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在ADVIA 120血液学系统上使用平均血小板成分来测量血小板活化。

Use of mean platelet component to measure platelet activation on the ADVIA 120 haematology system.

作者信息

Macey M G, Carty E, Webb L, Chapman E S, Zelmanovic D, Okrongly D, Rampton D S, Newland A C

机构信息

Department of Haematology, The Royal London Hospital, London, United Kingdom.

出版信息

Cytometry. 1999 Oct 15;38(5):250-5. doi: 10.1002/(sici)1097-0320(19991015)38:5<250::aid-cyto8>3.3.co;2-b.

Abstract

Platelet activation results in changes in a number of cell surface molecules including an increase in P-Selectin (CD62P) that may be rapidly and conveniently measured by immunofluorescent flow cytometry. The ADVIA 120 (Bayer) is a new system that facilitates more accurate measurement of platelet volume and in addition provides an approximate measure of the mean refractive index (RI) of the platelets reported as mean platelet component (MPC) concentration. We were interested to determine whether changes in MPC might reflect changes in platelet activation status. To investigate this, the platelet CD62P expression, determined by flow cytometry, and change in MPC, measured on the ADVIA 120 system, was first examined in vitro after stimulation of EDTA anticoagulated whole blood with submaximal concentrations of bovine thrombin in the presence or absence of the thromboxane synthase inhibitor, Ridogrel. Thrombin produced a dose-dependent increase in platelet CD62P expression and a decrease in MPC that could be inhibited by Ridogrel at physiological concentrations. In the second set of experiments, blood from 20 normal controls was collected into both EDTA and sodium citrate (SC) anticoagulants. Within 30 min of venesection and again at 3 h post-venesection after storage at room temperature, the platelet MPC and CD62P expression were determined. Platelets in all samples with both anticoagulants showed very low levels of CD62P expression when first analysed. At 3 h there was a small increase in CD62P expression on platelets in whole blood anticoagulated with SC, but a significant (P < 0.001) increase was observed on platelets anti-coagulated with EDTA. A negative correlation was found between the change in MPC of the platelets and the increase in the mean fluorescence intensity (MFI) (r = -0.69, P < 0.001, n = 20) and the percentage (r = -0.72, P < 0.001, n = 20) of CD62P positive platelets at 3 h in blood anticoagulated with EDTA. We conclude that a reduction in MPC as measured by the ADVIA 120 may be used to detect anticoagulant induced, as well as thrombin stimulated, in vitro platelet activation in blood anticoagulated with EDTA. Further, we conclude that platelet activation is negligible for up to 3 h in sodium citrate anticoagulated whole blood.

摘要

血小板活化会导致多种细胞表面分子发生变化,包括P-选择素(CD62P)增加,这可以通过免疫荧光流式细胞术快速方便地进行检测。ADVIA 120(拜耳公司)是一种新系统,它有助于更准确地测量血小板体积,此外还能提供血小板平均折光指数(RI)的近似测量值,以平均血小板成分(MPC)浓度表示。我们感兴趣的是确定MPC的变化是否可能反映血小板活化状态的变化。为了对此进行研究,在用亚最大浓度的牛凝血酶刺激EDTA抗凝全血时,在有或没有血栓素合酶抑制剂利多格雷的情况下,首先在体外检测通过流式细胞术测定的血小板CD62P表达以及在ADVIA 120系统上测量的MPC变化。凝血酶使血小板CD62P表达呈剂量依赖性增加,MPC降低,在生理浓度下利多格雷可抑制这种变化。在第二组实验中,将20名正常对照者的血液分别采集到EDTA和枸橼酸钠(SC)抗凝剂中。在静脉穿刺后30分钟内以及在室温下储存3小时后再次静脉穿刺时,测定血小板MPC和CD62P表达。首次分析时,所有用两种抗凝剂处理的样本中的血小板CD62P表达水平都非常低。3小时时,用SC抗凝的全血中的血小板CD62P表达略有增加,但用EDTA抗凝的血小板上观察到显著增加(P<0.001)。在用EDTA抗凝的血液中,3小时时血小板MPC的变化与平均荧光强度(MFI)的增加(r=-0.69,P<0.001,n=20)以及CD62P阳性血小板的百分比(r=-0.72,P<0.001,n=20)之间发现呈负相关。我们得出结论,通过ADVIA 120测量的MPC降低可用于检测EDTA抗凝血液中抗凝剂诱导的以及凝血酶刺激的体外血小板活化。此外,我们得出结论,在枸橼酸钠抗凝的全血中,长达3小时血小板活化可忽略不计。

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