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Construction and evaluation of anti-gastrin immunogen based on P64K protein

机译:基于P64K蛋白的抗胃泌素免疫原的构建与评价

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摘要

AIM: To construct two kinds of anti-gastrin immunogen based on P64K protein from Neisseria meningitids and to compare their immunogenic effect.METHODS: G17P64K gene was cloned and ligated into pET28a plasmid, then transformed into BL21(DE3). After inoculation of LB medium and IPTG induction, the recombinant protein was solubly expressed at a high level.The purification of G17P64K fusion protein was similar to that of P64K. An initial step of purification consisting of 30 % saturated ammonium sulfate precipitation was done. Additional fine optimizations included phenyl-sepharose, G200 Sephadex gel filtration and Q-sepharose anion exchanger chromatography. Highly purified protein was obtained and sequenced at the N-terminal amino acid residues. Polypeptide was synthesized by Fmoc solid phase chemical method and cross-linked to carrier protein P64K and DT mutant by MBS method and then the rabbit anti-gastrin 17 antibody was prepared by immunizing rabbit with cross-linked and fused protein. The titer and the activity in vitro of antibody were assessed.RESULTS: G17P64K gene and the recombinant bacteria were obtained. After four steps purification, protein sample that has the purity above 90 % was achieved. At the 84th day after the first immunization, the titer of antibody against cross-linked protein reached 51 200. Evaluation of the antibody in vitro manifested that it had a high inhibitory activity on the growth of tumor cell SW480.CONCLUSION: The P64K-polypeptide cross-linked immunogen immunized rabbit and achieved a higher titer antibody against gastrin 17 than the G17P64K fusion protein immunogen, which could inhibit the growth of the tumor cell SW480.
机译:目的:基于脑膜炎奈瑟氏球菌的P64K蛋白构建两种抗胃泌素免疫原,并比较其免疫原性。方法:克隆G17P64K基因并连接到pET28a质粒中,然后转化为BL21(DE3)。接种LB培养基并诱导IPTG后,重组蛋白高水平可溶表达。G17P64K融合蛋白的纯化与P64K相似。完成了由30%饱和硫酸铵沉淀组成的纯化第一步。其他精细优化包括苯基琼脂糖,G200 Sephadex凝胶过滤和Q-琼脂糖阴离子交换色谱。获得了高度纯化的蛋白质,并在N末端氨基酸残基处测序。通过Fmoc固相化学方法合成多肽,并通过MBS方法与载体蛋白P64K和DT突变体交联,然后用交联融合蛋白免疫兔,制备兔抗胃泌素17抗体。结果:获得了G17P64K基因,并获得了重组细菌。经过四步纯化,获得的蛋白样品的纯度在90%以上。第一次免疫后第84天,抗交联蛋白的抗体效价达到51200。体外评估表明,该抗体对肿瘤细胞的生长具有很高的抑制活性。结论:P64K-多肽交联免疫原免疫家兔,与G17P64K融合蛋白免疫原相比,对胃泌素17的效价更高,可以抑制肿瘤细胞SW480的生长。

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