[Prediction of epitope region and preparation of mouse polyclonal antibody of human Shisa-like protein 1(SHISAL1)].

Jinli Wang, Xinzhan Zhang, Yisha Gao, Lili Zhou, Daquan Sun
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Abstract

Objective To investigate antigen optimization of Shisa like protein 1 (SHISAL1) for preparing mouse anti-human SHISAL1 polyclonal antibody and to identify the specificity of the prepared antibody. Methods Bioinformatics was employed to predict the antigenic epitope region of SHISAL1 protein, and then a polypeptide composed of amino acid residues from the site of 28 to 97 of SHISAL1, termed SHISAL1-N, was selected as the antigen. The coding region of SHISAL1-N was cloned by molecular cloning technique, and then it was inserted into pET-28a to generate pET28a-SHISAL1-N recombinant plasmid. The two recombinant plasmids pET28a-SHISAL1-N and pET28a-SHISAL1 were transformed into BL21 (DE3) bacteria and induced to express by IPTG. The two proteins were purified and immunized to female Kunming mice, respectively. The specificities and sensitivities of the acquired antibodies were detected by Western blot analysis, immunoprecipitation and immunofluorescent cytochemical staining. Results pET28a-SHISAL1-N recombinant plasmid was successfully constructed, and the two fused proteins, SHISAL1 and SHISAL1-N, were induced to express. Moreover, two types of SHISAL1 mouse polyclonal antibodies, derived from SHISAL1-N and SHISAL1 antigens, were obtained. Western blot results showed that the antibody prepared from SHISAL1 antigen was less specific and sensitive compared with the antibody prepared from SHISAL1-N antigen which could specifically identify different endogenous SHISAL1 protein. Immunoprecipitation results showed that SHISAL1-N antibody could specifically pull down SHIISAL1 protein in hepatocellular carcinoma cells and immunofluorescence results demonstrated that SHISAL1-N antibody could specifically bind to SHISAL1 protein in the cytoplasm. Conclusion We have optimized the SHISAL1 antigen and prepared the mouse anti-human SHISAL1 polyclonal antibodies successfully, which can be used for Western blot analysis, immunoprecipitation and immunofluorescence cytochemical staining.

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[人shisa样蛋白1(SHISAL1)小鼠多克隆抗体的制备及表位区预测]。
目的研究Shisa样蛋白1 (SHISAL1)制备小鼠抗人SHISAL1多克隆抗体的抗原优化,并鉴定其特异性。方法采用生物信息学方法对SHISAL1蛋白抗原表位区域进行预测,选择由SHISAL1的28 ~ 97位氨基酸残基组成的多肽SHISAL1- n作为抗原。利用分子克隆技术克隆出SHISAL1-N的编码区,并将其插入pET-28a中,生成pET28a-SHISAL1-N重组质粒。将重组质粒pET28a-SHISAL1- n和pET28a-SHISAL1转化至BL21 (DE3)菌中,经IPTG诱导表达。纯化后分别免疫昆明雌性小鼠。免疫印迹法、免疫沉淀法和免疫荧光细胞化学染色法检测所得抗体的特异性和敏感性。结果成功构建了pET28a-SHISAL1-N重组质粒,并诱导表达了融合蛋白SHISAL1和SHISAL1- n。此外,还获得了两种SHISAL1小鼠多克隆抗体,分别来自SHISAL1- n和SHISAL1抗原。Western blot结果显示,与SHISAL1- n抗原制备的抗体相比,SHISAL1抗原制备的抗体特异性和敏感性较低,可特异性识别不同的内源性SHISAL1蛋白。免疫沉淀结果显示SHISAL1- n抗体能特异性拉低肝癌细胞中的SHIISAL1蛋白,免疫荧光结果显示SHISAL1- n抗体能特异性结合细胞质中的SHISAL1蛋白。结论对SHISAL1抗原进行了优化,成功制备了小鼠抗人SHISAL1多克隆抗体,可用于Western blot分析、免疫沉淀和免疫荧光细胞化学染色。
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