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血栓弹力图法量化因子 XIII 对凝血动力学的贡献。

Thrombelastographic method to quantify the contribution of factor XIII to coagulation kinetics.

作者信息

Nielsen Vance G, Kirklin James K, Hoogendoorn Hugh, Ellis Truitt C, Holman William L

机构信息

Department of Anesthesiology, The University of Alabama at Birmingham, Birmingham, Alabama 35249, USA.

出版信息

Blood Coagul Fibrinolysis. 2007 Mar;18(2):145-50. doi: 10.1097/MBC.0b013e32802f7d91.

Abstract

Factor XIII (FXIII) plays a critical role in clot strength, and FXIII deficiency or excess is associated with hemorrhage or thrombosis, respectively. Our goal was to design a thrombelastography-based method to characterize the effects of FXIII on plasma clot strength. Normal human plasma was exposed to 0 or 200 mug/ml anti-FXIII antibodies for 20 min prior to celite activation and calcium addition. Other plasma had addition of fibrinogen (625 mg/dl)/FXIII (2 U/ml) or 30% dilution with hydroxyethyl starch before exposure to 0 or 200 mug/ml anti-FXIII antibodies. Thromboelastography was performed and data were collected until stable clot strength was observed. The exposure of normal plasma to anti-FXIII antibodies resulted in a significant (P < 0.05) decrease in clot strength (63%) compared with plasma without antibodies. Further samples exposed to anti-FXIII antibodies had clot strength no different from FXIII-deficient plasma. The FXIII-mediated clot strength varied between 44 and 50% in hypercoagulable and hypocoagulable plasma, respectively. In conclusion, the present investigation successfully demonstrated a novel method to detect the impact of FXIII activity in plasma samples. Further actuarial investigation will be required to determine the utility of this approach in the diagnosis and treatment of patients with either acquired FXIII deficiency or excess and concordant coagulopathy.

摘要

凝血因子 XIII(FXIII)在血凝块强度方面起着关键作用,FXIII 缺乏或过量分别与出血或血栓形成相关。我们的目标是设计一种基于血栓弹力图的方法来表征 FXIII 对血浆凝块强度的影响。在硅藻土激活和添加钙之前,将正常人血浆暴露于 0 或 200 μg/ml 的抗 FXIII 抗体中 20 分钟。其他血浆在暴露于 0 或 200 μg/ml 的抗 FXIII 抗体之前添加了纤维蛋白原(625 mg/dl)/FXIII(2 U/ml)或用羟乙基淀粉进行 30%稀释。进行血栓弹力图检查并收集数据,直至观察到稳定的凝块强度。与未接触抗体的血浆相比,正常血浆暴露于抗 FXIII 抗体导致凝块强度显著降低(P < 0.05)(63%)。进一步接触抗 FXIII 抗体的样本的凝块强度与 FXIII 缺乏的血浆无差异。在高凝和低凝血浆中,FXIII 介导的凝块强度分别在 44%至 50%之间变化。总之,本研究成功展示了一种检测血浆样本中 FXIII 活性影响的新方法。需要进一步的 actuarial 研究来确定这种方法在诊断和治疗获得性 FXIII 缺乏或过量及相应凝血病患者中的效用。 (注:“actuarial”在医学语境中可能有误用,一般该词多用于精算领域,这里可能影响对整体内容理解,但按要求不做修改。)

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