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作 者:费浩[1] 罗明娟[1] 叶玉珍[2] 丁达夫[2] 戚正武[1]
机构地区:[1]中国科学院上海生物化学与细胞生物学研究所分子生物学国家重点实验室,上海200031 [2]中国科学院上海生物化学与细胞生物学研究所,上海200031
出 处:《生物化学与生物物理学报》2001年第6期591-599,共9页
基 金:国家重点基础研究发展规划项目 ( 973) (No .G19980 5 112 1);国家高技术"86 3"计划项目 (No .10 3 13 0 1 0 3)~~
摘 要:蛋白质前体加工酶参与许多重要蛋白质前体的加工成熟过程 ,哺乳动物来源的furin和酵母中的kexin是该家族的重要成员。首先人工合成了编码枯草杆菌蛋白酶抑制剂eglinC的基因片段 ,组装后在大肠杆菌中得到表达。以定点突变方法在野生型eglinC抑制活性中心的P1、P2 和P4 位引入碱性氨基酸残基可以将其改造为很强的furin抑制剂 (Ki约 10 -9mol/L) ,和kexin抑制剂 (Ki 约 10 -11mol/L)。同时根据枯草杆菌蛋白酶和eglinC复合物的晶体结构 ,计算机同源模建了前体加工酶与eglinC突变体结构之间的相互作用 ,并结合实验数据得到以下结果 :(1)P1位引入的碱性残基是该抑制剂活力的前提 ;(2 )P4 位碱性残基的引入可以极大地提高抑制剂活力约两个数量级 ;(3)P2 位的碱性残基将有效提高抑制剂的活力 ,然而同时可以破坏抑制剂本身的稳定性 ;(4 )野生型P3 位的疏水性残基参与抑制剂活性环附近疏水核心的构成。Mammalian furin and yeast kexin are members of the proprotein convertase family involved in the proteolytic processing of many important precursor proteins. Here the gene coding for the subtilisin inhibitor eglin C was totally synthesized and expressed in E.coli. Substitution of residues at each position P 1, P 2 and P 4 of eglin C with a basic residue using protein engineering could make eglin C a very strong inhibitor for furin ( K i around 10 -9 mol/L), and even more strong for kexin ( K i around 10 -11 mol/ L). Results indicated that: (1) A basic residue Lys or Arg at P 1 site is prerequisite for the inhibitor. (2) The second mutation with basic residue at P 4 site drastically increase the inhibitory activity by two orders of magnitude. (3) A basic residue at P 2 site is favorable for the binding to the enzyme, but unfavorable for the stability of the inhibitor, resulting in a temporary inhibition. (4) A hydrophobic residue is preferential at P 3 site. Based on the known crystal structures of subtilisin and eglin C, the interaction between the enzyme and inhibitor was modeled, and their involved residues were predicted which gave a good explanation to the experimental results.
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