Unkles S E, Smith J, Kanan G J, Millar L J, Heck I S, Boxer D H, Kinghorn J R
School of Environmental and Evolutionary Biology, University of St. Andrews, St. Andrews, Fife KY16 9TH, United Kingdom.
J Biol Chem. 1997 Nov 7;272(45):28381-90. doi: 10.1074/jbc.272.45.28381.
The Aspergillus nidulans complex locus, cnxABC, has been shown to be required for the synthesis of precursor Z, an intermediate in the molybdopterin cofactor pathway. The locus was isolated by chromosome walking a physical distance of 65-kilobase pairs from the brlA gene and defines a single transcript that encodes, most likely, a difunctional protein with two catalytic domains, CNXA and CNXC. Mutations (cnxA) affecting the CNXA domain, mutants (cnxC) in the CNXC domain, and frameshift (cnxB) mutants disrupting both domains have greatly reduced levels of precursor Z compared with the wild type. The CNXA domain is similar at the amino acid level to the Escherichia coli moaA gene product, while CNXC is similar to the E. coli moaC product, with both E. coli products encoded by different cistrons. In the wild type, precursor Z levels are 3-4 times higher in nitrate-grown cells than in those grown on ammonium, and there is an approximately parallel increase in the 2.4-kilobase pair transcript following growth on nitrate, suggesting nitrate induction of this early section of the pathway. Analysis of the deduced amino acid sequence of several mutants has identified residues critical for the function of the protein. In the CNXA section of the protein, insertion of three amino acid residues into a domain thought to bind an iron-sulfur cofactor leads to a null phenotype as judged by complete loss of activity of the molybdoenzyme, nitrate reductase. More specifically, a mutant has been characterized in which tyrosine replaces cysteine 345, one of several cysteine residues probably involved in binding the cofactor. This supports the proposition that these residues play an essential catalytic role. An insertion of seven amino acids between residues valine 139 and serine 140, leads to a temperature-sensitive phenotype, suggesting a conformational change affecting the catalytic activity of the CNXA region only. A single base pair deletion leading to an in frame stop codon in the CNXC region, which causes a null phenotype, effectively deletes the last 20 amino acid residues of the protein, indicating that these residues are necessary for catalytic function.
构巢曲霉复合基因座cnxABC已被证明是合成前体Z所必需的,前体Z是钼蝶呤辅因子途径中的一个中间体。该基因座是通过从brlA基因开始染色体步移65千碱基对的物理距离分离得到的,它定义了一个单一的转录本,最有可能编码一种具有两个催化结构域CNXA和CNXC的双功能蛋白。与野生型相比,影响CNXA结构域的突变(cnxA)、CNXC结构域中的突变体(cnxC)以及破坏两个结构域的移码(cnxB)突变体,前体Z的水平都大大降低。CNXA结构域在氨基酸水平上与大肠杆菌的moaA基因产物相似,而CNXC与大肠杆菌的moaC产物相似,这两种大肠杆菌产物由不同的顺反子编码。在野生型中,硝酸盐培养的细胞中前体Z的水平比铵培养的细胞高3 - 4倍,并且在硝酸盐上生长后,2.4千碱基对的转录本也有大致平行的增加,这表明该途径的这一早期部分受到硝酸盐诱导。对几个突变体推导的氨基酸序列分析确定了对该蛋白功能至关重要的残基。在该蛋白的CNXA部分,在一个被认为结合铁硫辅因子的结构域中插入三个氨基酸残基会导致无效表型,从钼酶硝酸还原酶的活性完全丧失可以判断出来。更具体地说,已经鉴定出一个突变体,其中酪氨酸取代了半胱氨酸345,半胱氨酸345是可能参与结合辅因子的几个半胱氨酸残基之一。这支持了这些残基发挥重要催化作用的观点。在缬氨酸139和丝氨酸140残基之间插入七个氨基酸会导致温度敏感表型,这表明构象变化仅影响CNXA区域的催化活性。在CNXC区域导致框内终止密码子的单个碱基对缺失会导致无效表型,有效地删除了该蛋白的最后20个氨基酸残基,表明这些残基对于催化功能是必需的。
