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凝血酶刺激的血小板对培养的内皮细胞的损伤。

Injury to cultured endothelial cells by thrombin-stimulated platelets.

作者信息

Jørgensen L, Grøthe A G, Larsen T, Kinlough-Rathbone R L, Mustard J F

出版信息

Lab Invest. 1986 Apr;54(4):408-15.

PMID:3959543
Abstract

In vivo, stimulated platelets may injure the endothelium. We have used cultured endothelial cells to assess endothelial cell damage caused by platelet stimulation with thrombin. Endothelial cells were cultured from umbilical veins and semiconfluent cultures were labeled with Na2 51CrO4. Twenty four hours later washed human platelets (final concentration 200,000 platelets/microliters) and thrombin (final concentration 4 units/ml) were added to the medium and the culture dish was shaken for 15 minutes. The percentage of cells detached from the culture dish and the percentage of 51Cr lost from the endothelial cells into the ambient fluid during the shaking were determined and used as indicators of cell injury. Increased percentages of loosened cells and 51Cr in the ambient fluid were observed with platelet suspension and thrombin compared to controls with neither platelet suspension nor thrombin and controls with either platelet suspension or thrombin. The platelet-free supernatant obtained after reaction of the platelets with thrombin also increased the percentage of loosened cells, but it did not increase the percentage of 51Cr in the ambient fluid to a significant degree. Thrombin alone caused a moderate loss of 51Cr, but no increased loosening of cells. Treatment of the platelets with acetylsalicylic acid prior to the experiment depressed the detachment effect of thrombin-stimulated platelets, but did not alter the effect on the release of 51Cr into the ambient fluid. Scanning and transmission electron microscopy of cultured endothelial cells exposed to thrombin-stimulated platelets confirmed the presence of loosening and injury to the endothelial cells. Thus, platelet stimulation with thrombin had at least two effects on the cultured endothelial cells: a loosening effect caused by material released from the platelets; an injury effect which, in order to reach its maximum, required the presence of stimulated platelets.

摘要

在体内,受刺激的血小板可能会损伤内皮细胞。我们利用培养的内皮细胞来评估凝血酶刺激血小板所导致的内皮细胞损伤。内皮细胞取自脐静脉进行培养,亚汇合培养物用Na2 51CrO4进行标记。24小时后,将洗涤过的人血小板(终浓度为200,000个血小板/微升)和凝血酶(终浓度为4单位/毫升)加入培养基中,培养皿振荡15分钟。测定振荡过程中从培养皿上脱离的细胞百分比以及内皮细胞中51Cr释放到周围液体中的百分比,并将其用作细胞损伤的指标。与既无血小板悬液也无凝血酶的对照组以及仅有血小板悬液或仅有凝血酶的对照组相比,血小板悬液和凝血酶组观察到周围液体中松散细胞百分比和51Cr百分比增加。血小板与凝血酶反应后获得的无血小板上清液也增加了松散细胞的百分比,但未使周围液体中51Cr百分比显著增加。单独的凝血酶导致51Cr有适度损失,但细胞未出现明显松散。实验前用乙酰水杨酸处理血小板可抑制凝血酶刺激血小板的脱离作用,但未改变对51Cr释放到周围液体中的影响。对暴露于凝血酶刺激血小板的培养内皮细胞进行扫描和透射电子显微镜检查证实存在内皮细胞松散和损伤。因此,凝血酶刺激血小板对培养的内皮细胞至少有两种作用:一种是由血小板释放的物质引起的松散作用;一种是损伤作用,该作用要达到最大程度需要有受刺激的血小板存在。

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