。对嗜铬粒蛋白-EGFP和吖啶橙的同步观察表明,EGFP荧光的下降发生在吖啶橙释放时,而表达EGFP的囊泡的横向移动在此之后发生。因此,INS-1细胞中囊泡膜的胞吐后回收是缓慢的,并且可能涉及空囊泡在质膜下的移动(“亲吻并滑行”)。

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Simultaneous evanescent wave imaging of insulin vesicle membrane and cargo during a single exocytotic event.在单个胞吐事件中对胰岛素囊泡膜和货物进行同步倏逝波成像。
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