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来自大肠杆菌的具有生物活性的人乙酰胆碱酯酶的表达与重组。

Expression and reconstitution of biologically active human acetylcholinesterase from Escherichia coli.

作者信息

Fischer M, Ittah A, Liefer I, Gorecki M

机构信息

Bio-Technology General Ltd., Kiryat Weizmann, Rehovot, Israel.

出版信息

Cell Mol Neurobiol. 1993 Feb;13(1):25-38. doi: 10.1007/BF00712987.

Abstract
  1. Authentic human acetylcholinesterase (AChE) was expressed in Escherichia coli under regulation of the constitutive deo promoter or the thermo-inducible lambda PL promoter. 2. To facilitate expression in the prokaryotic system, recombinant human AChE (rhAChE) cDNA was modified at the N terminus by oligonucleotide substitutions in order to replace some of the GC-rich regions by AT. These modifications did not alter the amino acid sequence but resulted in ample production of the protein. 3. rhAChE accumulated in the cells and reached a level of 10% of total bacterial proteins. A partially purified inactive recombinant protein was recovered from inclusion bodies. 4. Active rhAChE was obtained after solubilization, folding, and oxidation, although the recovery of the active enzyme was low. A 20- to 40-fold increase in enzymatically active rhAChE was achieved by replacing Cys580 by serine. 5. The recombinant enzyme analogue was indistinguishable from native AChE isolated from erythrocytes in terms of substrate specificity and inhibitor selectivity.
摘要
  1. 人源真性乙酰胆碱酯酶(AChE)在组成型deo启动子或热诱导型λPL启动子的调控下于大肠杆菌中表达。2. 为便于在原核系统中表达,重组人AChE(rhAChE)cDNA在N端通过寡核苷酸替换进行修饰,以用AT替换一些富含GC的区域。这些修饰未改变氨基酸序列,但导致该蛋白大量产生。3. rhAChE在细胞中积累,达到细菌总蛋白的10%水平。从包涵体中回收了部分纯化的无活性重组蛋白。4. 经溶解、折叠和氧化后获得了活性rhAChE,尽管活性酶的回收率较低。通过将Cys580替换为丝氨酸,酶活性rhAChE提高了20至40倍。5. 重组酶类似物在底物特异性和抑制剂选择性方面与从红细胞中分离的天然AChE无法区分。

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