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血小板活化因子乙酰水解酶可使脂磷壁酸单脱酰基并使其失活。

Platelet-activating factor-acetylhydrolase can monodeacylate and inactivate lipoteichoic acid.

作者信息

Seo Ho Seong, Kim Je Hak, Nahm Moon H

机构信息

Department of Pathology, University of Alabama at Birmingham, 845 19th St. South (BBRB 614), Birmingham, AL 35249-7331, USA.

出版信息

Clin Vaccine Immunol. 2006 Apr;13(4):452-8. doi: 10.1128/CVI.13.4.452-458.2006.

Abstract

Bacterial lipoteichoic acid (LTA) shares a structural motif with platelet-activating factor (PAF). Both molecules are strong inflammatory agents and have a glycerol backbone with two lipid chains at the sn-1 and sn-2 positions. PAF is normally inactivated by PAF-acetylhydrolase (PAF-AH), a phospholipase A2 (PLA2), which removes a short acyl group at the sn-2 position. To investigate whether PAF-AH can similarly degrade LTA, we studied the effects of porcine PLA2, bee venom PLA2, and recombinant human PAF-AH on pneumococcal LTA (PnLTA) and staphylococcal LTA (StLTA). After incubation with a porcine or bee venom PLA2, a large fraction of PnLTA lost 264 Da, which corresponds to the mass of the oleic acid group at the sn-2 position. After incubation with recombinant human PAF-AH, PnLTA lost 264 Da; the reduction did not occur when PAF-AH was exposed to Pefabloc SC, an irreversible inhibitor of the PAF-AH active site. Following PAF-AH treatment, PnLTA and StLTA were not able to stimulate mouse RAW 264.7 cells to produce tumor necrosis factor alpha but could stimulate CHO cells expressing human TLR2. This stimulation pattern has been observed with monoacyl PnLTA prepared by mild alkali hydrolysis (22). Taking these data together, we conclude that PAF-AH can remove one acyl chain at the sn-2 position of LTA and produce a monoacyl-LTA that is inactive against mouse cells.

摘要

细菌脂磷壁酸(LTA)与血小板活化因子(PAF)具有相同的结构基序。这两种分子都是强效炎症介质,并且都有一个甘油主链,在sn-1和sn-2位置带有两条脂链。PAF通常由PAF-乙酰水解酶(PAF-AH,一种磷脂酶A2,即PLA2)使其失活,该酶会去除sn-2位置的一个短酰基。为了研究PAF-AH是否能以类似方式降解LTA,我们研究了猪PLA2、蜂毒PLA2和重组人PAF-AH对肺炎球菌LTA(PnLTA)和葡萄球菌LTA(StLTA)的作用。用猪或蜂毒PLA2孵育后,大部分PnLTA损失了264 Da,这相当于sn-2位置油酸基团的质量。用重组人PAF-AH孵育后,PnLTA损失了264 Da;当PAF-AH暴露于PAF-AH活性位点的不可逆抑制剂Pefabloc SC时,这种减少并未发生。经PAF-AH处理后,PnLTA和StLTA无法刺激小鼠RAW 264.7细胞产生肿瘤坏死因子α,但能刺激表达人TLR2的CHO细胞。用温和碱水解制备的单酰基PnLTA也观察到了这种刺激模式(22)。综合这些数据,我们得出结论,PAF-AH可以去除LTA的sn-2位置的一条酰基链,并产生对小鼠细胞无活性的单酰基-LTA。

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