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肌动蛋白结合蛋白 scinderin 在 PC12 细胞中发挥作用,在分泌前将致密核心囊泡固定。

The actin binding protein scinderin acts in PC12 cells to tether dense-core vesicles prior to secretion.

机构信息

Department of Anesthesia, Cincinnati Children's Hospital Medical Center, MLC2001, 3333 Burnet Avenue, Cincinnati, OH 45229, United States.

Department of Anesthesia, Cincinnati Children's Hospital Medical Center, MLC2001, 3333 Burnet Avenue, Cincinnati, OH 45229, United States; Department of Basic Pharmaceutical Sciences, Husson University School of Pharmacy, 1 College Circle, Bangor, ME 04401, United States.

出版信息

Mol Cell Neurosci. 2017 Dec;85:12-18. doi: 10.1016/j.mcn.2017.08.003. Epub 2017 Aug 18.

Abstract

Mechanistic understanding of the control of vesicle motion from within a secretory cell to the site of exocytosis remains incomplete. In this work, we have used total internal reflection (TIRF) microscopy to examine the mobility of secretory vesicles at the plasma membrane. Under resting conditions, we found vesicles showed little lateral mobility. Anchoring of vesicles in this membrane proximal compartment could be disrupted with latrunculin A, indicating an apparent actin dependent process. A candidate intermediary between vesicles and the actin skeleton is the actin binding protein scinderin. Co-transfection of an shRNA construct against scinderin blocked secretion, and also increased the mobility of vesicles in the membrane-proximal section of the cell, indicating a dual role for scinderin in secretion; tethering vesicles to the cytoskeleton, as well as liberating them following stimulation through the previously described calcium dependent actin severing activity. Analysis of lipid dependence indicates that scinderin exhibits calcium dependent binding to phosphatidyl-inositol monophosphate, providing a possible mechanism for vesicle binding.

摘要

从分泌细胞内部控制囊泡运动到胞吐部位的机制仍不完全清楚。在这项工作中,我们使用全内反射(TIRF)显微镜检查了质膜上分泌囊泡的流动性。在静息状态下,我们发现囊泡的侧向流动性很小。Latrunculin A 可以破坏囊泡在这个靠近膜的隔室中的锚定,表明这是一个明显依赖于肌动蛋白的过程。囊泡和肌动蛋白骨架之间的一个候选中间物是肌动蛋白结合蛋白 Scinderin。针对 Scinderin 的 shRNA 构建体的共转染阻断了分泌,并且还增加了细胞中靠近膜的区域中囊泡的流动性,表明 Scinderin 在分泌中具有双重作用;将囊泡固定在细胞骨架上,并在通过先前描述的钙依赖性肌动蛋白切割活性刺激后释放它们。对脂质依赖性的分析表明,Scinderin 表现出对肌醇单磷酸磷脂的钙依赖性结合,为囊泡结合提供了一种可能的机制。

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