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柠檬酸盐磷酸盐葡萄糖改变了体外凝血动力学。

Citrate Phosphate Dextrose Alters Coagulation Dynamics Ex Vivo.

机构信息

Department of Surgery, Center for Translational Injury Research, McGovern Medical School at The University of Texas Health Science Center at Houston, Houston, Texas.

McGovern Medical School at UTHealth, Houston, Texas.

出版信息

J Surg Res. 2023 Nov;291:43-50. doi: 10.1016/j.jss.2023.05.026. Epub 2023 Jun 16.

Abstract

INTRODUCTION

Citrate-phosphate-dextrose (CPD) is the most common anticoagulant for blood product storage in the United States. It was developed to prolong shelf life, though there is little research regarding its impact on function following transfusion. We used flow cytometry (FC), thromboelastography (TEG), and a clot contraction assay called the zFlex platform to measure platelet activation and global clot formation in blood samples anticoagulated with either CPD or in a standard blue top citrate (BTC) tube.

METHODS

Samples were obtained through venipuncture of the antecubital fossa from healthy donors who had not recently taken antiplatelet medication. Samples for FC analysis were spun to obtain platelet-rich plasma, while TEG and zFlex utilized recalcified whole blood.

RESULTS

Mean fluorescence intensity for CD62p (P-selectin, marker of platelet activation) in baseline samples was equal, while mean fluorescence intensity in samples activated with thrombin receptor activating peptide was higher in CPD than BTC (65,814 ± 4445 versus 52,483 ± 5435, P = 0.007). TEG results demonstrated similar maximum amplitude for CPD (62.7 ± 1.8 mm versus 61 ± 1 mm) (P = 0.33), though reaction time and kinetics time were significantly longer in CPD versus BTC. CPD R-time: 7.9 ± 0.4 min versus BTC: 3.8 ± 0.4 (P < 0.001). CPD K-time: 2.2 ± 0.2 min versus BTC: 1.6 ± 0.1 min (P < 0.001). Clot contraction strength was not different between the two groups on zFlex: CPD 4353 ± 6 = 517 μN versus BTC 4901 ± 390 μN (P = 0.39).

CONCLUSIONS

Our findings suggest that CPD does not affect platelet function (minimal difference on FC and no difference in ultimate clot strength, which is ∼80% due to platelet function) but may alter clot dynamics by attenuating thrombin generation.

摘要

简介

柠檬酸盐-磷酸盐-葡萄糖(CPD)是美国最常用的血液制品储存抗凝剂。它的开发目的是延长保质期,但关于输血后对其功能的影响的研究很少。我们使用流式细胞术(FC)、血栓弹力图(TEG)和一种称为 zFlex 平台的凝块收缩测定法来测量用 CPD 或标准蓝帽柠檬酸盐(BTC)管抗凝的血液样本中的血小板活化和整体凝块形成。

方法

通过肘前窝的静脉穿刺从未近期服用抗血小板药物的健康供者中获得样本。用于 FC 分析的样本离心以获得富含血小板的血浆,而 TEG 和 zFlex 使用再钙化的全血。

结果

基础样本中 CD62p(血小板活化标志物 P-选择素)的平均荧光强度相等,而用凝血酶受体激活肽激活后的样本中 CPD 比 BTC 的平均荧光强度更高(65814±4445 对 52483±5435,P=0.007)。TEG 结果表明 CPD 的最大振幅相似(62.7±1.8mm 对 61±1mm)(P=0.33),尽管 CPD 的反应时间和动力学时间明显长于 BTC。CPD R-时间:7.9±0.4min 对 BTC:3.8±0.4min(P<0.001)。CPD K-时间:2.2±0.2min 对 BTC:1.6±0.1min(P<0.001)。在 zFlex 上,两组之间的凝块收缩强度没有差异:CPD 4353±6=517μN 对 BTC 4901±390μN(P=0.39)。

结论

我们的发现表明 CPD 不会影响血小板功能(FC 上差异极小,最终凝块强度无差异,这大约 80%归因于血小板功能),但可能通过抑制凝血酶生成来改变凝块动力学。

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