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Cloning, sequence analysis, and expression of the structural gene encoding glucose-fructose oxidoreductase from Zymomonas mobilis.

机译:运动发酵单胞菌葡萄糖-果糖氧化还原酶编码基因的克隆,序列分析和表达。

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摘要

The gene encoding glucose-fructose oxidoreductase (gfo) from Zymomonas mobilis was cloned in Escherichia coli and sequenced. An open reading frame of 439 amino acids encoded a protein of 49 kDa. A leader sequence of 52 amino acids preceded the N-terminal sequence of the enzyme, indicating cleavage of the precursor protein at an Ala-Ala site to give rise to an active form of the enzyme of 43 kDa. Processing of the glucose-fructose oxidoreductase leader sequence, although not complete, was demonstrated in an in vitro translation system. The two Z. mobilis promoters of the gfo gene show considerable homology to other highly expressed Z. mobilis genes (pdc, adhB, gap, and pgk) as well as to the E. coli consensus sequence. Although translation of the gfo gene was demonstrated in vitro in an E. coli S30 coupled transcription-translation system, a functional stable protein was not produced in the E. coli clone. However, the gfo gene cloned into a shuttle vector was shown to overexpress glucose-fructose oxidoreductase to levels of up to 6% of the soluble protein in Z. mobilis.
机译:来自运动发酵单胞菌的葡萄糖-果糖氧化还原酶(gfo)的编码基因被克隆到大肠杆菌中并测序。 439个氨基酸的开放阅读框编码49 kDa的蛋白质。 52个氨基酸的前导序列位于酶的N端序列之前,表明前体蛋白在Ala-Ala位点处裂解,从而产生43 kDa酶的活性形式。葡萄糖-果糖氧化还原酶前导序列的加工虽然不完整,但在体外翻译系统中得到了证实。 gfo基因的两个运动发酵单胞菌启动子与其他高度表达的运动发酵单胞菌基因(pdc,adhB,gap和pgk)以及大肠杆菌共有序列显示出相当的同源性。尽管在大肠杆菌S30偶联的转录-翻译系统中证实了gfo基因的翻译,但在大肠杆菌克隆中未产生功能稳定的蛋白质。然而,克隆到穿梭载体中的gfo基因显示过表达葡萄糖-果糖氧化还原酶至运动发酵单胞菌中可溶性蛋白的水平高达6%。

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