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粗糙脉孢菌的arg-2基因座。精氨酸特异性氨甲酰磷酸合成酶小亚基编码基因的结构与表达。

The Neurospora crassa arg-2 locus. Structure and expression of the gene encoding the small subunit of arginine-specific carbamoyl phosphate synthetase.

作者信息

Orbach M J, Sachs M S, Yanofsky C

机构信息

Department of Biological Sciences, Stanford University, California 94305-5020.

出版信息

J Biol Chem. 1990 Jul 5;265(19):10981-7.

PMID:2141606
Abstract

We have characterized genomic and cDNA clones for arg-2, the gene encoding the small subunit of the Neurospora crassa arginine-specific carbamoyl phosphate synthetase (CPS-A), and examined its transcriptional regulation. The polypeptide's predicted amino acid sequence (453 residues) is 56% and 36% identical with the sequences of the homologous polypeptides of Saccharomyces cerevisiae and Escherichia coli, respectively. The ARG2 polypeptide has an additional amino-terminal domain with the hallmark features of a mitochondrial signal sequence. The arg-2 mRNA also encodes a 24-residue peptide in the segment upstream of the coding region for the ARG2 polypeptide. This upstream open reading frame (uORF) strongly resembles the uORF in the homologous S. cerevisiae transcript. Northern analyses indicate that arg-2 mRNA levels are reduced by arginine supplementation and increased by amino acid limitation. The large increase in arg-2 mRNA levels that occurs in response to amino acid limitation is not observed in a strain containing the cpc-1 mutation, indicating that the cross-pathway control system participates in arg-2 regulation. Four copies of the sequence TGACTC, the binding site for the CPC1 regulatory protein, are found in the arg-2 genetic region. Two copies are located upstream of the mRNA start sites, and two are present within introns in the arg-2 uORF.

摘要

我们已对编码粗糙脉孢菌精氨酸特异性氨甲酰磷酸合成酶(CPS-A)小亚基的基因arg-2的基因组和cDNA克隆进行了表征,并研究了其转录调控。该多肽预测的氨基酸序列(453个残基)分别与酿酒酵母和大肠杆菌同源多肽的序列有56%和36%的同一性。ARG2多肽有一个额外的氨基末端结构域,具有线粒体信号序列的典型特征。arg-2 mRNA在ARG2多肽编码区上游的片段中还编码一个24个残基的肽。这个上游开放阅读框(uORF)与同源酿酒酵母转录本中的uORF非常相似。Northern分析表明,补充精氨酸会降低arg-2 mRNA水平,而氨基酸限制会使其增加。在含有cpc-1突变的菌株中未观察到因氨基酸限制而导致的arg-2 mRNA水平的大幅增加,这表明交叉途径控制系统参与了arg-2的调控。在arg-2基因区域发现了四个TGACTC序列拷贝,即CPC1调节蛋白的结合位点。两个拷贝位于mRNA起始位点上游,两个存在于arg-2 uORF的内含子中。

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