摘要
用多聚酶链反应 (PCR)扩增小鼠 B细胞趋化因子 (BL C)基因片断并导入 Bam H1和 Pst1两个酶切位点 ,插入到原核表达载体 PQE30中 ,构建重组质粒 p BL C- PQE30 ,并诱导相对分子量为 10 Kda的重组目的蛋白r BL C的表达 ,通过 Ni柱亲和层析纯化目的蛋白。双酶切和测序分析显示小鼠 B细胞趋化因子片断正确插入原核表达载体 PQE30中 ,重组蛋白 Western blot分析显示出特异性条带。提示已通过基因工程方法获得并纯化了小鼠B细胞趋化因子重组蛋白。
A DNA fragment encoding mouse B Lymphocyte Chemoattractant (BLC, MV10Kda) was obtained by PCR. The amplified fragment was inserted into prokaryotic expression vector PQE30. Recombinant protein was expressed in E. Coli XL 1 blue and purified by affinity chromatography on a nickel nitrilotriacetic acid gel matrix. Then it was identified by sequence analysis and Western blot analysis. The fragment inserted into prokaryotic expression vector PQE30 was identified to be BLC gene fragment by sequence analysis. And a specfic band was shown by Western blot analysis. These findings provide the evidence that the recombinant protein obtained and purified in this study using gene engineering method is mouse B Lymphocyte Chemoattractant.
出处
《生物医学工程学杂志》
EI
CAS
CSCD
2004年第2期251-254,共4页
Journal of Biomedical Engineering
