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本文引用的文献

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Integrin CD11a cytoplasmic tail interacts with the CD45 membrane-proximal protein tyrosine phosphatase domain 1.整合素CD11a胞质尾与CD45膜近端蛋白酪氨酸磷酸酶结构域1相互作用。
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整合素α4β1通过c-Src的α4胞质结构域特异性激活促进不依赖粘着斑激酶的细胞运动。

Integrin alpha4beta1 promotes focal adhesion kinase-independent cell motility via alpha4 cytoplasmic domain-specific activation of c-Src.

作者信息

Hsia Datsun A, Lim Ssang-Taek, Bernard-Trifilo Joie A, Mitra Satyajit K, Tanaka Sakae, den Hertog Jeroen, Streblow Daniel N, Ilic Dusko, Ginsberg Mark H, Schlaepfer David D

机构信息

The Scripps Research Institute, Department of Immunology, IMM21, 10550 N. Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

Mol Cell Biol. 2005 Nov;25(21):9700-12. doi: 10.1128/MCB.25.21.9700-9712.2005.

DOI:10.1128/MCB.25.21.9700-9712.2005
PMID:16227616
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1265817/
Abstract

The fibronectin binding integrins alpha5beta1 and alpha4beta1 generate signals pivotal for cell migration through distinct yet undefined mechanisms. For alpha5beta1, beta1-mediated activation of focal adhesion kinase (FAK) promotes c-Src recruitment to FAK and the formation of a FAK-Src signaling complex. Herein, we show that FAK expression is essential for alpha5beta1-stimulated cell motility and that exogenous expression of human alpha4 in FAK-null fibroblasts forms a functional alpha4beta1 receptor that promotes robust cell motility equal to the alpha5beta1 stimulation of wild-type and FAK-reconstituted fibroblasts. alpha4beta1-stimulated FAK-null cell spreading and motility were dependent on the integrity of the alpha4 cytoplasmic domain, independent of direct paxillin binding to alpha4, and were not affected by PRNK expression, a dominant-negative inhibitor of Pyk2. alpha4 cytoplasmic domain-initiated signaling led to a approximately 4-fold activation of c-Src which did not require paxillin binding to alpha4. Notably, alpha4-stimulated cell motility was inhibited by catalytically inactive receptor protein-tyrosine phosphatase alpha overexpression and blocked by the p50Csk phosphorylation of c-Src at Tyr-529. alpha4beta1-stimulated cell motility of triple-null Src(-/-), c-Yes(-/-), and Fyn(-/-) fibroblasts was dependent on c-Src reexpression that resulted in p130Cas tyrosine phosphorylation and Rac GTPase loading. As p130Cas phosphorylation and Rac activation are common downstream targets for alpha5beta1-stimulated FAK activation, our results support the existence of a novel alpha4 cytoplasmic domain connection leading to c-Src activation which functions as a FAK-independent linkage to a common motility-promoting signaling pathway.

摘要

纤连蛋白结合整合素α5β1和α4β1通过不同但尚未明确的机制产生对细胞迁移至关重要的信号。对于α5β1,β1介导的粘着斑激酶(FAK)激活促进c-Src募集到FAK并形成FAK-Src信号复合物。在此,我们表明FAK表达对于α5β1刺激的细胞运动至关重要,并且在FAK缺失的成纤维细胞中外源表达人α4可形成功能性α4β1受体,该受体促进的强大细胞运动等同于野生型和FAK重组的成纤维细胞的α5β1刺激。α4β1刺激的FAK缺失细胞铺展和运动依赖于α4细胞质结构域的完整性,独立于桩蛋白与α4的直接结合,并且不受PRNK表达(一种Pyk2的显性负性抑制剂)的影响。α4细胞质结构域启动的信号传导导致c-Src约4倍的激活,这不需要桩蛋白与α4结合。值得注意的是,α4刺激的细胞运动受到催化失活的受体蛋白酪氨酸磷酸酶α过表达的抑制,并被c-Src在Tyr-529处的p50Csk磷酸化所阻断。α4β1刺激的Src(-/-)、c-Yes(-/-)和Fyn(-/-)三基因缺失成纤维细胞的细胞运动依赖于c-Src的重新表达,这导致p130Cas酪氨酸磷酸化和Rac GTP酶负载。由于p130Cas磷酸化和Rac激活是α5β1刺激的FAK激活的常见下游靶点,我们的结果支持存在一种新的α4细胞质结构域连接,导致c-Src激活,其作为与共同的促进运动信号通路的FAK非依赖性连接发挥作用。