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豆科根瘤菌中fixABC操纵子上游一个新基因fixW的特性及核苷酸序列

Characterization and nucleotide sequence of a novel gene fixW upstream of the fixABC operon in Rhizobium leguminosarum.

作者信息

Hontelez J G, Lankhorst R K, Katinakis P, van den Bos R C, van Kammen A

机构信息

Department of Molecular Biology, Agricultural University, Wageningen, The Netherlands.

出版信息

Mol Gen Genet. 1989 Sep;218(3):536-44. doi: 10.1007/BF00332421.

Abstract

On the Rhizobium leguminosarum PRE sym plasmid, fixABC and a novel gene fixW were identified upstream of the regulatory gene nifA. The molecular masses of FixABC, 29, 44 and 50 kDa respectively, were estimated by polyacrylamide gel electrophoresis (PAGE) and of FixW, 25 kDa, by PAGE and nucleotide sequencing. Hybridization studies using bacteroid mRNA as a probe showed that fixABC is one operon which can be transcribed independently of fixW. Nucleotide sequencing revealed that both fixW and fixA are preceded by a nif consensus promoter. The fixA promoter partly overlaps the 3'-terminal coding region of fixW, indicating that readthrough from fixW into fixA is possible. Two open reading frames, ORF71 and ORF79, precede fixW and form one operon with fixW. ORF71 contains sequences homologous to the fixA promoter and 5'-terminal coding region. One more duplication of fixA sequences was detected, also located within the sym plasmid nif/fix clusters. One duplication of fixW sequences was found. No fixW homologue could be found in other nitrogen fixing organisms except in a number of R. leguminosarum strains.

摘要

在豌豆根瘤菌PRE共生质粒上,在调控基因nifA的上游鉴定出了fixABC和一个新基因fixW。通过聚丙烯酰胺凝胶电泳(PAGE)估计FixABC的分子量分别为29、44和50 kDa,通过PAGE和核苷酸测序估计FixW的分子量为25 kDa。使用类菌体mRNA作为探针的杂交研究表明,fixABC是一个可独立于fixW转录的操纵子。核苷酸测序显示,fixW和fixA之前均有一个nif共有启动子。fixA启动子部分与fixW的3'-末端编码区重叠,这表明从fixW到fixA的通读是可能的。在fixW之前有两个开放阅读框,即ORF71和ORF79,它们与fixW形成一个操纵子。ORF71包含与fixA启动子和5'-末端编码区同源的序列。还检测到fixA序列的另外一次重复,也位于共生质粒的nif/fix簇内。发现了一次fixW序列的重复。除了一些豌豆根瘤菌菌株外,在其他固氮生物中未发现fixW的同源物。

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