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质膜 Ca2+泵酸性脂质结合区的缺失和突变:对 2 型同工型不同剪接变体的研究。

Deletions and mutations in the acidic lipid-binding region of the plasma membrane Ca2+ pump: a study on different splicing variants of isoform 2.

机构信息

Department of Biological Chemistry, University of Padova, 35131 Padova, Italy.

出版信息

J Biol Chem. 2010 Oct 1;285(40):30779-91. doi: 10.1074/jbc.M110.140475. Epub 2010 Jul 19.

Abstract

Acidic phospholipids increase the affinity of the plasma membrane Ca(2+)-ATPase pump for Ca(2+). They interact with the C-terminal region of the pump and with a domain in the loop connecting transmembrane domains 2 and 3 (A(L) region) next to site A of alternative splicing. The contribution of the two phospholipid-binding sites and the possible interference of splicing inserts at site A with the regulation of the ATPase activity of isoform 2 of the pump by phospholipids have been analyzed. The activity of the full-length z/b variant (no insert at site A), the w/b (with insert at site A), and the w/a variant, containing both the 45-amino acid A-site insert and a C-site insert that truncates the pump in the calmodulin binding domain, has been analyzed in microsomal membranes of overexpressing CHO cells. The A-site insertion did not modify the phospholipid sensitivity of the pump, but the doubly inserted w/a variant became insensitive to acidic phospholipids, even if containing the intact A(L) phospholipid binding domain. Pump mutants in which 12 amino acids had been deleted, or single lysine mutations introduced, in the A(L) region were studied by monitoring agonist-induced Ca(2+) transients in overexpressing CHO cells. The 12-residue deletion completely abolished the ATPase activity of the w/a variant but only reduced that of the z/b variant, which was also affected by the single lysine substitutions in the same domain. A structural interpretation of the interplay of the pump with phospholipids, and of the mechanism of their activation, is proposed on the basis of molecular modeling studies.

摘要

酸性磷脂可提高质膜 Ca(2+)-ATP 酶泵对 Ca(2+)的亲和力。它们与泵的 C 端区域以及跨膜域 2 和 3 之间的环(A(L) 区域)中的一个域相互作用,该域紧邻交替剪接的 A 位点。已分析了两个磷脂结合位点的贡献以及 A 位点剪接插入物对磷脂调节泵同工型 2 的 ATP 酶活性的可能干扰。全长 z/b 变体(A 位点无插入)、w/b(A 位点有插入)和 w/a 变体(含有 A 位点的 45 个氨基酸插入物和截断钙调蛋白结合域的 C 位点插入物)的活性在过表达 CHO 细胞的微粒体膜中进行了分析。A 位点的插入并没有改变泵对磷脂的敏感性,但双插入的 w/a 变体对酸性磷脂变得不敏感,即使含有完整的 A(L)磷脂结合域。在 A(L)区域中删除 12 个氨基酸或引入单个赖氨酸突变的泵突变体通过监测过表达 CHO 细胞中的激动剂诱导的 Ca(2+)瞬变进行了研究。12 个残基的缺失完全消除了 w/a 变体的 ATP 酶活性,但仅降低了 z/b 变体的活性,该变体也受到同一结构域中单个赖氨酸取代的影响。基于分子建模研究,提出了泵与磷脂相互作用的结构解释,以及它们的激活机制。

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