血栓素合成酶抑制对大鼠同种异体肾移植再灌注损伤及内皮素-1,2水平的影响。

O Büyükgebiz, A O Aktan, G Haklar, S Bilsel, M Dülger
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引用次数: 8

摘要

血栓素A2是一种促聚集性血管收缩剂,在再灌注损伤时合成并释放。本研究旨在探讨血栓素合成酶抑制剂UK 38485对肾移植早期肾内皮内皮素-1,2 (ET)反应及脂质过氧化和蛋白氧化的影响。四组大鼠(IV组n=8,其他组n=10)[校正]分别为I组(假肾切除)、II组(自体移植)、III组(同种异体移植)和IV组(同种异体移植组,同种异体移植物灌注UK 38485)。所有受试者在肾移植后均行右肾切除术。移植物用4ml冰冷的乳酸林格氏液冲洗,在IV组中,每个肾脏加入10微克UK 38485。在同种异体移植组中,肾脏取自同种异体白色Wistar白化大鼠。肾移植体在冷缺血期40 min后再灌注120 min。分析肾静脉血ET-1、2血浆浓度及脂质过氧化产物二烯偶联物(DC)、羟醛(HAA)、羟醛(HAE)和丙二醛(MDA)水平,以及作为蛋白质氧化指标的蛋白质羰基和蛋白质巯基。ⅱ组和ⅲ组血浆ET-1、2浓度显著升高(P
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The effects of thromboxane synthase inhibition on reperfusion injury and endothelin-1,2 levels in allograft kidney transplantation in rats.

Thromboxane A2 is a proaggregative vasoconstrictor that is synthesized and released in reperfusion injury. We aimed to investigate the effects of thromboxane synthase inhibitor, UK 38485, on endothelin-1,2 (ET) response of the renal endothelium and lipid peroxidation and protein oxidation in the early period of kidney transplantation. Four groups (n=8 in group IV and n=10 in the others) [corrected] of Sprague-Dawley rats were designed as Group I (sham nephrectomy), Group II (autotransplantation), Group III (allotransplantation) and Group IV (allotransplantation group in which the allografts were perfused with UK 38485. All subjects underwent right nephrectomy after transplantation. The grafts were flushed with 4 ml of ice-cold Ringer's lactate and in Group IV 10 microg of UK 38485 was added into the solution for each kidney. In allotransplantation groups, the kidneys were harvested from allogeneic white Wistar albino rats. The kidney grafts were allowed 120 min of reperfusion after 40 min of cold ischemic period. ET-1,2 plasma concentrations in the renal vein blood and diene conjugates (DC), hydroxyalkanals (HAA), hydroxyalkenals (HAE) and malondialdehyde (MDA) levels as the products of lipid peroxidation, protein carbonyls and protein sulfhydryls as the indicators of protein oxidation were analyzed in kidney tissue. Plasma ET-1,2 concentrations increased significantly in Group II and Group III (P<0.01) when compared to Group I but decreased in Group IV in comparison with Group III (P<0.05). DC, HAA, HAE and MDA levels increased in Groups II and III (P<0.001). Significant protein oxidation occurred only in Group III (P<0.01). Perfusion of the allografts with UK 38485 prevented lipid peroxidation and protein oxidation in Group IV. Histopathological changes were mild in the last group. We concluded that, in kidney transplantation, local administration of UK 38485 has cytopreservative effects on the allografts and this effect can be related to ET-1,2 concentrations.

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