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水牛SOX2基因5′调控序列的克隆与功能分析

张会娜 刘庆友 刘帅 路新梅 邓彦飞 罗婵 石德顺 崔奎青

中国畜牧兽医2013,Vol.40Issue(1):1-8,8.
中国畜牧兽医2013,Vol.40Issue(1):1-8,8.

水牛SOX2基因5′调控序列的克隆与功能分析

Cloning and Function Analysis of Buffalo SOX2 Gene 5′ Regulatory Region

张会娜 1刘庆友 1刘帅 1路新梅 1邓彦飞 1罗婵 1石德顺 1崔奎青1

作者信息

  • 1. 广西大学,亚热带生物资源保护利用国家重点实验室,广西南宁 530004
  • 折叠

摘要

Abstract

To explore the transcriptional regulatory mechanism of buffalo SOX2 gene, its 5' regulatory region (2555 bp) were cloned, then five deletion mutants -2263, -1816, -1275, -660 and -407 bp were designed and constructed as EGFP reporter vectors respectively. The transcriptional activity of each deletion mutant was analysed by producing transgenic embryos and transfecting into buffalo fetal fibroblast (BFF). The results showed that the green fluorescent protein could be observed in all groups in pig embryos (4. 5 d) except p-407-EGFP, and with the gradual reduction of the fragment, the activity of the deletion mutants had a highly significant decreasing trend(P<0. 01). After transfecting into BFF 48 h, a small number of cells was able to see fluorescence in all groups except p-407-EGFP, and the transcriptional activity differences from each other were highly significant(P<0. 01) , the -2263 bp fragment had the highest activity, followed by -660 bp, then -1275 bp, and finally -1816 bp. No fluorescence was observed in p-407-EGFP group both embryo and BFF level. The results suggested that the -660~-407 bp was an integral part of the buffalo SOX2 gene basic promoter, - 2263~-1816 bp contained the non-plu-ripotential cell-specific enhancer element, there were pluripotential cell-specific enhancer elements existed in -1816~-1275 bp and -1275~-660 bp.

关键词

水牛/SOX2基因/克隆/调控序列

Key words

buffalo/SOX2 gene/clone/regulatory sequence

分类

生物科学

引用本文复制引用

张会娜,刘庆友,刘帅,路新梅,邓彦飞,罗婵,石德顺,崔奎青..水牛SOX2基因5′调控序列的克隆与功能分析[J].中国畜牧兽医,2013,40(1):1-8,8.

基金项目

国家高技术研究发展计划(863)项目(2011AA100607) (863)

国家转基因重大专项(2011ZX08007-003) (2011ZX08007-003)

国家自然科学基金(30960251). (30960251)

中国畜牧兽医

OA北大核心CSTPCD

1671-7236

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