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胞质型磷脂酶A2的C2钙依赖性脂质结合结构域的独立折叠和配体特异性

Independent folding and ligand specificity of the C2 calcium-dependent lipid binding domain of cytosolic phospholipase A2.

作者信息

Nalefski E A, McDonagh T, Somers W, Seehra J, Falke J J, Clark J D

机构信息

Small Molecule Drug Discovery Group, Genetics Institute, Inc., Cambridge, Massachusetts 02140, USA.

出版信息

J Biol Chem. 1998 Jan 16;273(3):1365-72. doi: 10.1074/jbc.273.3.1365.

DOI:10.1074/jbc.273.3.1365
PMID:9430670
Abstract

The Ca(2+)-dependent lipid binding domain of the 85-kDa cytosolic phospholipase A2 (cPLA2) is a homolog of C2 domains present in protein kinase C, synaptotagmin, and numerous other proteins involved in signal transduction. NH2-terminal fragments of cPLA2 spanning the C2 domain were expressed as inclusion bodies in Escherichia coli, extracted with solvent to remove phospholipids, and refolded to yield a domain capable of binding phospholipid vesicles in a Ca(2+)-dependent manner. Unlike other C2 domains characterized to date, the cPLA2 C2 domain bound preferentially to vesicles comprised of phosphatidylcholine in response to physiological concentrations of Ca2+. Binding of the cPLA2 C2 domain to vesicles in the presence of excess Ca2+ chelator was induced by high concentrations of salts that promote hydrophobic interactions. Despite the selective hydrolysis of arachidonyl-containing phospholipid vesicles by cPLA2, the cPLA2 C2 domain did not discriminate among phospholipid vesicles containing saturated or unsaturated sn-2 fatty acyl chains. Moreover, the cPLA2 C2 domain bound to phospholipid vesicles containing sn-1 and -2 ether linkages and sphingomyelin at Ca2+ concentrations that caused binding to vesicles containing ester linkages, demonstrating that the carbonyl oxygens of the sn-1 and -2 ester linkage are not critical for binding. These results suggest that the cPLA2 C2 domain interacts primarily with the headgroup of the phospholipid. The cPLA2 C2 domain displayed selectivity among group IIA cations, preferring Ca2+ approximately 50-fold over Sr2+ and nearly 10,000-fold over Ba2+ for vesicle binding. No binding to vesicles was observed in the presence of greater than 10 mM Mg2+. Such strong selectivity for Ca2+ over Mg2+ reinforces the view that C2 domains link second messenger Ca2+ to signal transduction events at the membrane.

摘要

85 kDa的胞质磷脂酶A2(cPLA2)的钙依赖性脂质结合结构域是蛋白激酶C、突触结合蛋白以及众多参与信号转导的其他蛋白质中存在的C2结构域的同源物。跨越C2结构域的cPLA2的氨基末端片段在大肠杆菌中以包涵体形式表达,用溶剂提取以去除磷脂,然后重折叠以产生能够以钙依赖性方式结合磷脂囊泡的结构域。与迄今所表征的其他C2结构域不同,cPLA2 C2结构域在生理浓度的Ca2+作用下优先结合由磷脂酰胆碱组成的囊泡。在存在过量钙螯合剂的情况下,cPLA2 C2结构域与囊泡的结合是由促进疏水相互作用的高浓度盐诱导的。尽管cPLA2对含花生四烯酰基的磷脂囊泡有选择性水解作用,但cPLA2 C2结构域在含有饱和或不饱和sn-2脂肪酰链的磷脂囊泡之间没有区分。此外,cPLA2 C2结构域在Ca2+浓度下与含有sn-1和-2醚键以及鞘磷脂的磷脂囊泡结合,而该Ca2+浓度会导致其与含有酯键的囊泡结合,这表明sn-1和-2酯键的羰基氧对于结合并非至关重要。这些结果表明,cPLA2 C2结构域主要与磷脂的头部基团相互作用。cPLA2 C2结构域在IIA族阳离子中表现出选择性,对于囊泡结合,其对Ca2+的偏好性约为Sr2+的50倍,约为Ba2+的近10000倍。在存在大于10 mM Mg2+的情况下未观察到与囊泡的结合。这种对Ca2+相对于Mg2+的强选择性强化了这样一种观点,即C2结构域将第二信使Ca2+与膜上的信号转导事件联系起来。

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