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黑曲霉柠檬酸合酶的特性及citA过表达对柠檬酸生产的影响。

Properties of Aspergillus niger citrate synthase and effects of citA overexpression on citric acid production.

作者信息

Ruijter G J, Panneman H, Xu D, Visser J

机构信息

Section Molecular Genetics of Industrial Microorganisms, Wageningen Agricultural University, Dreijenlaan 2, 6703 HA, Wageningen, The Netherlands.

出版信息

FEMS Microbiol Lett. 2000 Mar 1;184(1):35-40. doi: 10.1111/j.1574-6968.2000.tb08986.x.

Abstract

Using a combination of dye adsorption and affinity elution we purified Aspergillus niger citrate synthase to homogeneity using a single column and characterised the enzyme. An A. niger citrate synthase cDNA was isolated by immunological screening and used to clone the corresponding citA gene. The deduced amino acid sequence showed high similarity to other fungal citrate synthases. After processing upon mitochondrial import, the calculated M(r) of A. niger citrate synthase is 48501, which agrees well with the estimated molecular mass of the purified protein (48 kDa). In addition to an N-terminal mitochondrial import signal, a peroxisomal target sequence (AKL) was found at the C-terminus of the protein. Whether both signals are functional in vivo is not clear. Strains overexpressing citA were made by transformation and cultured under citric acid-producing conditions. Up to 11-fold overproduction of citrate synthase did not increase the rate of citric acid production by the fungus, suggesting that citrate synthase contributes little to flux control in the pathway involved in citric acid biosynthesis by a non-commercial strain.

摘要

我们采用染料吸附和亲和洗脱相结合的方法,使用单一色谱柱将黑曲霉柠檬酸合酶纯化至同质,并对该酶进行了表征。通过免疫筛选分离出黑曲霉柠檬酸合酶cDNA,并用于克隆相应的citA基因。推导的氨基酸序列与其他真菌柠檬酸合酶具有高度相似性。在线粒体导入后进行加工,黑曲霉柠檬酸合酶的计算分子量为48501,这与纯化蛋白的估计分子量(48 kDa)非常吻合。除了N端线粒体导入信号外,在该蛋白的C端还发现了一个过氧化物酶体靶向序列(AKL)。尚不清楚这两个信号在体内是否都具有功能。通过转化构建了过表达citA的菌株,并在产柠檬酸条件下进行培养。柠檬酸合酶产量高达11倍的过量生产并未提高该真菌产柠檬酸的速率,这表明柠檬酸合酶对非商业菌株柠檬酸生物合成途径中的通量控制贡献不大。

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