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内毒素处理的兔子中内皮组织因子增强但血栓调节蛋白正常。

Enhanced endothelial tissue factor but normal thrombomodulin in endotoxin-treated rabbits.

作者信息

Semeraro N, Triggiani R, Montemurro P, Cavallo L G, Colucci M

机构信息

Dipartimento di Scienze Biomediche e Oncologia Umana, Università di Bari, Italy.

出版信息

Thromb Res. 1993 Sep 15;71(6):479-86. doi: 10.1016/0049-3848(93)90121-4.

DOI:10.1016/0049-3848(93)90121-4
PMID:8134907
Abstract

Exposure of cultured endothelial cells to bacterial endotoxin induces an enhancement of cell procoagulant activity (PCA) and a simultaneous reduction of thrombomodulin activity (TM). We evaluated the effect of endotoxin on the expression of both endothelial PCA and TM in vivo, in rabbits. Animals were given a single i.v. injection of endotoxin (E. coli 0111:B4 LPS, W, 10-200 micrograms/kg); the thoracic aorta was harvested after 2 or 4 hours and placed in an ad hoc device to expose the endothelial surface only. Endotoxin treatment resulted in a dose-dependent increase of endothelial PCA (p < 0.001, at 100 micrograms/kg or more), which was totally dependent on factor VII and thus identified as tissue factor. In contrast, endothelial TM activity, as measured by the rate of thrombin-induced protein C activation, was similar in control and endotoxemic rabbits, even when the animals were given two injections (50 micrograms/kg, 24 h apart), or a continuous infusion (40 micrograms/kg/h during 4 hours) of endotoxin. To explore the effect of endotoxin on TM activity at the microcirculation level, we measured the extent of protein C activation in vivo, induced by a continuous infusion of low doses of thrombin (1 NIH U/kg/min for 60 min). Again, endotoxin administration was not associated with significant changes in TM-dependent protein C activation, as assessed by the anticoagulant activity present in a barium citrate plasma eluate obtained at the end of thrombin infusion. Although reduction of TM during persistent endotoxemia cannot be definitively excluded, our data support a major role of endothelial PCA in LPS-induced coagulative changes.

摘要

将培养的内皮细胞暴露于细菌内毒素会导致细胞促凝活性(PCA)增强,同时血栓调节蛋白活性(TM)降低。我们评估了内毒素对家兔体内内皮PCA和TM表达的影响。给动物静脉内单次注射内毒素(大肠杆菌0111:B4 LPS,W,10 - 200微克/千克);2或4小时后采集胸主动脉,置于专用装置中仅暴露内皮表面。内毒素处理导致内皮PCA呈剂量依赖性增加(在100微克/千克或更高剂量时,p < 0.001),这完全依赖于因子VII,因此被确定为组织因子。相比之下,通过凝血酶诱导的蛋白C活化速率测量的内皮TM活性,在对照兔和内毒素血症兔中相似,即使动物接受两次注射(50微克/千克,间隔24小时)或连续输注(4小时内40微克/千克/小时)内毒素。为了探究内毒素在微循环水平对TM活性的影响,我们测量了连续输注低剂量凝血酶(1 NIH单位/千克/分钟,持续60分钟)在体内诱导的蛋白C活化程度。同样,如通过凝血酶输注结束时获得的柠檬酸钡血浆洗脱液中存在的抗凝活性评估,内毒素给药与TM依赖性蛋白C活化的显著变化无关。尽管不能完全排除持续性内毒素血症期间TM的降低,但我们的数据支持内皮PCA在LPS诱导的凝血变化中起主要作用。

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