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Cloning, Sequencing, and Characterization of thecgmB Gene of Sinorhizobium meliloti Involved in Cyclic β-Glucan Biosynthesis

机译:苜蓿根瘤菌参与循环β-葡聚糖生物合成的cgmB基因的克隆,测序与鉴定

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Periplasmic cyclic β-glucans of Rhizobium species provide important functions during plant infection and hypo-osmotic adaptation. In Sinorhizobium meliloti (also known asRhizobium meliloti), these molecules are highly modified with phosphoglycerol and succinyl substituents. We have previously identified an S. meliloti Tn5 insertion mutant, S9, which is specifically impaired in its ability to transfer phosphoglycerol substituents to the cyclic β-glucan backbone (M. W. Breedveld, J. A. Hadley, and K. J. Miller, J. Bacteriol. 177:6346–6351, 1995). In the present study, we have cloned, sequenced, and characterized this mutation at the molecular level. By using the Tn5 flanking sequences (amplified by inverse PCR) as a probe, an S. meliloti genomic library was screened, and two overlapping cosmid clones which functionally complement S9 were isolated. A 3.1-kb HindIII-EcoRI fragment found in both cosmids was shown to fully complement mutant S9. Furthermore, when a plasmid containing this 3.1-kb fragment was used to transformRhizobium leguminosarum bv. trifolii TA-1JH, a strain which normally synthesizes only neutral cyclic β-glucans, anionic glucans containing phosphoglycerol substituents were produced, consistent with the functional expression of an S. meliloti phosphoglycerol transferase gene. Sequence analysis revealed the presence of two major, overlapping open reading frames within the 3.1-kb fragment. Primer extension analysis revealed that one of these open reading frames, ORF1, was transcribed and its transcription was osmotically regulated. This novel locus of S. meliloti is designated thecgm (cyclic glucan modification) locus, and the product encoded by ORF1 is referred to as CgmB.
机译:根瘤菌种的周质环β-葡聚糖在植物感染和低渗适应过程中发挥重要作用。在(也称为 Rhizobium meliloti )中,这些分子被磷酸甘油和琥珀酰取代基高度修饰。我们之前已经确定了 S。 meliloti Tn 5 插入突变体S9,其将磷酸甘油取代基转移至环状β-葡聚糖骨架的能力特别受损(MW Breedveld,JA Hadley,and KJ Miller,J.细菌学杂志177:6346-6351,1995)。在本研究中,我们已经在分子水平上克隆,测序和表征了该突变。通过使用Tn 5 侧翼序列(通过反向PCR扩增)作为探针,形成 S。筛选了meliloti 基因组文库,并分离了两个重叠的功能互补S9的粘粒克隆。在两个粘粒中发现的一个3.1-kb的 Hin dIII- Eco RI片段显示出与突变体S9完全互补。此外,当使用含有该3.1kb片段的质粒转化豆科植物根瘤菌bv时。 trifolii TA-1JH,通常仅合成中性环状β-葡聚糖的菌株,产生了含有磷酸甘油取代基的阴离子葡聚糖,与 S的功能表达一致。 meliloti 磷酸甘油转移酶基因序列分析显示在3.1kb片段中存在两个主要的,重叠的开放阅读框。引物延伸分析表明,其中一个开放阅读框ORF1被转录且其转录受渗透调节。 S的这个新颖的地方meliloti 被指定为 cgm (环状葡聚糖修饰)基因座,ORF1编码的产物称为CgmB。

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