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人溶酶体磷脂酶 A2 的 N-糖基化在形成具有催化活性的酶中的作用。

Role of N-glycosylation of human lysosomal phospholipase A2 for the formation of catalytically active enzyme.

机构信息

Department of Ophthalmology, School of Medicine, Sapporo Medical University, Sapporo, Japan.

出版信息

J Lipid Res. 2013 Nov;54(11):3098-105. doi: 10.1194/jlr.M041640. Epub 2013 Aug 19.

Abstract

To understand the role of N-glycosylation of lysosomal phospholipase A2 (LPLA2), four potential N-glycosylation sites in human LPLA2 (hLPLA2) were individually modified replacing asparagine (Asn) with alanine by site-direct mutagenesis. COS-7 cells transiently transfected with wild-type (WT) hLPLA2 gene produced catalytically active LPLA2. A single mutation at 273-, 289-, or 398-Asn partially reduced production of active LPLA2. A single mutation at 99-Asn and quadruple mutations at all four Asn sites resulted in a marked reduction of active LPLA2 and loss of active LPLA2, respectively. Western blot analysis using anti-hLPLA2 antibody showed that the LPLA2 expression level was similar between all transfectants. N-glycosidase F digestion revealed that multiple forms of LPLA2 found in individual transfectants are due to different N-glycans linked to the core protein. The LPLA2 activity in individual transfectants was mostly recovered in the soluble fraction and correlated to the quantity of LPLA2 detected in the soluble fraction. LPLA2 mutated at 99-Asn was mostly retained in the membrane fraction. The WT transfectants treated with tunicamycin markedly lost LPLA2 activity. These data indicate that the 99-Asn is the most critical N-glycosylation site for formation of native hLPLA2 in vivo and that the N-glycosylation of LPLA2 is crucial for biosynthesis of catalytically active hLPLA2.

摘要

为了了解溶酶体磷脂酶 A2(LPLA2)的 N-糖基化作用,我们通过定点突变技术将人源 LPLA2(hLPLA2)的 4 个潜在 N-糖基化位点的天冬酰胺(Asn)突变为丙氨酸。用野生型(WT)hLPLA2 基因瞬时转染的 COS-7 细胞产生有催化活性的 LPLA2。单点突变 273-、289-或 398-Asn 会部分降低有活性的 LPLA2 的产生。单点突变 99-Asn 和四点突变所有四个 Asn 位点分别导致有活性的 LPLA2 的产量明显减少和完全丧失。用抗 hLPLA2 抗体的 Western blot 分析表明,所有转染子的 LPLA2 表达水平相似。N-糖苷酶 F 消化表明,单个转染子中发现的多种 LPLA2 形式是由于核心蛋白上连接的不同 N-聚糖。各个转染子的 LPLA2 活性主要在可溶性部分得到恢复,并且与可溶性部分检测到的 LPLA2 数量相关。单点突变 99-Asn 的 LPLA2 主要保留在膜部分。用衣霉素处理的 WT 转染子明显失去了 LPLA2 活性。这些数据表明,99-Asn 是体内形成天然 hLPLA2 的最关键的 N-糖基化位点,并且 LPLA2 的 N-糖基化对于有催化活性的 hLPLA2 的生物合成至关重要。

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本文引用的文献

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Lysosomal phospholipase A2 activity in pig aqueous humor.猪房水液中的溶酶体磷脂酶 A2 活性。
Invest Ophthalmol Vis Sci. 2012 Jan 20;53(1):152-6. doi: 10.1167/iovs.11-7891.
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The measurement of lysosomal phospholipase A2 activity in plasma.血浆中溶酶体磷脂酶 A2 活性的测定。
J Lipid Res. 2010 Aug;51(8):2464-70. doi: 10.1194/jlr.D007146. Epub 2010 Apr 21.
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Lysosomal phospholipase A2 and phospholipidosis.溶酶体磷脂酶A2与磷脂沉积症
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