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环状芽孢杆菌耐万古霉素临床分离株中的vanA基因簇。

vanA gene cluster in a vancomycin-resistant clinical isolate of Bacillus circulans.

作者信息

Ligozzi M, Lo Cascio G, Fontana R

机构信息

Istituto di Microbiologia, Università di Verona, Strada Le Grazie 8, 37100 Verona, Italy.

出版信息

Antimicrob Agents Chemother. 1998 Aug;42(8):2055-9. doi: 10.1128/AAC.42.8.2055.

Abstract

We report on the cloning and sequencing of the vanA gene cluster present in the glycopeptide-resistant clinical isolate Bacillus circulans VR0709 (R. Fontana, M. Ligozzi, C. Pedrotti, E. M. Padovani, and G. Cornaglia, Eur. J. Clin. Microbiol. Infect. Dis. 16:473-474, 1997). The presence of a vanA-related gene in VR0709 was demonstrated in a PCR assay which permitted the specific amplification of an internal segment of vanA. Southern blotting suggested that the vanA gene was located in the chromosome in a 7. 6-kb EcoRI fragment. DNA sequence analysis revealed the presence of all seven genes of the vanA cluster (vanR, vanS, vanH, vanA, vanX, vanY, and vanZ). The degree of identity between homologous proteins encoded by Tn1546 and the chromosome of B. circulans VR0709 ranged from 87 to 95%. Neither PCR nor Southern blotting with specific primers and probes, respectively, showed the presence of open reading frames (ORFs) 1 and 2 which encode the transposase and the resolvase of Tn1546, respectively, the transposon found to carry the vanA gene cluster in enterococci. Determination of the sequences of the flanking regions of the van gene cluster of B. circulans revealed perfect inverted repeats of 10 bp which delineated a 9.2-kb region containing the van gene cluster and an ORF which encoded a putative protein (178 residues) which displayed a low level of identity (28%) to the resolvase of Tn1546. These results suggest that glycopeptide resistance in B. circulans VR0709 is associated with the acquisition of a vanA gene cluster which shows a high degree of homology with that of enterococci. In B. circulans, however, the cluster is not carried by Tn1546 and is borne by the chromosome.

摘要

我们报道了存在于耐糖肽临床分离株环状芽孢杆菌VR0709中的vanA基因簇的克隆和测序情况(R. 丰塔纳、M. 利戈齐、C. 佩德罗蒂、E. M. 帕多瓦尼和G. 科尔纳利亚,《欧洲临床微生物学与感染疾病杂志》16:473 - 474,1997年)。在PCR检测中证实了VR0709中存在一个与vanA相关的基因,该检测能够特异性扩增vanA的一个内部片段。Southern印迹分析表明vanA基因位于染色体的一个7.6 kb的EcoRI片段中。DNA序列分析揭示了vanA基因簇的所有七个基因(vanR、vanS、vanH、vanA、vanX、vanY和vanZ)的存在。由Tn1546编码的同源蛋白与环状芽孢杆菌VR0709染色体之间的同一性程度在87%至95%之间。分别用特异性引物和探针进行的PCR和Southern印迹分析均未显示出开放阅读框(ORF)1和2的存在,这两个开放阅读框分别编码Tn1546的转座酶和解离酶,Tn1546是在肠球菌中发现携带vanA基因簇的转座子。对环状芽孢杆菌van基因簇侧翼区域序列的测定揭示了10 bp的完美反向重复序列,这些序列界定了一个包含van基因簇的9.2 kb区域以及一个编码推定蛋白(178个残基)的开放阅读框,该推定蛋白与Tn1546的解离酶显示出低水平的同一性(28%)。这些结果表明,环状芽孢杆菌VR0709中的糖肽抗性与获得一个与肠球菌的vanA基因簇具有高度同源性的vanA基因簇有关。然而,在环状芽孢杆菌中,该基因簇不是由Tn1546携带,而是由染色体携带。

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