Protein disulfide isomerase cleaves allosteric disulfides in histidine-rich glycoprotein to regulate thrombosis

Author:

Lv Keyu,Chen Shuai,Xu XulinORCID,Chiu JoyceORCID,Wang Haoqing J.,Han YunyunORCID,Yang Xiaodan,Bowley Sheryl R.,Wang Hao,Tang Zhaoming,Tang Ning,Yang Aizhen,Yang Shuofei,Wang Jinyu,Jin Si,Wu Yi,Schmaier Alvin H.,Ju Lining A.ORCID,Hogg Philip J.ORCID,Fang ChaoORCID

Abstract

AbstractThe essence of difference between hemostasis and thrombosis is that the clotting reaction is a highly fine-tuned process. Vascular protein disulfide isomerase (PDI) represents a critical mechanism regulating the functions of hemostatic proteins. Herein we show that histidine-rich glycoprotein (HRG) is a substrate of PDI. Reduction of HRG by PDI enhances the procoagulant and anticoagulant activities of HRG by neutralization of endothelial heparan sulfate (HS) and inhibition of factor XII (FXIIa) activity, respectively. Murine HRG deficiency (Hrg−/−) leads to delayed onset but enhanced formation of thrombus compared to WT. However, in the combined FXII deficiency (F12−/−) and HRG deficiency (by siRNA or Hrg−/−), there is further thrombosis reduction compared to F12−/− alone, confirming HRG’s procoagulant activity independent of FXIIa. Mutation of target disulfides of PDI leads to a gain-of-function mutant of HRG that promotes its activities during coagulation. Thus, PDI-HRG pathway fine-tunes thrombosis by promoting its rapid initiation via neutralization of HS and preventing excessive propagation via inhibition of FXIIa.

Funder

National Natural Science Foundation of China

Natural Science Foundation of Hubei Province

American Society of Hematology

Publisher

Springer Science and Business Media LLC

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