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人自噬相关基因LC3 B原核表达载体的构建及活性检测

黄蓉 叶棋浓 杜楠 徐小洁 梁迎春 王涛 冯滢滢 周丽英 李玲 冀全博 郭靖

军事医学Issue(11):867-870,4.
军事医学Issue(11):867-870,4.DOI:10.7644/j.issn.1674-9960.2014.11.007

人自噬相关基因LC3 B原核表达载体的构建及活性检测

Construction of prokaryotic expression vector with human autophagy-related LC3 B gene and its activity detection

黄蓉 1叶棋浓 2杜楠 1徐小洁 2梁迎春 2王涛 2冯滢滢 2周丽英 2李玲 2冀全博 2郭靖2

作者信息

  • 1. 解放军总医院第一附属医院,北京 100048
  • 2. 军事医学科学院生物工程研究所,北京 100850
  • 折叠

摘要

Abstract

Objective To construct the prokaryotic expression vector of human autophagy-related LC3B gene,obtain the GST-LC3B recombinant plasmid , purify the GST-LC3B fusion protein and identify its activity in vitro.Methods Human LC3B coding region was amplified from the human mammary gland cDNA by PCR and inserted into the prokaryotic expres -sion vector pGEX-KG.The recombinant plasmid pGEX-KG-LC3B was transformed into E.coli Rossate.The expressed product was purified by GST-Sepharose 4B beads and identified by SDS-PAGE and Western blot analysis .The function of the purified protein GST-LC3B was detected by GST pull-down assay.Results About 400 bp of the LC3B coding region was successfully amplified from the mammary gland library by PCR and inserted into pGEX -KG.The result of double diges-tion and sequencing showed that the GST-LC3B recombinant plasmid was successfully obtained .The GST-LC3B fusion pro-tein of about 40 000 (Mr) was successfully purified and identified by SDS-PAGE and Western blotting analysis.GST pull-down assay showed that GST-LC3B could interact with Atg4B, which identified its known function .Conclusion The pro-karyotic expression vector of GST-LC3B is constructed successfully , which will facilitate further research on the function of LC3B in autophagy.

关键词

人LC3B基因/原核表达/纯化/自噬

Key words

human LC3B/prokaryotic expression/purification/autophagy

分类

医药卫生

引用本文复制引用

黄蓉,叶棋浓,杜楠,徐小洁,梁迎春,王涛,冯滢滢,周丽英,李玲,冀全博,郭靖..人自噬相关基因LC3 B原核表达载体的构建及活性检测[J].军事医学,2014,(11):867-870,4.

基金项目

国家自然科学基金资助项目 ()

军事医学

OA北大核心CSCDCSTPCD

1674-9960

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