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用荧光相图法研究胃蛋白酶的去折叠过程 被引量:3

Unfolding of pepsin induced by urea or guanidine hydrochloride with fluorescence phase diagram
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摘要 蛋白质折叠机理的研究是基因重组蛋白质高效生产的前提条件,对于工业化生产重组蛋白以及治疗与蛋白集聚密切相关的疾病都有重要意义。为了探索一个统一的蛋白质折叠机理,用荧光相图法分别对脲和盐酸胍诱导的胃蛋白酶的去折叠过程进行了研究。结果表明,无论变性体系中有无还原剂2-巯基乙醇存在,当脲浓度为0-8.0 mol/L时,脲诱导胃蛋白酶的变性过程都符合“二态模型”;而无论变性体系中有无还原剂2-巯基乙醇存在,当盐酸胍浓度为0-6.0 mol/L时,该蛋白的变性过程均符合“三态模型”。 The research of the mechanism of the protein folding is the precondition of highly efficient production of genetic recombinant proteins,which has important significance to the industrial production of recombinant protein and treatment of those diseases closely related to the protein aggregation.To explore a unified mechanism of protein folding,the unfolding of pepsin induced by urea or guanidine hydrochloride has been studied by"phase diagram"method of fluorescence.The experimental results show that whether 2-mercaptoethanol exists in the denaturant solution or not,when urea concentrations are changed under the range of 0 to 8.0 mol/ L,the unfolding procedures of pepsin obey a typical"two-state model";while whether the 2-mercaptoethanol exists in the denaturant solution or not,when guanidine hydrochloride concentrations are changed under the range of 0 to 6.0 mol/ L,the unfolding of pepsin obey a typical "three-state model".
作者 刘莉 董发昕 胥耀平 边六交
机构地区 西北农林科技大学林学院 西北大学化学系 西北大学生命科学院基因工程药物研究开发中心
出处 《西北农林科技大学学报(自然科学版)》 CSCD 北大核心 2007年第11期187-190,共4页 Journal of Northwest A&F University(Natural Science Edition)
关键词 胃蛋白酶 去折叠 折叠中间态 荧光相图法 pepsin protein unfolding intermediates phase diagram method of fluorescence
分类号 Q518.4 [生物学—生物化学]
  • 相关文献

参考文献10

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共引文献22

同被引文献94

  • 1傅容湛,董发昕,边六交.荧光相图法研究脲诱导牛血清白蛋白的去折叠过程[J].分析测试学报,2006,25(6):19-22. 被引量:5
  • 2梁长利,边六交.用蛋白电泳和高效凝胶排阻色谱法分析还原脲变性蛋白溶菌酶稀释复性过程的集聚体[J].分析科学学报,2006,22(6):641-645. 被引量:5
  • 3师江波,边六交,董发昕.荧光相图法研究猪胰腺α-淀粉酶在脲和盐酸胍溶液中的去折叠过程[J].分析化学,2007,35(5):707-710. 被引量:9
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引证文献3

二级引证文献9

西北农林科技大学学报(自然科学版)
2007年 第11期

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