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首页> 外文期刊>Journal of Clinical Microbiology >Reliable Means of Diagnosis and Serovar Determination of Blood-Borne Salmonella Strains: Quick PCR Amplification of Unique Genomic Loci by Novel Primer Sets
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Reliable Means of Diagnosis and Serovar Determination of Blood-Borne Salmonella Strains: Quick PCR Amplification of Unique Genomic Loci by Novel Primer Sets

机译:诊断和血清型沙门氏菌血清学测定的可靠手段:独特的基因组位点的新型引物集的快速PCR扩增。

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Typhoid fever is becoming an ever increasing threat in the developing countries. We have improved considerably upon the existing PCR-based diagnosis method by designing primers against a region that is unique to Salmonella enterica subsp. enterica serovar Typhi and Salmonella enterica subsp. enterica serovar Paratyphi A, corresponding to the STY0312 gene in S. Typhi and its homolog SPA2476 in S. Paratyphi A. An additional set of primers amplify another region in S. Typhi CT18 and S. Typhi Ty2 corresponding to the region between genes STY0313 to STY0316 but which is absent in S. Paratyphi A. The possibility of a false-negative result arising due to mutation in hypervariable genes has been reduced by targeting a gene unique to typhoidal Salmonella serovars as a diagnostic marker. The amplified region has been tested for genomic stability by amplifying the region from clinical isolates of patients from various geographical locations in India, thereby showing that this region is potentially stable. These set of primers can also differentiate between S. Typhi CT18, S. Typhi Ty2, and S. Paratyphi A, which have stable deletions in this specific locus. The PCR assay designed in this study has a sensitivity of 95% compared to the Widal test which has a sensitivity of only 63%. As observed, in certain cases, the PCR assay was more sensitive than the blood culture test was, as the PCR-based detection could also detect dead bacteria.
机译:伤寒已成为发展中国家日益严重的威胁。通过设计针对沙门氏菌亚种独特区域的引物,我们在现有基于PCR的诊断方法上有了很大的改进。 enterica 血清型Typhi和 Salmonella enterica 子亚种。 enterica 血清副伤寒A,对应于 S 中的STY0312基因。在 S 中的Typhi及其同系物SPA2476。副伤寒A.另一组引物可扩增 S 中的另一个区域。 Typhi CT18和 S 。 Typhi Ty2对应于基因STY0313至STY0316之间的区域,但在 S 中不存在。副伤寒A.通过靶向伤寒沙门氏菌血清型独特基因作为诊断标记物,减少了因高变基因突变而导致假阴性结果的可能性。通过从印度各个地理位置的患者的临床分离株中扩增出的区域,对扩增区域进行了基因组稳定性测试,从而表明该区域具有潜在的稳定性。这些引物组也可以区分 S 。 Typhi CT18, S 。 Typhi Ty2和 S 。副伤寒A,在此特定基因座具有稳定的缺失。与Widal测试相比,这项研究中设计的PCR分析的灵敏度为95%,而Widal测试的灵敏度仅为63%。如所观察到的,在某些情况下,PCR分析比血液培养测试更为灵敏,因为基于PCR的检测还可以检测到死菌。

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