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Novel pyoverdine biosynthesis gene(s) of Pseudomonas aeruginosa PAO

机译:Pseudomonas铜绿假单胞菌的新型百倍葡萄酒生物合成基因

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Conjugational mobilization of a Pseudomonas aeruginosa PAO1 cosmid bank (in pMMB33) into a pyoverdine-deficient (pvd) mutant harbouring a mutation in the 47 min region of the chromosome yielded one clone which restored yellow-green pigmentation and fluorescence when grown on iron-deficient medium. The relevant pMMB33-derivative cosmid, pPYP17, contained a 15.1 kb insert which was subcloned into pKT240 as a 10.8 kb Sacl-Clal fragment conferring the same phenotype. This derivative, pPYP180, like pPYP17, also conferred an apparent wild-type phenotype on pvd mutants previously shown to map genetically in the 23 min region of the P. aeruginosa PAO chromosome. Physical mapping indicated that the cloned DNA fragment is located at the 66-70 min region of the PAO chromosome, demonstrating that the restored apparent wild-type phenotype observed for the transconjugants was not the result of a true gene complementation. A gene interruption was obtained by replacing a 0.6 kb Bglll-Bglll region of pPYP180 necessary for the expression of the pigmentation/fluorescence phenotype, by a Hgr interposon (ΩHg). After conjugational transfer and introduction of the mutagenized fragment into the PAO1 chromosome by gene replacement, pyoverdine-deficient mutants were recovered, indicating that the fragment indeed contained at least one gene involved in pyoverdine synthesis. The yellow-green fluorescent compound produced by such cells harbouring plasmids pPYP17 or pPYP180 differed from pyoverdine in several aspects and was consequently named pseudoverdine. Although pseudoverdine was able to complex iron, it was unable to restore growth to pvd mutants in the presence of the iron chelator ethylenediamine di(o-hydroxyphenylacetic acid), or to mediate iron uptake into PAO1. Pseudoverdine lacked a peptide chain but possessed spectral properties similar to pyoverdine, suggesting that it was structurally related to the chromophore of the pyoverdine molecule. The recent structural determination of pseudoverdine as a coumarin derivative confirmed this view and sheds some light on the biosynthetic pathway of the pyoverdine chromophore.
机译:将Pseudomonas Aeruginosa Pao1粘附池(PMMB33)的缀合物动员到含有染色体47分钟区域的易突变的蜂窝状缺陷(PVD)突变体中,在缺铁缺陷时恢复黄绿色素沉着和荧光的克隆中等的。相关的PMMB33衍生物COSMID PPYP17含有15.1kb插入物,其亚克隆到PKT240中,作为赋予相同表型的10.8kb Sacl-clal片段。这种衍生物PPYP180(如PPP717)还赋予了前面显示的PVD突变体的表观野生型表型,以在P.Foruginosa Pao染色体的23分钟区域遗传上映射。物理映射表明,克隆的DNA片段位于Pao染色体的66-70分钟区域,证明了对经杂交剂观察到的恢复表观野生型表型并不是真正基因互补的结果。通过用HGR interposon(ωHg)替换色素沉着/荧光表型表达所需的0.6kb bglll-bgll区域来获得基因中断。通过基因置换置换将诱变片段的结合转移和将诱变片段引入Pao1染色体之后,回收杂散缺陷型突变体,表明该片段确实含有至少一种参与彼多合成的基因。由含有质粒PPYM17或PPYP180的这种细胞产生的黄绿色荧光化合物在几个方面与百多叶片不同,因此被命名为假血症。虽然假血针能够复杂的铁,但在铁螯合剂乙二胺二(O-羟基苯基乙酸)存在下,它无法将生长恢复为PVD突变体,或者将铁吸收成PAO1。假血糖缺乏肽链,但具有与百voverdine类似的光谱性质,表明它与百voverdine分子的发色团结构有关。近期伪转移作为香豆素衍生物的结构测定证实了这种观点,并在百多叶片发色团的生物合成途径上脱落。

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