[Sequencing and analysis of the resistome of Streptomyces fradiae ATCC19609 in order to develop a test system for screening of new antimicrobial agents].

Genetika Pub Date : 2016-06-01
A A Vatlin, O B Bekker, L N Lysenkova, A M Korolev, A E Shchekotikhin, V N Danilenko
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Abstract

The paper provides the annotation and data on sequencing the antibiotic resistance genes in Streptomyces fradiae strain ATCC19609, highly sensitive to different antibiotics. Genome analysis revealed four groups of genes that determined the resistome of the tested strain. These included classical antibiotic resistance genes (nine aminoglycoside phosphotransferase genes, two beta-lactamase genes, and the genes of puromycin N-acetyltransferase, phosphinothricin N-acetyltransferase, and aminoglycoside acetyltransferase); the genes of ATP-dependent ABC transporters, involved in the efflux of antibiotics from the cell (MacB-2, BcrA, two-subunit MDR1); the genes of positive and negative regulation of transcription (whiB and padR families); and the genes of post-translational modification (serine-threonine protein kinases). A comparative characteristic of aminoglycoside phosphotransferase genes in S. fradiae ATCC19609, S. lividans TK24, and S. albus J1074, the causative agent of actinomycosis, is provided. The possibility of using the S. fradiae strain ATCC19609 as the test system for selection of the macrolide antibiotic oligomycin A derivatives with different levels of activity is demonstrated. Analysis of more than 20 semisynthetic oligomycin A derivatives made it possible to divide them into three groups according to the level of activity: inactive (>1 nmol/disk), 10 substances; with medium activity level (0.05–1 nmol/disk), 12 substances; and more active (0.01–0.05 nmol/disk), 2 substances. Important for the activity of semisynthetic derivatives is the change in the position of the 33rd carbon atom in the oligomycin A molecule.

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[对传统链霉菌ATCC19609的抗性组进行测序和分析,以开发新的抗菌药物筛选测试系统]。
本文提供了对不同抗生素高度敏感的链霉菌ATCC19609菌株耐药基因的注释和测序数据。基因组分析显示,四组基因决定了测试菌株的抗性组。其中包括经典的抗生素耐药基因(9个氨基糖苷磷酸转移酶基因,2个β -内酰胺酶基因,以及嘌呤霉素n -乙酰转移酶、膦-丙氨酸n -乙酰转移酶和氨基糖苷乙酰转移酶基因);atp依赖性ABC转运蛋白基因,参与抗生素从细胞外排(MacB-2、BcrA、双亚基MDR1);转录正调控基因和负调控基因(whb和padR家族);以及翻译后修饰基因(丝氨酸-苏氨酸蛋白激酶)。提供了放线菌病病原菌S. fradiae ATCC19609、S. lividans TK24和S. albus J1074中氨基糖苷磷酸转移酶基因的比较特征。证明了利用S. fradiae菌株ATCC19609作为测试系统选择不同活性水平的大环内酯类抗生素寡霉素A衍生物的可能性。对20多种半合成寡霉素A衍生物进行分析,根据活性水平将其分为三组:无活性(>1 nmol/盘),10种物质;中等活性水平(0.05-1 nmol/盘),12种物质;活性较高(0.01 ~ 0.05 nmol/盘),2种物质。对半合成衍生物活性的重要影响是寡霉素A分子中第33个碳原子位置的变化。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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