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指导在大肠杆菌中表达甲硫氨酸-凝乳酶原的质粒不稳定性研究。

Investigation of the instability of plasmids directing the expression of Met-prochymosin in Escherichia coli.

作者信息

Caulcott C A, Lilley G, Wright E M, Robinson M K, Yarranton G T

出版信息

J Gen Microbiol. 1985 Dec;131(12):3355-65. doi: 10.1099/00221287-131-12-3355.

Abstract

The causes of the instability of a multicopy plasmid, pCT70, which directs the expression of calf prochymosin in Escherichia coli, were investigated. Plasmid pAT153 and its derivative, pCT54, were stable for more than 90 generations in continuous culture with glucose limitation. The multicopy plasmid pCT66, which expressed very low levels of prochymosin due to poor translational efficiency, and low copy number plasmids which efficiently expressed the prochymosin gene, were also stable. These results indicated that high level translation of the recombinant gene was the cause of the instability of pCT70. The maximum specific growth rate of E. coli(pCT70) was reduced by 30% compared with E. coli(pCT66). To fulfil the requirements of a production system, a dual origin plasmid with controllable copy number was developed. Both this plasmid (pMG165) and a derivative which contained the prochymosin gene (pMG168) were stable when maintained at low copy number. When the copy number of plasmid pMG168 was increased by putting replication under the control of the lambda PR promoter and the cI857 temperature sensitive repressor, expression of prochymosin was achieved. This strategy enables large-scale production of prochymosin without the need for antibiotic selection or other methods of preventing plasmid loss.

摘要

对指导小牛凝乳酶原在大肠杆菌中表达的多拷贝质粒pCT70的不稳定性原因进行了研究。质粒pAT153及其衍生物pCT54在葡萄糖受限的连续培养中90多代都很稳定。由于翻译效率低而表达极低水平凝乳酶原的多拷贝质粒pCT66以及有效表达凝乳酶原基因的低拷贝数质粒也很稳定。这些结果表明重组基因的高水平翻译是pCT70不稳定的原因。与大肠杆菌(pCT66)相比,大肠杆菌(pCT70)的最大比生长速率降低了30%。为满足生产系统的要求,开发了一种具有可控拷贝数的双原点质粒。当维持在低拷贝数时,该质粒(pMG165)及其包含凝乳酶原基因的衍生物(pMG168)都很稳定。当通过将复制置于λPR启动子和cI857温度敏感阻遏物的控制下增加质粒pMG168的拷贝数时,实现了凝乳酶原的表达。该策略能够在无需抗生素选择或其他防止质粒丢失方法的情况下大规模生产凝乳酶原。

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