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在培养的人皮肤角质形成细胞中进行细胞外膜联蛋白II的免疫细胞化学检测以及分离细胞外池中富集的膜联蛋白II亚型。

Immunocytochemical detection of extracellular annexin II in cultured human skin keratinocytes and isolation of annexin II isoforms enriched in the extracellular pool.

作者信息

Ma A S, Bell D J, Mittal A A, Harrison H H

机构信息

Department of Medicine, University of Chicago, Illinois 60637.

出版信息

J Cell Sci. 1994 Jul;107 ( Pt 7):1973-84. doi: 10.1242/jcs.107.7.1973.

Abstract

Monoclonal antibodies were raised against trypsinized human skin epidermal cells and selected for their staining of the epidermal cells in a cell periphery pattern. One antibody, CP-1, immunoprecipitated a 36 kDa protein that was identified as annexin II heavy chain by microsequencing of a CNBr-generated peptide fragment from the antigen and by cross-identification with another anti-annexin II antibody. In addition to staining a broad cell periphery band in keratinocytes, CP-1 also detected annexin II outside and in between the top layer cells before cell permeabilization. Double-labeling of annexin II and F-actin revealed a distinct topographical relationship between the two, with intercellular annexin II flanked by the submembranously located actin of the juxta-positioned cells. Annexin II was isolated from cultured keratinocytes via immunoaffinity column chromatography in one step, using the same monoclonal antibody CP-1 and was found to be resolved into multiple isoforms when analyzed by two-dimensional gel electrophoresis. The predominant components of annexin II were basic, with pI of 6.5-8.5, and some of them formed disulfide-linked monomeric multimers under non-reducing conditions. Acidic annexin II isoforms with pI 5.4-5.8 were barely detectable among the total annexin II isolated but were selectively enriched in an extracellular pool created by 0.05% ethylenediaminetetraacetic acid (EDTA) dispersion of the cultured cells into single cell suspensions. Furthermore, they can be separated from the rest of annexin II by using a different elution condition. A 46 kDa protein, the identity of which is unclear, co-eluted with the acidic isoforms in the EDTA washes. These acidic isoforms, which co-eluted with the 46 kDa protein, are suspected of corresponding to the extracellular annexin II detected immunocytochemically.

摘要

制备了针对胰蛋白酶处理的人皮肤表皮细胞的单克隆抗体,并选择那些能以细胞周边模式对表皮细胞进行染色的抗体。一种名为CP-1的抗体免疫沉淀了一种36 kDa的蛋白质,通过对来自抗原的溴化氰生成的肽片段进行微量测序以及与另一种抗膜联蛋白II抗体交叉鉴定,该蛋白质被确定为膜联蛋白II重链。除了在角质形成细胞中染出一条宽的细胞周边带外,CP-1还能在细胞通透前检测到顶层细胞外部和之间的膜联蛋白II。膜联蛋白II和F-肌动蛋白的双重标记揭示了两者之间独特的拓扑关系,细胞间的膜联蛋白II两侧是相邻细胞位于膜下的肌动蛋白。使用相同的单克隆抗体CP-1,通过免疫亲和柱色谱一步从培养的角质形成细胞中分离出膜联蛋白II,二维凝胶电泳分析发现其可分为多种异构体。膜联蛋白II的主要成分呈碱性,pI为6.5 - 8.5,其中一些在非还原条件下形成二硫键连接的单体多聚体。在分离得到的总膜联蛋白II中几乎检测不到pI为5.4 - 5.8的酸性膜联蛋白II异构体,但在通过0.05%乙二胺四乙酸(EDTA)将培养细胞分散成单细胞悬液所形成的细胞外池中选择性富集。此外,通过不同的洗脱条件可以将它们与其余的膜联蛋白II分离。一种身份不明的46 kDa蛋白质在EDTA洗脱液中与酸性异构体共洗脱。这些与46 kDa蛋白质共洗脱的酸性异构体被怀疑对应于免疫细胞化学检测到的细胞外膜联蛋白II。

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