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磷脂酶A2激活及随后在公羊精子钙离子/离子载体诱导的顶体反应中的胞吐作用。

Phospholipase A2 activation and subsequent exocytosis in the Ca2+/ionophore-induced acrosome reaction of ram spermatozoa.

作者信息

Roldan E R, Fragio C

机构信息

Department of Development and Signalling, AFRC Babraham Institute, Cambridge, United Kingdom.

出版信息

J Biol Chem. 1993 Jul 5;268(19):13962-70.

PMID:8314762
Abstract

In ram spermatozoa treatment with Ca2+ and A23187 or ionomycin stimulated the release of arachidonic acid (20:4) and exocytosis of the acrosome in a time- and concentration-dependent manner. Diacylglycerol did not appear to be the source of 20:4. On the other hand, generation of 20:4 was significantly correlated with breakdown of phosphatidylcholine, phosphatidylserine, and phosphatidylethanolamine under a variety of conditions, thus indicating that 20:4 release was due to phospholipase A2 activity. Generation of 20:4 preceded acrosomal exocytosis. Moreover, it was significantly correlated with exocytosis when spermatozoa were stimulated with Ca2+ and A23187 or ionomycin for different periods of time or with different ionophore concentrations. Treatment with Ro 31-4493, a compound that has been found to inhibit sperm phospholipase A2 activity in vitro, considerably reduced both the release of 20:4 and exocytosis; addition of exogenous 20:4 or lysophosphatidylcholine overcame the inhibitory effect of Ro 31-4493. Spermatozoa preincubated with several unsaturated fatty acids, including 20:4, underwent exocytosis much more rapidly when treated with Ca2+/A23187. Exogenous lysophosphatidylcholine also enhanced acrosomal exocytosis and this effect was mimicked by an alkyl-containing analogue (1-O-alkyl-glycerophosphorylcholine = lyso-platelet activating factor). These results indicate that phospholipase A2 plays a fundamental role in the exocytosis of the acrosome elicited by Ca2+ and ionophore stimulation. Therefore, it is possible that activation of this enzyme constitutes an essential Ca2+-dependent event underlying exocytosis in response to physiological stimuli.

摘要

在公羊精子中,用Ca2+和A23187或离子霉素处理能以时间和浓度依赖的方式刺激花生四烯酸(20:4)的释放及顶体的胞吐作用。二酰基甘油似乎不是20:4的来源。另一方面,在多种条件下,20:4的生成与磷脂酰胆碱、磷脂酰丝氨酸和磷脂酰乙醇胺的分解显著相关,因此表明20:4的释放是由于磷脂酶A2的活性。20:4的生成先于顶体胞吐作用。此外,当精子用Ca2+和A23187或离子霉素刺激不同时间或不同离子载体浓度时,它与胞吐作用显著相关。用Ro 31 - 4493处理,一种已发现能在体外抑制精子磷脂酶A2活性的化合物,能显著降低20:4的释放和胞吐作用;添加外源性20:4或溶血磷脂酰胆碱可克服Ro 31 - 4493的抑制作用。用包括20:4在内的几种不饱和脂肪酸预孵育的精子,在用Ca2+/A23187处理时顶体胞吐作用发生得更快。外源性溶血磷脂酰胆碱也增强了顶体胞吐作用,这种作用被一种含烷基的类似物(1 - O - 烷基 - 甘油磷酸胆碱 = 溶血血小板活化因子)模拟。这些结果表明磷脂酶A2在由Ca2+和离子载体刺激引发的顶体胞吐作用中起基本作用。因此,这种酶的激活可能构成了响应生理刺激时胞吐作用所依赖的基本Ca2+依赖性事件。

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