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一种主要在上皮细胞中表达的与sec1相关的囊泡运输蛋白。

A sec1-related vesicle-transport protein that is expressed predominantly in epithelial cells.

作者信息

Riento K, Jäntti J, Jansson S, Hielm S, Lehtonen E, Ehnholm C, Keränen S, Olkkonen V M

机构信息

Department of Biochemistry, National Public Health Institute, Helsinki, Finland.

出版信息

Eur J Biochem. 1996 Aug 1;239(3):638-46. doi: 10.1111/j.1432-1033.1996.0638u.x.

Abstract

Sec1-related proteins are involved in docking and fusion of transport vesicles in eukaryotic cells. Here we report the cloning and molecular characterization of a Sec1-related protein expressed in the MDCK epithelial cell line. This protein represents a canine counterpart of the murine Munc-18-2/Munc-18b/muSec1 protein, displays 93% amino acid identity with these proteins, has a similar tissue mRNA expression pattern, and associates in vitro with syntaxins 1A, 2, and 3. In situ hybridization analysis of embryonic mouse tissues revealed prominent expression of the munc-18-2 mRNA in the epithelia of several tissues. Cell-fractionation studies demonstrated that the majority of Munc-18-2 is membrane associated. Most of the protein is washed off the membranes by sodium carbonate, pH 11.5. However, the protein is poorly solubilized by detergent treatment. The Munc-18-2 protein was localized, by immunofluorescence microscopy, to the plasma membrane of MDCK cells, and is apically distributed in the epithelial cells of mouse tissues. When overexpressed in COS-1 cells, the protein appeared to be largely cytosolic. However, upon expression with syntaxin 1A, it displayed a shift to the plasma membrane, where the two proteins colocalized. These results identified Munc-18-2 as a predominantly epithelial vesicle-transport protein with a polarized distribution and provided novel in vivo evidence for the association of Sec1-related proteins with members of the syntaxin family.

摘要

Sec1相关蛋白参与真核细胞中运输小泡的对接和融合。在此,我们报告了在MDCK上皮细胞系中表达的一种Sec1相关蛋白的克隆及分子特征。该蛋白代表鼠类Munc-18-2/Munc-18b/muSec1蛋白的犬类对应物,与这些蛋白具有93%的氨基酸同一性,具有相似的组织mRNA表达模式,并且在体外与 syntaxins 1A、2和3相互作用。对胚胎小鼠组织的原位杂交分析显示,munc-18-2 mRNA在多个组织的上皮中显著表达。细胞分级分离研究表明,大多数Munc-18-2与膜相关。大多数蛋白可被pH 11.5的碳酸钠从膜上洗脱。然而,该蛋白经去污剂处理后溶解性较差。通过免疫荧光显微镜观察,Munc-18-2蛋白定位于MDCK细胞的质膜,并在小鼠组织的上皮细胞中呈顶端分布。当在COS-1细胞中过表达时,该蛋白似乎主要存在于胞质中。然而,与syntaxin 1A一起表达时,它会向质膜转移,两种蛋白在质膜上共定位。这些结果确定Munc-18-2是一种主要存在于上皮细胞中的囊泡运输蛋白,具有极化分布,并为Sec1相关蛋白与syntaxin家族成员的关联提供了新的体内证据。

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