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钙诱导人角质形成细胞中钙黏蛋白、整合素及其相关细胞质蛋白的分布和溶解性变化。

Calcium-induced changes in distribution and solubility of cadherins, integrins and their associated cytoplasmic proteins in human keratinocytes.

作者信息

Braga V M, Hodivala K J, Watt F M

机构信息

Keratinocyte Laboratory, Imperial Cancer Research Fund, London, U.K.

出版信息

Cell Adhes Commun. 1995 Aug;3(3):201-15. doi: 10.3109/15419069509081287.

Abstract

Studies with cultured human epidermal keratinocytes have shown that stratification, the movement of differentiating cells out of the basal layer, involves changes in cell-extracellular matrix and cell-cell adhesiveness mediated by receptors of the integrin and cadherin families, respectively. Keratinocytes normally lose their integrins when they initiate terminal differentiation. However, when stratification is inhibited by a low concentration of calcium ions in the medium (0.1 mM) or by addition of antibodies to P- and E-cadherin in standard medium (1.8 mM calcium ions), differentiating, involucrin-positive, cells continue to express functional integrins. In order to investigate the mechanism by which cadherins may regulate integrin expression, we have examined the distribution and detergent solubility of the receptors and associated cytoplasmic proteins in keratinocytes grown as a monolayer in low calcium medium or transferred to standard medium to induce stratification. Within 1 hour of raising the concentration of calcium ions, integrins, cadherins, alpha-catenin, beta-catenin, plakoglobin, vinculin and alpha-actinin appeared to accumulate at cell-cell borders, whereas the focal contact proteins, paxillin and talin, did not. The change in distribution was correlated with decreased solubility in 0.5% Triton X-100 of some of the proteins examined, but the integrins, alpha-actinin, paxillin and talin remained completely soluble. Addition of cytochalasin D inhibited both the redistribution of proteins and subsequent stratification of involucrin-positive cells. Cycloheximide treatment allowed protein redistribution and stratification, but involucrin-positive cells continued to express integrins. These results suggest that stratification requires the interactions of cadherins and integrins with the actin cytoskeleton and that the selective loss of integrins from differentiating cells requires de novo protein synthesis.

摘要

对培养的人表皮角质形成细胞的研究表明,分层现象,即分化细胞从基底层移出的过程,分别涉及由整合素家族和钙黏蛋白家族受体介导的细胞 - 细胞外基质及细胞 - 细胞黏附性的变化。角质形成细胞在开始终末分化时通常会失去其整合素。然而,当培养基中低浓度钙离子(0.1 mM)或在标准培养基(1.8 mM钙离子)中添加针对P - 钙黏蛋白和E - 钙黏蛋白的抗体抑制分层时,正在分化的、表达内聚蛋白的细胞会继续表达功能性整合素。为了研究钙黏蛋白调节整合素表达的机制,我们检测了在低钙培养基中单层生长或转移至标准培养基以诱导分层的角质形成细胞中,这些受体及相关细胞质蛋白的分布和去污剂溶解性。钙离子浓度升高后1小时内,整合素、钙黏蛋白、α - 连环蛋白、β - 连环蛋白、桥粒斑蛋白、纽蛋白和α - 辅肌动蛋白似乎在细胞 - 细胞边界处聚集,而粘着斑蛋白桩蛋白和踝蛋白则没有。分布的变化与所检测的一些蛋白质在0.5% Triton X - 100中的溶解性降低相关,但整合素、α - 辅肌动蛋白、桩蛋白和踝蛋白仍完全可溶。细胞松弛素D的添加抑制了蛋白质的重新分布以及随后内聚蛋白阳性细胞的分层。放线菌酮处理允许蛋白质重新分布和分层,但内聚蛋白阳性细胞继续表达整合素。这些结果表明,分层需要钙黏蛋白和整合素与肌动蛋白细胞骨架相互作用,并且分化细胞中整合素的选择性丢失需要从头合成蛋白质。

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