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蛋白二硫键异构酶过表达增强维生素 K 环氧化物还原酶活性。

Overexpression of protein disulfide isomerase enhances vitamin K epoxide reductase activity.

机构信息

USC 1233 RS2GP, VetAgro Sup, INRAE, University of Lyon, 69280, Marcy L'Etoile, France.

出版信息

Biochem Cell Biol. 2022 Apr;100(2):152-161. doi: 10.1139/bcb-2021-0441. Epub 2022 Jan 10.

Abstract

Vitamin K epoxide reductase (VKOR) activity is catalyzed by the VKORC1 enzyme. It is a target of vitamin K antagonists (VKA). Numerous mutations of VKORC1 have been reported and are suspected to confer resistance to VKA and (or) affect its velocity. Nevertheless, the results of these studies have been conflicting, and the functional characterization of these mutations in the cell system is complex because of the interweaving of VKOR activity in the vitamin K cycle. In this study, a new cellular approach was implemented to evaluate the vitamin K cycle in HEK293 cells. This global approach was based on the vitamin K quinone/vitamin K epoxide (K/KO) balance. In the presence of VKA or when VKORC1 and VKORC1L1 were knocked out, the K/KO balance decreased significantly due to the accumulation of vitamin KO. In contrast, when VKORC1 was overexpressed, the balance remained unchanged, demonstrating the limitation of VKOR activity. This limitation was shown to be due to insufficient expression of the activation partner of VKORC1, as overexpression of protein disulfide isomerase (PDI) overcomes this limitation. This study is the first to demonstrate the functional interaction between VKORC1 and PDI.

摘要

维生素 K 环氧化物还原酶 (VKOR) 活性由 VKORC1 酶催化。它是维生素 K 拮抗剂 (VKA) 的靶点。已经报道了许多 VKORC1 的突变,这些突变被怀疑赋予了对 VKA 的抗性和(或)影响其速度。然而,这些研究的结果存在冲突,并且由于 VKOR 活性在维生素 K 循环中的交织,这些突变在细胞系统中的功能特征变得复杂。在这项研究中,实施了一种新的细胞方法来评估 HEK293 细胞中的维生素 K 循环。这种全局方法基于维生素 K 醌/维生素 K 环氧化物 (K/KO) 平衡。在 VKA 存在下或当 VKORC1 和 VKORC1L1 被敲除时,由于 KO 的积累,K/KO 平衡显著降低。相比之下,当 VKORC1 过表达时,平衡保持不变,表明 VKOR 活性受到限制。这种限制是由于 VKORC1 的激活伴侣表达不足所致,因为过表达蛋白二硫键异构酶 (PDI) 克服了这种限制。这项研究首次证明了 VKORC1 和 PDI 之间的功能相互作用。

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