磷脂酶A2参与庆大霉素诱导的大鼠系膜细胞活化。
Involvement of phospholipase A2 in gentamicin-induced rat mesangial cell activation.
作者信息
Martínez-Salgado C, Rodríguez-Barbero A, Rodríguez-Puyol D, Pérez de Lema G, López-Novoa J M
机构信息
Departamento de Fisiología y Farmacología, Universidad de Salamanca, Spain.
出版信息
Am J Physiol. 1997 Jul;273(1 Pt 2):F60-6. doi: 10.1152/ajprenal.1997.273.1.F60.
The role of the phospholipase A2 (PLA2) activation in the gentamicin (Gent)-induced rat mesangial cell activation has been studied. Gent (10(-5) M) induced a time-dependent mesangial planar cell surface area reduction that was significantly inhibited by the PLA2 inhibitors aristolochic acid (AA) and quinacrine, by the platelet-activating factor (PAF) blocker BN-52021 (BN), and by verapamil. These substances also inhibited Gent-induced [3H]thymidine incorporation into DNA (AA, 504 +/- 20; quinacrine, 555 +/- 66; BN, 1,126 +/- 120; and verapamil, 896 +/- 109; vs. 1,818 +/- 35 cpm/well in cells treated with Gent alone) and the Gent-induced increase in cell number (AA, 20,116 +/- 2,696; quinacrine, 24,687 +/- 1,481; BN, 26,122 +/- 1,016; and verapamil, 27,566 +/- 1,214; vs. 47,486 +/- 1,124 cells/well in cells treated with Gent alone). Gent induced a twofold increase in [3H]acetate incorporation into PAF (27 +/- 3 vs. 12 +/- 2 cpm/microgram protein in control conditions) that was completely blocked by AA, BN, or verapamil. Gent increased thromboxane B2 and prostaglandin E2 (PGE2) production, with both increases inhibited by either AA or verapamil. BN only inhibited the Gent-induced mesangial PGE2 production. In addition, Gent increased PLA2 activity (measured as [3H]arachiodonic acid release, 29,849 +/- 2,151 vs. 20,104 +/- 2,308 cpm/well in basal conditions), an effect that was blocked by AA (11,804 +/- 684 cpm/well). These data suggest a major role for PLA2 activation in Gent-induced mesangial cell contraction, proliferation and prostanoid secretion.
已经研究了磷脂酶A2(PLA2)激活在庆大霉素(Gent)诱导的大鼠系膜细胞激活中的作用。庆大霉素(10^(-5) M)诱导系膜平面细胞表面积呈时间依赖性减少,该作用被PLA2抑制剂马兜铃酸(AA)和奎纳克林、血小板活化因子(PAF)阻滞剂BN - 52021(BN)以及维拉帕米显著抑制。这些物质还抑制庆大霉素诱导的[3H]胸苷掺入DNA(AA为504±20;奎纳克林为555±66;BN为1126±120;维拉帕米为896±109;而单独用庆大霉素处理的细胞中为1818±35 cpm/孔)以及庆大霉素诱导的细胞数量增加(AA为20116±2696;奎纳克林为24687±1481;BN为26122±1016;维拉帕米为27566±1214;而单独用庆大霉素处理的细胞中为47486±1124个细胞/孔)。庆大霉素诱导[3H]乙酸掺入PAF增加两倍(对照条件下为27±3 vs. 12±2 cpm/μg蛋白质),该增加被AA、BN或维拉帕米完全阻断。庆大霉素增加血栓素B2和前列腺素E2(PGE2)的产生,这两种增加均被AA或维拉帕米抑制。BN仅抑制庆大霉素诱导的系膜PGE2产生。此外,庆大霉素增加PLA2活性(以[3H]花生四烯酸释放量衡量,基础条件下为29849±2151 vs. 20104±2308 cpm/孔),该作用被AA(11804±684 cpm/孔)阻断。这些数据表明PLA2激活在庆大霉素诱导的系膜细胞收缩、增殖和类前列腺素分泌中起主要作用。
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