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Molecular analysis of Mycobacterium tuberculosis DNA from a family of 18th century Hungarians

机译:18世纪匈牙利人家庭分枝杆菌DNA的分子分析

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The naturally mummified remains of a mother and two daughters found in an 18th century Hungarian crypt were analysed, using multiple molecular genetic techniques to examine the epidemiology and evolution of tuberculosis. DNA was amplified from a number of targets on the Mycobacterium tuberculosis genome, including DNA from IS6110, gyrA, katG codon 463, oxyR, dnaA–dnaN, mtp40, plcD and the direct repeat (DR) region. The strains present in the mummified remains were identified as M. tuberculosis and not Mycobacterium bovis, from katG and gyrA genotyping, PCR from the oxyR and mtp40 loci, and spoligotyping. Spoligotyping divided the samples into two strain types, and screening for a deletion in the MT1801–plcD region initially divided the strains into three types. Further investigation showed, however, that an apparent deletion was due to poor DNA preservation. By comparing the effect of PCR target size on the yield of amplicon, a clear difference was shown between 18th century and modern M. tuberculosis DNA. A two-centre system was used to confirm the findings of this study, which clearly demonstrate the value of using molecular genetic techniques to study historical cases of tuberculosis and the care required in drawing conclusions. The genotyping and spoligotyping results are consistent with the most recent theory of the evolution and spread of the modern tuberculosis epidemic.
机译:通过多种分子遗传技术分析了在18世纪的匈牙利地区发现的母亲和两个女儿的自然留下的遗体,以检查结核病的流行病学和演化。从结核分枝杆菌基因组的许多靶标扩增DNA,包括来自IS6110,Gyra,Katg密码子463,Oxyr,DNA-DNA,MTP40,PLCD和直接重复(DR)区域的DNA。在Mumbified遗体中存在的菌株被鉴定为M.结核病,而不是肉毒杆菌,来自奥克斯和奥克斯和MTP40基因座的PCR和Spoligotyping。 SpoliGotyping将样品分为两个应变类型,并在MT1801-PLCD区域中筛选缺失最初将菌株分成三种类型。然而,进一步的研究表明,表观缺失是由于DNA保存不良。通过比较PCR靶尺寸对扩增子产率的影响,18世纪与现代M.结核病DNA之间显示出明显差异。使用双中心系统来确认本研究的结果,该研究表明,清楚地证明了使用分子遗传技术研究历史结核病患者和绘制结论中所需的护理。基因分型和香料型结果与现代结核病流行病的进化和传播的最新理论一致。

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