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SLC35B2 和 TPST2 介导的 FLAG 标签硫酸化影响抗体识别。

Sulfation of a FLAG tag mediated by SLC35B2 and TPST2 affects antibody recognition.

机构信息

Key Laboratory of Carbohydrate Chemistry and Biotechnology, Ministry of Education, School of Biotechnology, Jiangnan University, Wuxi, Jiangsu, China.

出版信息

PLoS One. 2021 May 5;16(5):e0250805. doi: 10.1371/journal.pone.0250805. eCollection 2021.

Abstract

A FLAG tag consisting of DYKDDDDK is an epitope tag that is frequently and widely used to detect recombinant proteins of interest. In this study, we performed a CRISPR-based genetic screening to identify factors involved in the detection of a FLAG-tagged misfolded model protein at the cell surface. In the screening, SLC35B2, which encodes 3'-phosphoadenosine-5'-phosphosulfate transporter 1, was identified as the candidate gene. The detection of FLAG-tagged misfolded proteins at the cell surface was significantly increased in SLC35B2-knockout cells. Furthermore, protein tyrosine sulfation mediated by tyrosyl-protein sulfotransferase 2 (TPST2) suppressed FLAG-tagged protein detection. Localization analysis of the FLAG-tagged misfolded proteins confirmed that defects in tyrosine sulfation are only responsible for enhancing anti-FLAG staining on the plasma membrane but not inducing the localization change of misfolded proteins on the plasma membrane. These results suggest that a FLAG tag on the misfolded protein would be sulfated, causing a reduced detection by the M2 anti-FLAG antibody. Attention should be required when quantifying the FLAG-tagged proteins in the secretory pathway.

摘要

FLAG 标签由 DYKDDDDK 组成,是一种常用于检测目的重组蛋白的表位标签。在这项研究中,我们进行了基于 CRISPR 的遗传筛选,以鉴定参与细胞表面 FLAG 标记错误折叠模型蛋白检测的因素。在筛选中,鉴定出编码 3'-磷酸腺苷-5'-磷酸硫酸转运蛋白 1 的 SLC35B2 为候选基因。SLC35B2 敲除细胞中 FLAG 标记错误折叠蛋白的检测显著增加。此外,由酪氨酸蛋白硫转移酶 2(TPST2)介导的蛋白酪氨酸硫酸化抑制 FLAG 标记蛋白的检测。FLAG 标记错误折叠蛋白的定位分析证实,酪氨酸硫酸化缺陷仅负责增强质膜上抗 FLAG 染色,而不诱导错误折叠蛋白在质膜上的定位变化。这些结果表明,错误折叠蛋白上的 FLAG 标签会发生硫酸化,从而导致 M2 抗 FLAG 抗体的检测减少。在定量分泌途径中的 FLAG 标记蛋白时应注意这一点。

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