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将狂犬病毒核蛋白结构基因重组到原核表达质粒pMAL-C_2X中,经IPTG诱导表达出的MBP-NP融合蛋白分子量约 98 kD,用支链淀粉琼脂糖凝胶亲和层析纯化得到电泳均一的融合蛋白,融合蛋白用因子 Xa裂解后,经 Q-Sepharose离子交换层析可将 MBP与 NP分开,得到了电泳均一、分子量约 56 kD的 NP蛋白,经 Western blot分析证实抗原性正确,为进一步利用NP蛋白制备抗体或单克隆抗体打下了基础。
The rabies virus nucleoprotein structural gene was recombined into the prokaryotic expression plasmid pMAL-C_2X, and the molecular weight of the MBP-NP fusion protein induced by IPTG was about 98 kD. The molecular weight of the MBP-NP fusion protein purified by amylose agarose gel electrophoresis was uniform After the fusion protein and the fusion protein were cleaved with factor Xa, MBP and NP were separated by Q-Sepharose ion exchange chromatography to obtain a homogeneous electrophoresis protein with a molecular weight of about 56 kD. Western blot analysis confirmed the antigenicity was correct The use of NP protein preparation of antibodies or monoclonal antibodies laid the foundation.