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Revisiting Pneumococcal Carriage by Use of Broth Enrichment and PCR Techniques for Enhanced Detection of Carriage and Serotypes▿

机译:通过肉汤富集和PCR技术重温肺炎球菌的运输,以增强对运输和血清型的检测▿

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摘要

The measurement of pneumococcal carriage in the nasopharyngeal reservoir is subject to potential confounders that include low-density and multiple-strain colonization. To compare different methodologies, we picked a random sampling of 100 nasopharyngeal specimens recovered from infants less than 2 years of age who were previously assessed for pneumococcal carriage and serotypes by a conventional method that used direct plating from the transport/storage medium (50 specimens were culture negative and 50 specimens were culture positive for pneumococci). We used a broth enrichment approach and a conventional PCR approach (with and without broth enrichment) to determine pneumococcal carriage and serotypes, and the results were compared to the initial conventional culture-based results. Additionally, we used a lytA-targeted real-time PCR for pneumococcal detection. Broth enrichment for both the culture-based and the PCR-based methods enhanced the isolation of pneumococci and detection of serotype diversity, with the most effective serotype deduction method being one that used broth enrichment prior to sequential multiplex PCR. Similarly, we also found that broth enrichment followed by the lytA-specific real-time PCR was the most sensitive for the detection of apparent pneumococcal carriage. The broth enrichment, conventional multiplex PCR, and real-time PCR approaches used in this study were effective in detecting pneumococcal carriage in the 50 specimens that were negative by conventional direct plating from transport medium (range of numbers of positive specimens, 8/50 to 22/50 [16 to 44%]), and the three different serotyping approaches that used broth enrichment increased the number of serotype identifications from the 100 specimens (12 to 29 additional serotype identifications to be positive). A PCR-based approach that employed a broth enrichment step appeared to best enhance the detection of mixed serotypes and low-density pneumococcal carriage.
机译:鼻咽水库中肺炎球菌携带的测量受到潜在混杂因素的影响,包括低密度和多菌株定植。为了比较不同的方法,我们随机抽取了100例从2岁以下的婴儿中回收的鼻咽标本,这些标本以前通过常规方法从运输/存储介质中进行了直接平板接种,从而评估了肺炎球菌的携带和血清型(50例标本培养阴性,有50个标本为肺炎球菌培养阳性。我们使用肉汤富集方法和常规PCR方法(有或没有肉汤富集)来确定肺炎球菌的携带和血清型,并将结果与​​基于常规培养的初始结果进行比较。此外,我们使用针对lytA的实时PCR进行肺炎球菌检测。用于基于培养物和基于PCR的方法的肉汤富集可增强肺炎链球菌的分离和血清型多样性的检测,最有效的血清型推导方法是在顺序多重PCR之前使用肉汤富集的一种方法。同样,我们还发现,富集肉汤,然后进行lytA特异性实时PCR对表观肺炎球菌携带的检测最敏感。本研究中使用的肉汤富集,常规多重PCR和实时PCR方法可有效地检测50份标本中的肺炎球菌携带,这些标本是通过常规直接从运输培养基直接铺板而阴性的(阳性标本数量范围为8/50至50)。 22/50 [16至44%]),使用肉汤富集的三种不同的血清分型方法增加了100个标本中血清型鉴定的数量(另外12到29种血清型鉴定为阳性)。一种采用肉汤富集步骤的基于PCR的方法似乎可以最好地增强对混合血清型和低密度肺炎球菌携带的检测。

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