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外源性添加溶血磷脂酰胆碱至 NRK52E 细胞后,溶血磷脂酶 D 胞外和胞内产生溶血磷脂酸和环磷酸脂酸。

Extracellular and intracellular productions of lysophosphatidic acids and cyclic phosphatidic acids by lysophospholipase D from exogenously added lysophosphatidylcholines to cultured NRK52E cells.

机构信息

Pharmaceutics, Graduate School of Clinical Pharmacy, Kyushu University of Health and Welfare, 1714-1 Yoshino-machi, Nobeoka, Miyazaki 882-8508, Japan.

Faculty of Pharmacy, Yasuda Women's University, Hiroshima, Japan.

出版信息

Biochim Biophys Acta Mol Cell Biol Lipids. 2023 Sep;1868(9):159349. doi: 10.1016/j.bbalip.2023.159349. Epub 2023 Jun 7.

DOI:10.1016/j.bbalip.2023.159349
PMID:37295607
Abstract

Lysophosphatidic acid (LPA) is a bioactive lysophospholipid that is a notable biomarker of kidney injury. However, it is not clear how LPA is produced in renal cells. In this study, we explored LPA generation and its enzymatic pathway in a rat kidney-derived cell, NRK52E cells. Culturing of NRK52E cells with acyl lysophosphatidylcholine (acyl LPC), or lyso-platelet activating factor (lysoPAF, alkyl LPC) was resulted in increased extracellular level of choline, co-product with LPA by lysophospholipase D (lysoPLD). Their activities were enhanced by addition of calcium ions to the cell culture medium, but failed to be inhibited by S32826, an autotaxin (ATX)-specific inhibitor. Liquid chromatography-tandem mass spectrometric analysis revealed the small, but significant extracellular production of acyl LPA/cyclic phosphatidic acid (cPA) and alkyl LPA/cPA. The mRNA expression of glycerophosphodiesterase (GDE) 7 with lysoPLD activity was elevated in confluent NRK52E cells cultured over 3 days. GDE7 plasmid-transfection of NRK52E cells augmented both extracellular and intracellular productions of LPAs (acyl and alkyl) as well as extracellular productions of cPAs (acyl and alkyl) from exogenous LPCs (acyl and alkyl). These results suggest that intact NRK52E cells are able to produce choline and LPA/cPA from exogenous LPCs through the enzymatic action of GDE7 that is located on the plasma membranes and intracellular membranes.

摘要

溶血磷脂酸(LPA)是一种生物活性溶血磷脂,是肾脏损伤的显著生物标志物。然而,目前尚不清楚 LPA 在肾细胞中是如何产生的。在这项研究中,我们探索了 LPA 在大鼠肾源细胞 NRK52E 细胞中的产生及其酶途径。NRK52E 细胞与酰基溶血磷脂酰胆碱(酰基 LPC)或溶血小板激活因子(lysoPAF,烷基 LPC)孵育,导致细胞外胆碱水平升高,LPA 的副产物,由溶血磷脂酶 D(lysoPLD)产生。钙离子的加入增强了它们的活性,但不能被 S32826 抑制,S32826 是一种特定的自分泌酶(ATX)抑制剂。液相色谱-串联质谱分析显示,酰基 LPA/环磷酸(cPA)和烷基 LPA/cPA 有少量但显著的细胞外产生。在培养超过 3 天的汇合 NRK52E 细胞中,具有溶血磷脂酶 D 活性的甘油磷酸二酯酶(GDE)7 的 mRNA 表达升高。NRK52E 细胞的 GDE7 质粒转染增强了细胞外和细胞内 LPAs(酰基和烷基)以及细胞外 cPAs(酰基和烷基)的产生,来自外源性 LPCs(酰基和烷基)。这些结果表明,完整的 NRK52E 细胞能够通过位于质膜和细胞内膜上的 GDE7 的酶促作用,从外源性 LPC 产生胆碱和 LPA/cPA。

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