[The Effect of VWF Propeptide on VWF Mutant in D1 Domain].

Zhongguo shi yan xue ye xue za zhi Pub Date : 2022-10-01 DOI:10.19746/j.cnki.issn.1009-2137.2022.05.037

Xiu-Qun Yu, Zhen-Ni Ma, Jing Ling, Yun-Xiao Zhao, Jie Yin, Zi-Qiang Yu, Chang-Geng Ruan

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Abstract

Objective: To investigate whether co-transfection of wild-type VWFpp with VWF mutant in D1 region is able to correct VWF defects in biosynthesis and secretion.

Methods: Four VWF mutant plasmids were single transfected into HEK 293 cells, or co-transfected into HEK 293 cells with the wild type VWFpp plasmids. The VWF in supernatant and lysate of transfected cells were analyzed by ELISA, vertical VWF multimer electrophoresis. The retention of VWF in endoplasmic reticulum of transfected cells were detected by immunofluorescence confocal microscope.

Results: In the vertical VWF multimer analysis, with co-expressing VWF mutant and VWFpp, the VWF multimer bands disappeared, and the VWF antigen in both supernatant and lysate of cells decreased, compared with the single expression of VWF mutant. Although the intracellular levels of VWF antigens decreased after co-expression, the retention rate of VWF mutant decreased in endoplasmic reticulum.

Conclusion: VWFpp can reduce the retention of VWF in endoplasmic reticulum, assists the transport of VWF between subcellular organelles. However, VWFpp inhibits the biosynthesis and secretion of VWF about the mutant in D1 domain.

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VWF前肽对VWF D1结构域突变体的影响

目的:探讨野生型VWFpp与D1区VWF突变体共转染是否能够纠正VWF在生物合成和分泌方面的缺陷。方法:将4个VWF突变质粒单独转染HEK 293细胞，或与野生型VWFpp质粒共转染HEK 293细胞。采用ELISA、垂直VWF多段电泳对转染细胞的上清液和裂解液中的VWF进行分析。免疫荧光共聚焦显微镜检测转染细胞内质网中VWF的滞留情况。结果:在垂直VWF多聚体分析中，与单独表达VWF突变体相比，VWF突变体与VWFpp共表达时，VWF多聚体条带消失，细胞上清液和细胞溶出液中VWF抗原减少。虽然共表达后VWF抗原的细胞内水平降低，但VWF突变体在内质网中的保留率降低。结论:VWFpp可减少VWF在内质网的滞留，促进VWF在亚细胞器间的转运。而VWFpp抑制突变体D1结构域VWF的生物合成和分泌。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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