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埃尔朗根蛋白 S 突变 PROS1c.1904T>C(F635S)抑制分泌。

The Protein S Erlangen Mutation PROS1c.1904T>C (F635S) Suppresses Secretion.

出版信息

Clin Lab. 2024 Mar 1;70(3). doi: 10.7754/Clin.Lab.2023.230906.

Abstract

BACKGROUND

The recently identified PROS1 mutation Protein S Erlangen c.1904T>C, resulting in amino acid exchange F635S, is associated with severe quantitative protein S (PS) deficiency and clinical thrombosis. It was hypothesized that this deficiency is due to a secretion defect [1]. This report aims to further elucidate the potential secretion defect of PS Erlangen.

METHODS

Coding sequences (CDS) of wild type (WT) PROS1 (encoding PS) and mutated PROS1c.1904T>C (encoding PSF635S) were cloned in front of the CDS of green fluorescent protein (GFP), and the respective plasmids were introduced into HEK293T cells. PROS1-GFP and PROS1c.1904T>C-GFP expressing HEK293T cell lines were analyzed by confocal laser scanning microscopy and western blot for cellular proteins and proteins secreted to the growth medium.

RESULTS

Western blot analysis revealed a significantly reduced secretion of PSF635S compared to WT PS. This observation was confirmed by the detection of mutant PSF635S-GFP fusion exclusively in the endoplasmic reticulum (ER), while PS-GFP passed through the entire secretory pathway, as indicated by the localization within both the ER and Golgi apparatus.

CONCLUSIONS

The Protein S Erlangen mutation results in type I PS deficiency caused by a secretion defect.

摘要

背景

最近发现的 PROS1 突变蛋白 S 埃尔朗根 c.1904T>C,导致氨基酸交换 F635S,与严重的定量蛋白 S(PS)缺乏和临床血栓形成有关。据推测,这种缺乏是由于分泌缺陷[1]。本报告旨在进一步阐明 PS 埃尔朗根的潜在分泌缺陷。

方法

野生型(WT)PROS1(编码 PS)和突变型 PROS1c.1904T>C(编码 PSF635S)的编码序列(CDS)被克隆在绿色荧光蛋白(GFP)的 CDS 之前,分别将相应的质粒转染到 HEK293T 细胞中。通过共聚焦激光扫描显微镜和 Western blot 分析 PROS1-GFP 和 PROS1c.1904T>C-GFP 表达的 HEK293T 细胞系,以检测细胞内蛋白和分泌到生长培养基中的蛋白。

结果

Western blot 分析显示,与 WT PS 相比,PSF635S 的分泌显著减少。这种观察结果通过仅在内质网(ER)中检测到突变型 PSF635S-GFP 融合得到证实,而 PS-GFP 通过整个分泌途径,如在 ER 和高尔基体中的定位所示。

结论

蛋白 S 埃尔朗根突变导致 I 型 PS 缺乏,原因是分泌缺陷。

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