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ndvF是位于苜蓿根瘤菌大质粒pRmeSU47b(pEXO)上的一个新基因座,是正常根瘤发育所必需的。

ndvF, a novel locus located on megaplasmid pRmeSU47b (pEXO) of Rhizobium meliloti, is required for normal nodule development.

作者信息

Charles T C, Newcomb W, Finan T M

机构信息

Department of Biology, McMaster University, Hamilton, Ontario, Canada.

出版信息

J Bacteriol. 1991 Jul;173(13):3981-92. doi: 10.1128/jb.173.13.3981-3992.1991.

Abstract

Rhizobium meliloti strains carrying either of two overlapping deletions (delta 5408 and delta F114) of the megaplasmid pRmeSU47b form nodules on alfalfa which fail to fix N2 (Fix-). Strains carrying these deletions also fail to fluoresce on media containing calcofluor, indicating a defect in synthesis of the acidic exopolysaccharide (Exo-) of R. meliloti. We have isolated cosmid clones (pTH21 and pTH22) which complement the Fix- but not the Exo- phenotype of the strains carrying the delta 5408 and delta F114 deletions. In addition, cosmid clones which complement the Exo- phenotype fail to complement the Fix- phenotype of these deletions; thus, the Exo- phenotype is not related to the Fix- phenotype. A 5-kb region within a 7.3-kb BamHI restriction fragment was found to be required for complementation of the Fix- phenotype of the delta 5408 and delta F114 deletion strains. Tn5 insertions in the 5-kb region generated a Fix- phenotype when recombined into the wild-type genome. We have designated this locus ndvF, for nodule development. TnphoA mutagenesis of this region generated active alkaline-phosphatase gene fusions, indicating that ndvF encodes extracytoplasmic protein(s). Induction of nodules by the ndvF mutants was delayed by 2 to 3 days compared with induction by the wild-type strain. Light microscopy of nodules elicited by strains carrying the large 150-kb delta F114 deletion, a 12-kb deletion removing ndvF, or an individual ndvF::Tn5 insertion mutation demonstrated that many nodules contained few infected cortical cells, indicating that nodule development was blocked early in the infection process, before the release of bacteria from the infection threads.

摘要

携带苜蓿中华根瘤菌(Rhizobium meliloti)大质粒pRmeSU47b两个重叠缺失片段(δ5408和δF114)之一的菌株能在苜蓿上形成根瘤,但不能固氮(Fix-)。携带这些缺失片段的菌株在含有荧光增白剂的培养基上也不能产生荧光,这表明苜蓿中华根瘤菌酸性胞外多糖(Exo-)的合成存在缺陷。我们分离到了黏粒克隆(pTH21和pTH22),它们能互补携带δ5408和δF114缺失片段菌株的Fix-表型,但不能互补其Exo-表型。此外,能互补Exo-表型的黏粒克隆不能互补这些缺失片段的Fix-表型;因此,Exo-表型与Fix-表型无关。在一个7.3 kb的BamHI限制性片段内发现一个5 kb的区域是互补δ5408和δF114缺失菌株Fix-表型所必需的。当重组到野生型基因组中时,5 kb区域内的Tn5插入产生了Fix-表型。我们将这个位点命名为ndvF,即根瘤发育相关基因。该区域的TnphoA诱变产生了活性碱性磷酸酶基因融合体,表明ndvF编码胞外蛋白。与野生型菌株诱导相比,ndvF突变体诱导根瘤的时间延迟了2至3天。对携带150 kb大δF114缺失片段、去除ndvF的12 kb缺失片段或单个ndvF::Tn5插入突变的菌株所诱导的根瘤进行光学显微镜观察发现,许多根瘤中感染的皮层细胞很少,这表明根瘤发育在感染过程早期被阻断,即在细菌从感染丝中释放之前。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/de4a/208044/2978241a0ef6/jbacter00103-0062-a.jpg

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