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肌球蛋白 IIB 和 F-肌动蛋白控制胃壁细胞中含 H-K-ATPase 的小管泡囊的顶泡形态和组胺诱导的运输。

Myosin IIB and F-actin control apical vacuolar morphology and histamine-induced trafficking of H-K-ATPase-containing tubulovesicles in gastric parietal cells.

机构信息

Department of Molecular and Cell Biology, University of California, Berkeley, California; and.

出版信息

Am J Physiol Gastrointest Liver Physiol. 2014 Apr 15;306(8):G699-710. doi: 10.1152/ajpgi.00316.2013. Epub 2014 Feb 27.

Abstract

Selective inhibitors of myosin or actin function and confocal microscopy were used to test the role of an actomyosin complex in controlling morphology, trafficking, and fusion of tubulovesicles (TV) containing H-K-ATPase with the apical secretory canaliculus (ASC) of primary-cultured rabbit gastric parietal cells. In resting cells, myosin IIB and IIC, ezrin, and F-actin were associated with ASC, whereas H-K-ATPase localized to intracellular TV. Histamine caused fusion of TV with ASC and subsequent expansion resulting from HCl and water secretion; F-actin and ezrin remained associated with ASC whereas myosin IIB and IIC appeared to dissociate from ASC and relocalize to the cytoplasm. ML-7 (inhibits myosin light chain kinase) caused ASC of resting cells to collapse and most myosin IIB, F-actin, and ezrin to dissociate from ASC. TV were unaffected by ML-7. Jasplakinolide (stabilizes F-actin) caused ASC to develop large blebs to which actin, myosin II, and ezrin, as well as tubulin, were prominently localized. When added prior to stimulation, ML-7 and jasplakinolide prevented normal histamine-stimulated transformations of ASC/TV and the cytoskeleton, but they did not affect cells that had been previously stimulated with histamine. These results indicate that dynamic pools of actomyosin are required for maintenance of ASC structure in resting cells and for trafficking of TV to ASC during histamine stimulation. However, the dynamic pools of actomyosin are not required once the histamine-stimulated transformation of TV/ASC and cytoskeleton has occurred. These results also show that vesicle trafficking in parietal cells shares mechanisms with similar processes in renal collecting duct cells, neuronal synapses, and skeletal muscle.

摘要

选择肌球蛋白或肌动蛋白功能的抑制剂和共聚焦显微镜来测试肌动球蛋白复合物在控制形态、运输和含有 H-K-ATPase 的小管泡(TV)与初级培养兔胃壁细胞的顶分泌道(ASC)融合中的作用。在静止细胞中,肌球蛋白 IIB 和 IIC、埃兹蛋白和 F-肌动蛋白与 ASC 相关,而 H-K-ATPase 定位于细胞内的 TV。组胺引起 TV 与 ASC 融合,随后由于 HCl 和水分泌而导致扩张;F-肌动蛋白和埃兹蛋白仍然与 ASC 相关,而肌球蛋白 IIB 和 IIC 似乎从 ASC 解离并重新定位到细胞质。ML-7(抑制肌球蛋白轻链激酶)导致静止细胞的 ASC 崩溃,大多数肌球蛋白 IIB、F-肌动蛋白和埃兹蛋白从 ASC 解离。TV 不受 ML-7 影响。 Jasplakinolide(稳定 F-肌动蛋白)导致 ASC 形成大泡,其中肌动蛋白、肌球蛋白 II 和埃兹蛋白以及微管蛋白都明显定位于 ASC。在刺激之前添加 ML-7 和 jasplakinolide 可防止正常的组胺刺激引起的 ASC/TV 和细胞骨架的转化,但它们不影响先前已被组胺刺激的细胞。这些结果表明,在静止细胞中维持 ASC 结构和在组胺刺激期间 TV 向 ASC 的运输需要肌动球蛋白的动态池。然而,一旦组胺刺激的 TV/ASC 和细胞骨架的转化发生,肌动球蛋白的动态池就不再需要了。这些结果还表明,壁细胞中的囊泡运输与肾集合管细胞、神经元突触和骨骼肌中的类似过程具有共同的机制。

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