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The ARO4 gene of Candida albicans encodes a tyrosine-sensitive DAHP synthase: evolution, functional conservation and phenotype of Aro3p-, Aro4p-deficient mutants

机译:念珠菌的ARO4基因编码酪氨酸敏感的DAHP合酶:ARO3P-,ARO4P缺陷型突变体的演化,功能养护和表型

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The enzyme 3-deoxy-D-arabinoheptulosonate-7-phosphate (DAHP) synthase catalyses the first step in aromatic amino acid biosynthesis in prokaryotes, plants and fungi. Cells of Saccharomyces cerevisiae contain two catalytically redundant DAHP synthases, encoded by the genes ARO3 and ARO4, whose activities are feedback-inhibited by phenylalanine and tyrosine, respectively. ARO3/4 gene transcription is controlled by GCN4. The authors previously cloned an ARO3 gene orthologue from Candida albicans and found that: (1) it can complement an aro3 aro4 double mutation in S. cerevisiae, an effect inhibited by excess phenylalanine, and (2) a homozygous aro3-deletion mutant of C. albicans is phenotypically Aro+, suggesting the existence of another isozyme(s). They now report the identification and functional characterization of the C. albicans orthologue of S. cerevisiae Aro4p. The two Aro4p enzymes share 68% amino acid identity. Phylogenetic analysis places the fungal DAHP synthases in a cluster separate from prokaryotic orthologues and suggests that ARO3 and ARO4 arose from a single gene via a gene duplication event early in fungal evolution. C. albicans ARO4 mRNA is elevated upon amino acid starvation, consistent with the presence of three putative Gcn4p-responsive elements (GCREs) in the gene promoter sequence. C. albicans ARO4 complements an aro3 aro4 double mutation in S. cerevisiae, an effect inhibited by excess tyrosine. The authors engineered Δaro3/Δaro3 Δaro4/MET3p::ARO4 cells of C. albicans (with one wild-type copy of ARO4 placed under control of the repressible MET3 promoter) and found that they fail to grow in the absence of aromatic amino acids when ARO4 expression is repressed, and that this growth defect can be partially rescued by aromatic amino acids and certain aromatic amino acid pathway intermediates. It is concluded that, like S. cerevisiae, C. albicans contains two DAHP synthases required for the first step in the aromatic amino acid biosynthetic pathway.
机译:酶3-脱氧-D-亚溴磺酸盐-7-磷酸盐(DAHP)合成酶催化剂在原核生物,植物和真菌中芳香族氨基酸生物合成的第一步。酿酒酵母细胞含有两个催化冗余的DAHP合成酶,由ARO3和ARO4编码,其活性分别由苯丙氨酸和酪氨酸的反馈抑制。 ARO3 / 4基因转录由GCN4控制。此前提法克隆了来自念珠菌蛋白的ArO3基因正面,发现:(1)它可以补充S.Cerevisiae中的ARO3 ARO4双突变,其抑制过量的苯丙氨酸的效果,以及(2)C的纯合芳烃缺失突变体。albicans是表型aro +,表明存在另一种同工酶。他们现在报告了酿酒酵母ARO4P的C. albicans原序的鉴定和功能表征。两种ARO4P酶共享68%的氨基酸同一性。系统发育分析将真菌DAHP合成酶与原核原子产生分开的簇中,并表明ARO3和ARO4通过在真菌演化中早期通过基因重复事件从单一基因产生。 C. albicans ARO4 mRNA在氨基酸饥饿后升高,与基因启动子序列中的三个推定的GCN4P响应元件(GCRES)一致。 C. albicans ARO4补充了S.Cerevisiae的ARO3 ARO4双突变,其抑制过量的酪氨酸的效果。作者的工程化Δaro3/Δaro3Δar4/ met3p :: aro4细胞的C. albicans(用一个野生型ARO4副本置于可抑制的MET3启动子的控制),发现它们不能在没有芳族氨基酸的情况下生长抑制ARO 4表达,并且可以通过芳族氨基酸和某些芳族氨基酸途径中间体部分地抵抗这种生长缺陷。结论是,与S.Cerevisiae一样,C. albicans含有芳族氨基酸生物合成途径的第一步所需的两种DAHP合成酶。

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