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首页> 外文期刊>Journal of Clinical Microbiology >Evaluation of a Low-Density Hydrogel Microarray Technique for Mycobacterial Species Identification
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Evaluation of a Low-Density Hydrogel Microarray Technique for Mycobacterial Species Identification

机译:低密度水凝胶微阵列技术鉴定分枝杆菌种类的评估

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In addition to the obligatory pathogenic species of the Mycobacterium tuberculosis complex and Mycobacterium leprae, the genus Mycobacterium also includes conditionally pathogenic species that in rare cases can lead to the development of nontuberculous mycobacterial diseases. Because tuberculosis and mycobacteriosis have similar clinical signs, the accurate identification of the causative agent in a clinical microbiology laboratory is important for diagnostic verification and appropriate treatment. This report describes a low-density hydrogel-based microarray containing oligonucleotide probes based on the species-specific sequences of the gyrB gene fragment for mycobacterial species identification. The procedure included the amplification of a 352-nucleotide fragment of the gene and its hybridization on a microarray. The triple-species-specific probe design and the algorithm for hybridization profile recognition based on the calculation of Pearson correlation coefficients, followed by the construction of a profile database, allowed for the reliable and accurate identification of mycobacterial species, including mixed-DNA samples. The assay was used to evaluate 543 clinical isolates from two regions of Russia, demonstrating its ability to detect 35 mycobacterial species, with 99.8% sensitivity and 100% specificity when using gyrB, 16S, and internal transcribed spacer (ITS) fragment sequencing as the standard. The testing of clinical samples showed that the sensitivity of the assay was 89% to 95% for smear-positive samples and 36% for smear-negative samples. The large number of identified species, the high level of sensitivity, the ability to detect mycobacteria in clinical samples, and the up-to-date profile database make the assay suitable for use in routine laboratory practice.
机译:除结核分枝杆菌复合体和麻风分枝杆菌的强制性致病物种外,分枝杆菌属还包括有条件的致病物种,在极少数情况下可导致非结核性分枝杆菌疾病的发展。由于结核病和分枝杆菌病具有相似的临床症状,因此在临床微生物学实验室中准确确定病原体对于诊断验证和适当治疗很重要。本报告介绍了一种基于寡核苷酸探针的低密度水凝胶微阵列,该探针基于用于鉴定分枝杆菌物种的 gyrB 基因片段的物种特异性序列。该程序包括该基因的352个核苷酸片段的扩增及其在微阵列上的杂交。基于皮尔逊相关系数的计算的特定于三物种的探针设计和杂交图谱识别算法,然后建立一个图谱数据库,可以可靠,准确地鉴定分枝杆菌物种,包括混合DNA样品。该方法用于评估来自俄罗斯两个地区的543株临床分离株,证明了使用 gyrB ,16S和内部转录间隔子检测35种分枝杆菌的能力,灵敏度为99.8%,特异性为100%( ITS)片段测序为标准。临床样品测试表明,涂片阳性样品的测定灵敏度为89%至95%,涂片阴性样品的测定灵敏度为36%。鉴定出的物种数量众多,灵敏度高,临床样品中分枝杆菌的检测能力以及最新的资料数据库使该测定法适合常规实验室实践。

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