利用SUMO系统高效表达可溶性猪圆环病毒2型Cap蛋白
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国家自然科学青年基金(30800826);农业微生物学重点实验室开发课题(20090010);华南农业大学校长基金(5500-K08240)


Efficient Expression of Cap Gene of Porcine Circovirus Type 2 by pCold-SUMO Expression Vector
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    摘要:

    利用pCold-SUMO可溶性原核表达载体,构建表达猪圆环病毒2型缺失核定位信号肽的Cap基因的重组表达载体pCold-SUMO-dCap,并将其转入Arctic-Express表达菌株中15 ℃低温诱导表达.表达产物经SDS-PAGE分析,结果表明SUMO-dCap融合蛋白获得了高效表达,可溶性SUMO-dCap融合蛋白约占总融合蛋白的50%;用NI-NTA树脂纯化可溶性的融合蛋白,然后利用SUMO蛋白酶特异性去除SUMO标签,从而得到不含任何标签的dCap蛋白,进一步的Western-blot分析表明,表达的dCap蛋白具有良好的反应原性.

    Abstract:

    The objective of this study was to utilize pCold-SUMO expression vector to efficiently express capsid(Cap)protein gene without nuclear localization signal (NLS) of porcine circovirus 2 (PCV2).Cap gene without NLS was subcloned into the pCold-SUMO expression vetor, which named as pCold-SUMO-dCap, and the recombinant plasmid was transformed into Arctic-Express competent cells.It was induced by IPTG at 15 ℃ and efficiently produced active fusion protein of SUMO-dCap. SDS-PAGE analysis of the recombinant protein demonstrated that soluble SUMO-dCap in the supernatant was expressed at approximately 50% of total recombinant fusion proteins.Then,the soluble SUMO-dCap was purified by Ni-NTA resin purification kits, whereas the SUMO tag was removed by SUMO protease.In addition,the purification effect and specificity of recombinant fusion protein and capsid protein without NLS were detected by Western-blot assay.The results showed that both of them had been well purified and possessed good reactionogenicity.

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陈春丽,郭宇飞,陈筱薇,叶昱,王强,廖明,樊惠英.利用SUMO系统高效表达可溶性猪圆环病毒2型Cap蛋白[J].华南农业大学学报,2012,33(3):393-397

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  • 收稿日期:2011-09-06
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  • 在线发布日期: 2012-07-29