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应用共聚焦显微镜评估流动状态下血栓中血小板激活状态的新方法。

New approaches for the assessment of platelet activation status in thrombus under flow condition using confocal microscopy.

机构信息

Department of Biopharmacy, Medical University of Bialystok, Mickiewicza 2C, 15-089, Bialystok, Poland.

Department of Physical Chemistry, Medical University of Bialystok, Mickiewicza 2B, 15-089, Bialystok, Poland.

出版信息

Naunyn Schmiedebergs Arch Pharmacol. 2020 Apr;393(4):727-738. doi: 10.1007/s00210-019-01789-x. Epub 2019 Dec 13.

Abstract

The goal of the study was the assessment of heterogeneous platelet activation status in thrombus. In a ferric(III) chloride (FeCl) thrombosis (intravital) model of C57BL/6 J mice, the area of irreversibly activated (phosphatidylserine (PS)-positive) platelets was assessed after 1-s exposure of a vessel to FeCl. In a laser-induced thrombosis (intravital) model of GFP mice, the area of the thrombus composed of PS-negative platelets was evaluated. The ratio of the area of PECAM-1 to the area of the thrombus was used as a marker to assess the activity of PS-negative platelets. In the in vitro flow chamber model, the thrombus area (PS-negative and PS-positive platelets) and the platelet activation index (ratio of the area of PS-positive platelets to the area of thrombus) were determined. To assess platelet activation status with these models, acetylsalicylic acid (ASA) and iloprost (Ilo) were used. In the FeCl thrombosis, ASA (10 mg/kg, 100 mg/kg) decreased the area of PS-positive platelets. In the laser thrombosis, ASA (10 mg/kg) decreased the thrombus area, but the decrease in platelet activity was evident even at 3 mg/kg by an increased PECAM-1/thrombus ratio. In the flow chamber, ASA (0.02 mg/ml, 0.2 mg/ml) equally decreased the platelet activation index, whereas only at 0.2 mg/ml, it decreased the thrombus area. Ilo (3.6 ng/ml, 36 ng/ml) decreased the thrombus area but at 36 ng/ml increased the platelet activation index. We showed that intravital models and flow chamber provide a detailed assessment of platelet activation status and the mechanism of drug action.

摘要

研究目的是评估血栓中血小板的异质性激活状态。在 C57BL/6J 小鼠的三氯化铁(FeCl)血栓(活体)模型中,通过将血管暴露于 FeCl 1 秒来评估不可逆激活(血小板磷脂酰丝氨酸(PS)阳性)血小板的区域。在 GFP 小鼠的激光诱导血栓(活体)模型中,评估了由 PS 阴性血小板组成的血栓区域。PECAM-1 区域与血栓区域的比值用作评估 PS 阴性血小板活性的标志物。在体外流动室模型中,确定了血栓区域(PS 阴性和 PS 阳性血小板)和血小板激活指数(PS 阳性血小板区域与血栓区域的比值)。为了使用这些模型评估血小板激活状态,使用了乙酰水杨酸(ASA)和伊洛前列素(Ilo)。在 FeCl 血栓中,ASA(10mg/kg,100mg/kg)减少了 PS 阳性血小板的区域。在激光血栓中,ASA(10mg/kg)减少了血栓区域,但通过增加 PECAM-1/血栓比值,即使在 3mg/kg 时,血小板活性的降低也很明显。在流动室中,ASA(0.02mg/ml,0.2mg/ml)同样降低了血小板激活指数,而仅在 0.2mg/ml 时,它降低了血栓区域。Ilo(3.6ng/ml,36ng/ml)减少了血栓区域,但在 36ng/ml 时增加了血小板激活指数。我们表明,活体模型和流动室提供了对血小板激活状态和药物作用机制的详细评估。

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