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Regulation of sodium-calcium exchanger activity by creatine kinase

机译:肌酸激酶对钠钙交换剂活性的调节

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摘要

It has been shown that in rat heart NCX1 exists in a macromolecular complex including PKA, PKA-anchoring protein, PKC, and phosphatases PP1 and PP2A. In addition, several lines of evidence suggest that the interactions of the exchanger with other molecules are closely associated with its function in regulation of [Ca2+]i. NCX contains a large intracellular loop (NCXIL) that is responsible for regulating NCX activity. We used the yeast two-hybrid method to screen a human heart cDNA library and found that the C-terminal region of sarcomeric mitochondrial creatine kinase (sMiCK) interacted with NCX1IL. Among the four creatine kinase (CK) isozymes, both sMiCK and the muscle-type cytosolic creatine kinase (CKM) co-immunoprecipitated with NCX1. Both sMiCK and CKM were able to produce a recovery in the decreased NCX1 activity that was lost under energy-compromised conditions. This regulation is mediated through a putative PKC phosphorylation site of sMiCK and CKM. The catalytic activity of sMiCK and CKM is not required for their regulation of NCX1 activity. Our results suggest a novel mechanism for the regulation of NCX1 activity and a novel role for CK.
机译:已经显示,在大鼠心脏中,NCX1存在于大分子复合物中,包括PKA,锚定PKA的蛋白质,PKC和磷酸酶PP1和PP2A。此外,一些证据表明,交换剂与其他分子的相互作用与其在[Ca2 +] i调控中的功能密切相关。 NCX包含一个大的细胞内环(NCXIL),负责调节NCX活性。我们使用酵母双杂交法筛选人心脏cDNA文库,发现肌节线粒体肌酸激酶(sMiCK)的C末端区域与NCX1IL相互作用。在四种肌酸激酶(CK)同工酶中,sMiCK和肌肉型胞质肌酸激酶(CKM)均与NCX1免疫共沉淀。 sMiCK和CKM都能在能量受损条件下丧失的NCX1活性下降中恢复。该调节通过假定的sMiCK和CKM的PKC磷酸化位点介导。 sMiCK和CKM的催化活性对于调节NCX1活性不是必需的。我们的结果提出了一种调控NCX1活性的新机制和CK的新作用。

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