欢迎访问《现代生物医学进展》编辑部！

目的：构建鹿茸富脯氨酸多肽（APRP）基因融合表达载体，并诱导表达融合蛋白GST-APRP。方法：以鹿茸顶端组织总cDNA 为模板，PCR 方法扩增目的片段，连接pMDTM18-T 载体，转化DH5琢进行TA克隆。酶切与测序鉴定合格后，将目的片段与pGEX-6P-1 质粒连接，完成pGEX-6P-1-APRP融合表达载体的构建。利用原核表达系统进行初步诱导表达。SDS-PAGE 蛋白电泳检测蛋白表达情况。结果：PCR 成功扩增出目的基因片段，目的基因片段大小为216 bp。提取表达载体质粒经酶切及测序分析证实pGEX-6P-1-APRR 融合表达载体构建成功。利用终浓度为0.5 mMIPTG 诱导，融合蛋白成功表达，分子量为35 kDa。结论：目前利用基因工程技术获得特定的鹿茸多肽的报道很少。本研究结果表明，利用原核表达系统可在体外对鹿茸富脯氨酸多肽基因（APRP）进行融合表达，并且融合蛋白GST-APRP 以可溶形式表达，有利于进一步研究APRP。这也为研究其他鹿茸多肽单体成分提供重要参考。

英文摘要:

Objective:To construct the fusion expression vector of antler proline-rich polypeptide (APRP), and induce the expression of fusion protein GST-APRP.Methods:The APRP segment was amplified by PCR technology with total cDNA template of velvet antler top organization. The product of amplification was linked with pMDTM18-T vector, and the plasmid was transformed into DH5琢to accomplish TA clone. The fusion expression vector pGEX-6P-1-APRP was constructed by linking the target segment with pGEX-6P-1 vector after the correct identification of enzyme digestion and sequencing. Prokaryotic expression system was used to induce the expression of protein preliminarily, and expression was detect by SDS-PAGE protein electrophoresis.Results:We amplified the APRP gene fragment by PCR, the length of it was 216bp, and constructed the fusion expression vector pGEX-6P-1-APRR successfully. We obtained the fusion protein whose molecular weight was 35 kDa by using 0.5 mMIPTG of final concentration.Conclusion:The reports' quantity of obtaining specific velvet antler polypeptides by genetic engineering technology is rare currently. This study results show that we can induce the fusion expression of antler proline-rich polypeptide(APRP) in vitro, and GST-APRP fusion protein expressed with soluble form, which is helpful for further research of APRP. These efforts are also providing a valuable reference for the researching of other monomer composition of velvet antler polypeptides.

查看全文查看/发表评论下载PDF阅读器

关闭