牛支原体武威株fba基因的克隆、表达及亚细胞定位

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摘要摘要牛支原体(Mycoplasma bovis, Mb)是牛(Bos taurus)的一种重要致病性支原体，其感染可引起牛的多种疾病。果糖二磷酸醛缩酶(fructose bisphosphate aldolase, FBA)是参与糖酵解过程中的关键酶，为3-磷酸甘油醛脱氢反应提供底物，并广泛存在于生物界中。为了研究FBA在Mb细胞内的分布，本研究参照GenBank中Mb PG45株fba基因序列设计特异性引物，应用PCR扩增获得Mb武威株fba基因并将其克隆至pMD19-T载体，在完成测序及基因优化的基础上，构建原核表达载体pET-fba并转化大肠杆菌(Escherichia coli)表达菌Transetta (DE3)后经异丙基硫代半乳糖苷(isopropyl β-D-1-thiogalactopyranoside, IPTG)诱导表达，表达产物纯化后免疫新西兰兔(Oryctolagus cuniculus)制备多克隆抗体，并采用间接酶联免疫吸附试验(enzyme linked immunosorbent assay, ELISA)测定抗体效价。进而应用Western blot对Mb FBA在细胞内的分布进行了初步的定位。结果表明，Mb武威株fba基因编码框全长876 bp (GenBank登录号: KX828563)，编码292个氨基酸，优化后的基因在大肠杆菌中成功获得表达，重组蛋白rMbFBA大小约为34 kD，主要以可溶性蛋白的形式存在；ELISA测定制备的多克隆抗体效价为1∶25 600，Western blot分析结果显示，该蛋白具有良好的免疫原性，且在Mb胞浆及膜表面均有分布。上述结果为进一步研究Mb FBA的生物学功能提供了理论依据。

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	高翔
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	包世俊

关键词 ：牛支原体, 醛缩酶, 原核表达, 亚细胞定位

Abstract：Abstract Mycoplasma bovis (Mb) is an important pathogenic mycoplasma, which can cause a variety of diseases if cow (Bos taurus) infected with the Mb. Fructose bisphosphate aldolase (FBA) is one of the pivotal enzymes that involves in the p rocess of glycolysis pathway, which provided the substrate for the dehydrogenation of glyceraldehyde 3-phosphate, and widely exists in the living nature. In order to study the distribution of FBA in Mb cells, In this study, a pair of specific primers were designed according to fba gene sequence of Mb PG45 reported in GenBank. Then the fba of Mb Wuwei stain was amplified by PCR, and it was cloned into pMD19-T vector. After finished sequencing and comparing in the NCBI with other strains of Mb isolating from China, the phylogenetic trees were constructed applying with DNA Star software. Based on the sequencing and gene optimization, the prokaryotic expression vector pET-fba was constructed and transformed into Escherichia coli Transetta (DE3). Then, The target protein was induced by isopropyl β-D-1-thiogalactopyr-Anoside (IPTG). After that, we purified recombinant protein rMbFBA using Ni-NTA His Bind to immunize New Zealand rabbit (Oryctolagus cuniculus), Which aimed at preparing the polyclonal antibodies against rMbFBA. Subsequently, the antibody lever was detected by enzyme linked immunosorbent assay (ELISA). What's more, subcellular localization of FBA in Mb was performed using Western bolt. In conclusion, The results showed that the open reading frame of fba gene contains 876 nucleotides (GenBank No. KX828563), encoding a protein with 292 amino acids protein. However, there were 2 TGA codes in the sequence, which encodes trptophan in mycoplasma, but it is translated as the terminator coden in Escherichia coli. So the overlap PCR was used to make the 2 TGA termination coden mutations successfully mutate into synonymous coden TGG. The phylogenetic tree analysis from fba gene sequence of Mb Wuwei strain has high homology with other Mb strains separating from China, which indicated that the fba gene is highly conserved. Flowing that, the optimized gene was successfully expressed in Escherichia coli Transetta(DE3) when induced with final concentration of 1 mmol/L IPTG for 10 h at 20 ℃, after detected by the technology of sodium dodecyl sulfonate-polyacrylamide geleletrophoresis (SDS-PAGE), the result display that the relative molecular weight was approximately 34 kD, which existed mainly in the form of soluble protein. However, the negative control in this non target strip. The ELISA titer of antiserum was approximately up to 1∶25 600. The results of Western bolt confirmed that the prokaryotic expression products of fba gene of Mb Wuwei strain has good immunogenicity, and the FBA of Mb distributed in both cytoplasm and the membrance equally. All the results of this research lay a foundation data for further study on the biological function of FBA of Mb.

Key words： Mycoplasma bovis Fructose bisphosphate aldolase Prokaryotic expression Subcellular localization

收稿日期: 2016-10-14 出版日期: 2017-01-13

通讯作者: 包世俊 E-mail: bsjdy@126.com

引用本文:

高翔邢小勇冯娜薛慧文温峰琴包世俊. 牛支原体武威株fba基因的克隆、表达及亚细胞定位[J]. , 2017, 25(2): 274-281.

链接本文:

http://journal05.magtech.org.cn/Jwk_ny/CN/ 或 http://journal05.magtech.org.cn/Jwk_ny/CN/Y2017/V25/I2/274

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