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柠檬假单胞菌中的嘧啶核苷酸生物合成与调控。

Pyrimidine Nucleotide Biosynthesis and Regulation in Pseudomonas lemonnieri.

机构信息

Department of Chemistry, Texas A&M University, Commerce, TX, 75429, USA.

出版信息

Curr Microbiol. 2024 Nov 22;82(1):3. doi: 10.1007/s00284-024-03957-6.

DOI:10.1007/s00284-024-03957-6
PMID:39576324
Abstract

The pyrimidine biosynthetic pathway regulation in the bacterium Pseudomonas lemonnieri ATCC 12983 was investigated since this strain synthesizes a blue aromatic pigment that could have a commercial application as a dye. The effect of the pyrimidine bases, orotic acid and uracil metabolites, on the enzymes unique to the pyrimidine biosynthetic pathway was studied. It was found that pyrimidine addition to the medium affected the biosynthetic enzymes differently depending on the carbon source present. Using chemical mutagenesis and 5-fluoroorotic acid resistance, a mutant strain deficient for OMP decarboxylase activity was isolated. The uracil-requiring mutant strain could also utilize cytosine, uridine, or uridine monophosphate as a pyrimidine source. When the mutant strain was limited for pyrimidines for 1 or 2 h, derepression of pyrimidine biosynthetic enzyme activities was observed in the glucose-grown cells but not in the succinate-grown cells. Clearly, carbon source was a factor in the regulation of pyrimidine biosynthesis in P. lemonierri. The regulation of the known regulatory pyrimidine biosynthetic enzyme aspartate transcarbamoylase activity was examined in succinate-grown ATCC 12983 cells, and its activity was controlled by AMP, ADP, GTP, and CTP under saturating substrate concentrations. This study also provides new information as to the taxonomic relatedness of P. lemonnieri to other species classified within the Pseudomonas fluorescens homology group relative to regulation of pyrimidine biosynthesis.

摘要

研究了假单胞菌属柠檬杆菌 ATCC 12983 中嘧啶生物合成途径的调控,因为该菌株合成的蓝色芳香色素可能具有商业应用价值,可用作染料。研究了嘧啶碱基(乳清酸和尿嘧啶代谢物)对嘧啶生物合成途径特有酶的影响。结果发现,嘧啶添加到培养基中会根据存在的碳源而对生物合成酶产生不同的影响。通过化学诱变和 5-氟乳清酸抗性,分离出一种缺乏 OMP 脱羧酶活性的嘧啶缺陷型突变株。需要尿嘧啶的突变株也可以利用胞嘧啶、尿苷或尿苷单磷酸作为嘧啶源。当突变株受到嘧啶限制 1 或 2 小时时,在葡萄糖生长的细胞中观察到嘧啶生物合成酶活性的去阻遏,但在琥珀酸生长的细胞中没有观察到。显然,碳源是柠檬杆菌嘧啶生物合成调节的一个因素。对琥珀酸生长的 ATCC 12983 细胞中已知的调节嘧啶生物合成酶天冬氨酸转氨甲酰酶活性进行了研究,在饱和底物浓度下,其活性受 AMP、ADP、GTP 和 CTP 控制。这项研究还提供了有关柠檬杆菌与假单胞菌荧光素同源群内其他分类群的种间关系以及嘧啶生物合成调节的新信息。

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