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硼替佐米介导的长期蛋白酶体抑制对血小板反应性的影响。

Influence of long-term proteasome inhibition on platelet responsiveness mediated by bortezomib.

机构信息

Institute of Transfusion Medicine and Haemotherapy, University of Wuerzburg, Oberduerrbacher Straße 6, D-97080 Wuerzburg, Germany.

出版信息

Vascul Pharmacol. 2021 Jun;138:106830. doi: 10.1016/j.vph.2021.106830. Epub 2021 Jan 8.

DOI:10.1016/j.vph.2021.106830
PMID:33422688
Abstract

INTRODUCTION

Although platelets contain a full proteasome system, its role in platelet function is not completely understood yet. Since the proteasome system may be involved in time-delayed processes, platelet responsiveness was investigated after long-term, bortezomib-mediated proteasome inhibition.

MATERIALS AND METHODS

Citrate-anticoagulated whole blood was stored with 5 nM and 1 μM bortezomib for 24 h. Consecutively, aggregation was measured by light transmission in platelet-rich-plasma (PRP). Flow cytometry was performed to determine phosphorylation levels of the vasodilator-stimulated phosphoprotein (VASP), fibrinogen binding, PAC1-antibody binding and purinergic receptor expression in PRP, P2Y12 activity or glycoprotein (GP) Ib and IIb expression in whole blood. P2Y1 and P2X1 activities were assessed by calcium flux-induced fluorescence in washed platelets. Using PRP, adherent platelets on fibrinogen-, collagen- and ristocetin-coated surfaces were visualized and quantified by immunostaining.

RESULTS

Under bortezomib, VASP phosphorylation was less inducible and nitric oxide-induced inhibition of fibrinogen binding was slightly reduced. Proteasome inhibition did not tamper adenosine diphosphate-mediated aggregation or purinergic receptor expression and activity. Induced expression of activated fibrinogen receptors and fibrinogen binding were not significantly influenced by incubation with bortezomib for 24 h. Aggregation values with threshold agonist concentrations were increased under bortezomib. Despite unchanged GPIb expression, bortezomib-treated platelets showed enhanced adhesion on coated surfaces.

CONCLUSIONS

In platelets incubated for 24 h, bortezomib mediates a slight attenuation of inhibitory signaling, associated with facilitated platelet aggregation using threshold agonist concentrations and enhanced adhesion on agonist-coated surfaces.

摘要

简介

尽管血小板含有完整的蛋白酶体系统,但它在血小板功能中的作用尚未完全了解。由于蛋白酶体系统可能参与延迟时间的过程,因此研究了长期硼替佐米介导的蛋白酶体抑制后血小板的反应性。

材料和方法

用 5 nM 和 1 μM 硼替佐米储存柠檬酸抗凝全血 24 小时。随后,通过富含血小板的血浆(PRP)中的光传输测量聚集。通过流式细胞术测定 PRP 中血管扩张刺激磷蛋白(VASP)的磷酸化水平、纤维蛋白原结合、PAC1 抗体结合和嘌呤能受体表达、全血中的 P2Y12 活性或糖蛋白(GP)Ib 和 IIb 表达。通过在洗涤血小板中钙通量诱导荧光来评估 P2Y1 和 P2X1 活性。使用 PRP,通过免疫染色可视化和量化纤维蛋白原、胶原蛋白和瑞斯托菌素涂层表面上的黏附血小板。

结果

在硼替佐米作用下,VASP 磷酸化的诱导能力降低,一氧化氮诱导的纤维蛋白原结合抑制作用略有减弱。蛋白酶体抑制不会干扰二磷酸腺苷介导的聚集或嘌呤能受体的表达和活性。用硼替佐米孵育 24 小时不会显著影响诱导表达的活化纤维蛋白原受体和纤维蛋白原结合。在硼替佐米作用下,阈值激动剂浓度下的聚集值增加。尽管 GPIb 表达不变,但硼替佐米处理的血小板在涂层表面上表现出增强的黏附。

结论

在孵育 24 小时的血小板中,硼替佐米介导抑制信号的轻微减弱,与使用阈值激动剂浓度增强的血小板聚集和在激动剂涂层表面上增强的黏附相关。

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