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鉴定一种将离子转运与蛋白激酶活性偶联的潜在受体。

Identification of a potential receptor that couples ion transport to protein kinase activity.

机构信息

Department of Physiology, University of Toledo College of Medicine, Toledo, Ohio 43614, USA.

出版信息

J Biol Chem. 2011 Feb 25;286(8):6225-32. doi: 10.1074/jbc.M110.202051. Epub 2010 Dec 27.

Abstract

In our previous studies, we have demonstrated that the Src-coupled α1 Na/K-ATPase works as a receptor for cardiotonic steroids, such as ouabain, to regulate cellular protein kinase cascades. Here, we explore further the structural determinants of the interaction between the α1 Na/K-ATPase and Src and demonstrate that the Src-coupled α1 Na/K-ATPase allows the cell to decode the transmembrane transport activity of the Na/K-ATPase to turn on/off protein kinases. The α1 Na/K-ATPase undergoes E1/E2 conformational transition during an ion pumping cycle. The amount of E1 and E2 Na/K-ATPase is regulated by extracellular K(+) and intracellular Na(+). Using purified enzyme preparations we find that the E1 Na/K-ATPase can bind both the Src SH2 and kinase domains simultaneously and keep Src in an inactive state. Conversely, the E1 to E2 transition releases the kinase domain and activates the associated Src. Moreover, we demonstrate that changes in E1/E2 Na/K-ATPase by either Na(+) or K(+) are capable of regulating Src and Src effectors in live cells. Together, the data suggest that the Src-coupled α1 Na/K-ATPase may act as a Na(+)/K(+) receptor, allowing salt to regulate cellular function through Src and Src effectors.

摘要

在我们之前的研究中,已经证明Src 偶联的α1 Na/K-ATP 酶可以作为强心甾类物质(如哇巴因)的受体,调节细胞蛋白激酶级联反应。在这里,我们进一步探讨了α1 Na/K-ATP 酶与Src 相互作用的结构决定因素,并证明 Src 偶联的α1 Na/K-ATP 酶允许细胞解码 Na/K-ATP 酶的跨膜转运活性,从而开启/关闭蛋白激酶。α1 Na/K-ATP 酶在离子转运循环中经历 E1/E2 构象转变。E1 和 E2 Na/K-ATP 酶的数量受细胞外 K+和细胞内 Na+的调节。使用纯化的酶制剂,我们发现 E1 Na/K-ATP 酶可以同时结合Src SH2 和激酶结构域,并使 Src 处于非活性状态。相反,E1 到 E2 的转变释放激酶结构域并激活相关的 Src。此外,我们证明了 Na+或 K+引起的 E1/E2 Na/K-ATP 酶的变化能够调节活细胞中的 Src 和 Src 效应物。总之,这些数据表明,Src 偶联的α1 Na/K-ATP 酶可能作为 Na+/K+受体,允许盐通过 Src 和 Src 效应物来调节细胞功能。

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