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鼠伤寒沙门氏菌LT2拥有三个不同的23S核糖体RNA间隔序列。

Salmonella typhimurium LT2 possesses three distinct 23S rRNA intervening sequences.

作者信息

Mattatall N R, Sanderson K E

机构信息

Salmonella Genetic Stock Centre, Uniersity of Calgary, Alberta, Canada.

出版信息

J Bacteriol. 1996 Apr;178(8):2272-8. doi: 10.1128/jb.178.8.2272-2278.1996.

Abstract

The rrl genes for 23S rRNA of Salmonella typhimurium LT2 are known to carry intervening sequences (IVSs) at two sites, helix-25 and helix-45, which are excised by RNase III during rRNA maturation, resulting in rRNA which is fragmented but nevertheless functional. We isolated DNA fragments containing the seven rrl genes from BlnI, I-CeuI, and SpeI genomic digests following pulsed-field gel electrophoresis and used these DNA fragments as templates for PCRs utilizing primers upstream and downstream of helix-25 and helix-45. Variance in amplicon length and cycle sequencing indicated that rrlG and rrlH have IVSs in helix-25 of approximately 110 bp which are only 56% identical. rrnA, rrnB, rrnC, rrnD, rrnE, and rrnH have IVSs of approximately 90 bp in helix-45, and all have the same nucleotide sequence. Twenty-one independent wild-type strains of S. typhimurium from Salmonella Reference Collection A were analyzed for IVSs by using PCRs with genomic DNAs and by denaturing agarose electrophoresis of RNAs. Many strains resemble LT2, but some have no IVSs in helix-25 and others have IVSs in helix-45 in all seven rrl genes. However, the IVSs in individual wild-type lines are relatively stable, for several LT2 isolates separated over many years by many single-colony isolations are indistinguishable from one another, with the exception of line LB5010, which differs by one helix-25 IVS. We postulate that IVSs have entered strain LT2 by three independent lateral-transfer events and that the IVS in helix-45 was dispersed to and maintained in the same sequence in six of the seven rrl genes by the mechanism of gene conversion.

摘要

已知鼠伤寒沙门氏菌LT2的23S rRNA的rrl基因在两个位点(螺旋-25和螺旋-45)带有间隔序列(IVS),这些间隔序列在rRNA成熟过程中被RNase III切除,产生的rRNA虽有片段但仍有功能。我们通过脉冲场凝胶电泳从BlnI、I-CeuI和SpeI基因组消化物中分离出包含七个rrl基因的DNA片段,并将这些DNA片段用作PCR模板,使用螺旋-25和螺旋-45上下游的引物。扩增子长度和循环测序的差异表明,rrlG和rrlH在螺旋-25中有大约110 bp的IVS,它们的同一性仅为56%。rrnA、rrnB、rrnC、rrnD、rrnE和rrnH在螺旋-45中有大约90 bp的IVS,并且它们都具有相同的核苷酸序列。我们使用基因组DNA进行PCR并通过RNA的变性琼脂糖电泳,对来自沙门氏菌参考菌株A的21个独立野生型鼠伤寒沙门氏菌菌株进行了IVS分析。许多菌株与LT2相似,但有些菌株在螺旋-25中没有IVS,而其他菌株在所有七个rrl基因的螺旋-45中都有IVS。然而,单个野生型品系中的IVS相对稳定,因为通过多次单菌落分离在多年间分离的几个LT2分离株彼此无法区分,但品系LB5010除外,它在一个螺旋-25 IVS上有所不同。我们推测IVS通过三个独立的横向转移事件进入LT2菌株,并且螺旋-45中的IVS通过基因转换机制分散到七个rrl基因中的六个基因中并以相同序列维持。

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