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Cloning sequence analysis and functional expression of the acetyl coenzyme A synthetase gene from Methanothrix soehngenii in Escherichia coli.

机译:产甲烷甲烷菌的乙酰辅酶A合成酶基因的克隆序列分析和功能表达

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摘要

In the acetoclastic methanogen Methanothrix soehngenii, acetate is activated to acetyl coenzyme A by acetyl coenzyme A synthetase (Acs). The acs gene, coding for the single Acs subunit, was isolated from a genomic library of M. soehngenii DNA in Escherichia coli by using antiserum raised against the purified Acs. After introduction in E. coli, the acs gene was expressed, resulting in the production of an immunoreactive protein of 68 kDa, which is approximately 5 kDa smaller than the known size of purified Acs. In spite of this difference in size, the Acs enzymes are produced in similar quantities in E. coli and M. soehngenii and show comparable specific activities. Upstream from the acs gene, consensus archaeal expression signals were identified. Immediately downstream from the acs gene there was a putative transcriptional stop signal. The amino acid sequence deduced from the nucleotide sequence of the acs gene showed homology with those of functionally related proteins, i.e., proteins involved in the binding of coenzyme A, ATP, or both.
机译:在乙酰碎裂性产甲烷菌Methanothrix soehngenii中,乙酸盐被乙酰辅酶A合成酶(Acs)活化为乙酰辅酶A。通过使用针对纯化的Acs的抗血清从大肠杆菌中的M. soehngenii DNA基因组文库中分离出编码单个Acs亚基的acs基因。导入大肠杆菌后,表达acs基因,从而产生68 kDa的免疫反应蛋白,该蛋白比已知大小的纯化Acs小约5 kDa。尽管存在大小差异,但是Acs酶在大肠杆菌和M. soehngenii中的产生量相似,并显示出相当的比活性。从acs基因上游,鉴定出共识古细菌表达信号。紧接在acs基因下游的是一个假定的转录终止信号。从acs基因的核苷酸序列推导的氨基酸序列显示出与功能相关蛋白,即参与辅酶A,ATP或两者结合的蛋白的同源性。

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