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细胞黏附于纤连蛋白的协同位点的需求取决于整合素α5β1的激活状态。

Requirement for the synergy site for cell adhesion to fibronectin depends on the activation state of integrin alpha 5 beta 1.

作者信息

Danen E H, Aota S, van Kraats A A, Yamada K M, Ruiter D J, van Muijen G N

机构信息

Department of Pathology, University Hospital, Nijmegen, The Netherlands.

出版信息

J Biol Chem. 1995 Sep 15;270(37):21612-8. doi: 10.1074/jbc.270.37.21612.

DOI:10.1074/jbc.270.37.21612
PMID:7545166
Abstract

We investigated the influence of the activation state of integrin alpha 5 beta 1 on its dependence on the PHSRN synergy site for binding to RGD in fibronectin. K562 and MV3 cells lacked alpha v beta 3 expression and adhered to fibronectin through alpha 5 beta 1. Mel57 cells adhered through alpha v beta 3 and alpha 5 beta 1. A recombinant fibronectin polypeptide, containing five type III repeats from the central cell binding domain 3Fn6-10, and a mutated polypeptide lacking the synergy site were equally effective in promoting Mel57 adhesion. For K562 and MV3, the mutated polypeptide was not or poorly active compared to the control polypeptide. Expression of alpha v beta 3 in MV3 induced strong adhesion to the mutated polypeptide. TS2/16 stimulatory beta 1-integrin antibodies or Mn2+ induced alpha 5 beta 1-mediated adhesion of K562 and MV3 to GRGDSP. In the presence of TS2/16 or Mn2+, alpha 5 beta 1-mediated MV3 adhesion to the mutated polypeptide was equally strong as adhesion to the control polypeptide. Mn2+ or TS2/16 induced weak K562 binding to the mutated polypeptide, and in the presence of a combination of phorbol 12-myristate 13-acetate, Mn2+, and TS2/16, alpha 5 beta 1-mediated K562 adhesion to the mutated and control polypeptide was equally strong. Our findings demonstrate that requirement for the PHSRN synergy site for alpha 5 beta 1-mediated adhesion to RGD in fibronectin depends on the activation state of the integrin.

摘要

我们研究了整合素α5β1的激活状态对其依赖PHSRN协同位点与纤连蛋白中RGD结合的影响。K562和MV3细胞缺乏αvβ3表达,通过α5β1黏附于纤连蛋白。Mel57细胞通过αvβ3和α5β1黏附。一种包含来自中央细胞结合结构域的五个III型重复序列的重组纤连蛋白多肽3Fn6 - 10,以及一个缺乏协同位点的突变多肽在促进Mel57黏附方面同样有效。对于K562和MV3,与对照多肽相比,突变多肽无活性或活性较差。MV3中αvβ3的表达诱导了对突变多肽的强烈黏附。TS2/16刺激型β1整合素抗体或Mn2+诱导K562和MV3的α5β1介导的对GRGDSP的黏附。在存在TS2/16或Mn2+的情况下,α5β1介导的MV3对突变多肽的黏附与对对照多肽的黏附同样强烈。Mn2+或TS2/16诱导K562与突变多肽的弱结合,并且在佛波醇12 - 肉豆蔻酸酯13 - 乙酸酯、Mn2+和TS2/16的组合存在时,α5β1介导的K562对突变多肽和对照多肽的黏附同样强烈。我们的研究结果表明,α5β1介导的与纤连蛋白中RGD黏附对PHSRN协同位点的需求取决于整合素的激活状态。

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