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前列环素受体刺激有助于检测 PFA-100 系统对人血小板 P2Y(12)受体的抑制作用。

Prostacyclin receptor stimulation facilitates detection of human platelet P2Y(12) receptor inhibition by the PFA-100 system.

机构信息

Institute of Clinical Biochemistry and Pathobiochemistry-Central Laboratory, University Clinic Wuerzburg, Wuerzburg, Germany.

出版信息

Platelets. 2010;21(2):112-6. doi: 10.3109/09537100903440937.


DOI:10.3109/09537100903440937
PMID:20085435
Abstract

The rationale for monitoring platelet inhibition by thienopyridines for the identification of patients at risk for future recurrent arterial thrombosis or ischemic events is intensively discussed, as well as which monitoring systems are appropriate, robust and reliable. Flow cytometric measurement of phosphorylated VASP (vasodilator-stimulated phosphoprotein), expressed as platelet reactivity index (PRI), is presently "the gold standard method" for evaluating P2Y(12) receptor inhibition. The PFA-100 system, a commercially available and clinically widely used platelet test system, is based on a different principle, not that of VASP phosphorylation. The aim of the present study was to compare the two methods and evaluate whether the conventional PFA-100 collagen/ADP cartridge could be pharmacologically improved to enable its routine clinical use for detection of platelet P2Y(12) receptor inhibition. The effects of increasing concentrations of the competitive P2Y(12) receptor antagonist cangrelor (AR-C69931MX) and the time-dependent effects of a single oral loading dose of clopidogrel (600 mg) were analysed with human whole blood. P2Y(12) receptor inhibition was measured by the VASP/PRI assay and the PFA-100 collagen/ADP cartridge system, with and without preincubation with the prostacyclin analog iloprost (Ilomedin). In vitro addition of iloprost (0.5 nM) enabled PFA-100 collagen/ADP cartridge system detection of P2Y(12) receptor inhibition in whole blood by cangrelor in vitro or by clopidogrel treatment of volunteers. The addition of a prostacyclin analog facilitates PFA-100 collagen/ADP system detection of P2Y(12) receptor inhibition, achieving a sensitivity similar to that of the VASP/PRI reference method. Future studies should now evaluate whether this modified PFA-100 system, like the VASP assay, is a reliable test system for monitoring P2Y(12) receptor inhibition under clinical conditions.

摘要

正在深入讨论监测噻吩吡啶类药物抑制血小板以确定未来复发性动脉血栓形成或缺血事件风险患者的基本原理,以及哪些监测系统是合适、稳健和可靠的。流式细胞术测量磷酸化 VASP(血管扩张刺激磷蛋白),表示为血小板反应指数(PRI),目前是评估 P2Y(12)受体抑制的“金标准方法”。PFA-100 系统是一种商业上可用且临床上广泛使用的血小板测试系统,其基于不同的原理,而不是 VASP 磷酸化。本研究的目的是比较两种方法,并评估常规 PFA-100 胶原/ADP 筒是否可以通过药理学改善以使其常规用于检测血小板 P2Y(12)受体抑制。分析了增加浓度的竞争性 P2Y(12)受体拮抗剂坎格雷洛(AR-C69931MX)和单次口服负荷剂量氯吡格雷(600mg)的时间依赖性效应,方法是使用人全血。通过 VASP/PRI 测定和 PFA-100 胶原/ADP 筒系统分析 P2Y(12)受体抑制,不进行预处理和预处理前列腺素类似物依洛前列素(Ilomedin)。体外添加依洛前列素(0.5nM)使 PFA-100 胶原/ADP 筒系统能够检测全血中的坎格雷洛或志愿者氯吡格雷治疗的 P2Y(12)受体抑制。添加前列腺素类似物可促进 PFA-100 胶原/ADP 系统检测 P2Y(12)受体抑制,达到与 VASP/PRI 参考方法相似的灵敏度。未来的研究现在应该评估这种改良的 PFA-100 系统是否像 VASP 测定一样,是监测临床条件下 P2Y(12)受体抑制的可靠测试系统。

相似文献

[1]
Prostacyclin receptor stimulation facilitates detection of human platelet P2Y(12) receptor inhibition by the PFA-100 system.

Platelets. 2010

[2]
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[3]
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[4]
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[5]
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[6]
Comparison of a new ELISA assay with the flow cytometric assay for platelet vasodilator-associated stimulated phosphoprotein (VASP) phosphorylation in whole blood to assess P2Y(12) inhibition.

Thromb Haemost. 2011-12-21

[7]
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[8]
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[9]
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[10]
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Thromb Haemost. 2010-10-12

引用本文的文献

[1]
Prostanoid Signaling in Cancers: Expression and Regulation Patterns of Enzymes and Receptors.

Biology (Basel). 2022-4-13

[2]
The role of adenosine diphosphate mediated platelet responsiveness for the stability of platelet integrity in citrated whole blood under ex vivo conditions.

PLoS One. 2017-11-20

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