首页> 外文OA文献 >Complete Nucleotide Sequence of the 113-Kilobase Linear Catabolic Plasmid pAL1 of Arthrobacter nitroguajacolicus Rü61a and Transcriptional Analysis of Genes Involved in Quinaldine Degradation▿ †
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Complete Nucleotide Sequence of the 113-Kilobase Linear Catabolic Plasmid pAL1 of Arthrobacter nitroguajacolicus Rü61a and Transcriptional Analysis of Genes Involved in Quinaldine Degradation▿ †

机译:硝基拟南芥Rü61a细菌的113碱基线性分解代谢质粒pAL1的完整核苷酸序列和涉及喹诺定降解的基因的转录分析▿†

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摘要

The nucleotide sequence of the linear catabolic plasmid pAL1 from the 2-methylquinoline (quinaldine)-degrading strain Arthrobacter nitroguajacolicus Rü61a comprises 112,992 bp. A total of 103 open reading frames (ORFs) were identified on pAL1, 49 of which had no annotatable function. The ORFs were assigned to the following functional groups: (i) catabolism of quinaldine and anthranilate, (ii) conjugation, and (iii) plasmid maintenance and DNA replication and repair. The genes for conversion of quinaldine to anthranilate are organized in two operons that include ORFs presumed to code for proteins involved in assembly of the quinaldine-4-oxidase holoenzyme, namely, a MobA-like putative molybdopterin cytosine dinucleotide synthase and an XdhC-like protein that could be required for insertion of the molybdenum cofactor. Genes possibly coding for enzymes involved in anthranilate degradation via 2-aminobenzoyl coenzyme A form another operon. These operons were expressed when cells were grown on quinaldine or on aromatic compounds downstream in the catabolic pathway. Single-stranded 3′ overhangs of putative replication intermediates of pAL1 were predicted to form elaborate secondary structures due to palindromic and superpalindromic terminal sequences; however, the two telomeres appear to form different structures. Sequence analysis of ORFs 101 to 103 suggested that pAL1 codes for one or two putative terminal proteins, presumed to be covalently bound to the 5′ termini, and a multidomain telomere-associated protein (Tap) comprising 1,707 amino acids. Even if the putative proteins encoded by ORFs 101 to 103 share motifs with the Tap and terminal proteins involved in telomere patching of Streptomyces linear replicons, their overall sequences and domain structures differ significantly.
机译:降解2-甲基喹啉(喹诺定)的菌株硝基古菌Rü61a的线性分解代谢质粒pAL1的核苷酸序列包含112,992 bp。在pAL1上总共鉴定出103个开放阅读框(ORF),其中49个没有注释功能。 ORF被分配给以下功能组:(i)奎奴定和邻氨基苯甲酸的分解代谢,(ii)缀合,和(iii)质粒维持以及DNA复制和修复。喹诺定转化为邻氨基苯甲酸的基因组织在两个操纵子中,其中包括推测为编码参与奎纳丁-4-氧化酶全酶装配的蛋白质的ORF,即MobA样推定的钼蝶呤胞嘧啶二核苷酸合酶和XdhC样蛋白。可能需要插入钼辅助因子。可能编码通过2-氨基苯甲酰辅酶A参与邻氨基苯甲酸酯降解的酶的基因形成另一个操纵子。当细胞在喹诺定或分解代谢途径下游的芳族化合物上生长时,这些操纵子得以表达。预测由于回文和超回文末端序列,pAL1的假定复制中间体的单链3'突出端会形成复杂的二级结构。然而,两个端粒似乎形成不同的结构。 ORF 101至103的序列分析表明,pAL1编码一个或两个假定的末端蛋白(假定与5'末端共价结合),以及一个包含1,707个氨基酸的多域端粒相关蛋白(Tap)。即使由ORF 101至103编码的推定蛋白质与涉及链霉菌线性复制子的端粒修补的Tap和末端蛋白质共享基序,它们的整体序列和域结构也明显不同。

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