Evaluation and Improvement of Real-Time PCR Assays Targeting lytA, ply, and psaA Genes for Detection of Pneumococcal DNA

Maria da Gloria S. Carvalho; Maria Lucia Tondella; Karen McCaustland; Luciana Weidlich; Lesley McGee; Leonard W. Mayer; Arnold Steigerwalt; Melissa Whaley; Richard R. Facklam; Barry Fields; George Carlone; Edwin W. Ades; Ron Dagan; Jacquelyn S. Sampson

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Evaluation and Improvement of Real-Time PCR Assays Targeting lytA, ply, and psaA Genes for Detection of Pneumococcal DNA

机译：评价和改进靶向lytA，ply和psaA基因检测肺炎球菌DNA的实时PCR方法

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The accurate diagnosis of pneumococcal disease has frequently been hampered not only by the difficulties in obtaining isolates of the organism from patient specimens but also by the misidentification of pneumococcus-like viridans group streptococci (P-LVS) as Streptococcus pneumoniae. This is especially critical when the specimen comes from the respiratory tract. In this study, three novel real-time PCR assays designed for the detection of specific sequence regions of the lytA, ply, and psaA genes were developed (lytA-CDC, ply-CDC, and psaA, respectively). These assays showed high sensitivity (<10 copies for lytA-CDC and ply-CDC and an approximately twofold less sensitivity for psaA). Two additional real-time PCR assays for lytA and ply described previously for pneumococcal DNA detection were also evaluated. A panel of isolates consisting of 67 S. pneumoniae isolates (44 different serotypes and 3 nonencapsulated S. pneumoniae isolates from conjunctivitis outbreaks) and 104 nonpneumococcal isolates was used. The 67 S. pneumoniae isolates were reactive in all five assays. The new real-time detection assays targeting the lytA and psaA genes were the most specific for the detection of isolates confirmed to be S. pneumoniae, with lytA-CDC showing the greatest specificity. Both ply PCRs were positive for all isolates of S. pseudopneumoniae, along with 13 other isolates of other P-LVS isolates confirmed to be non-S. pneumoniae by DNA-DNA reassociation. Thus, the use of the ply gene for the detection of pneumococci can lead to false-positive reactions in the presence of P-LVS. The five assays were applied to 15 culture-positive cerebrospinal fluid specimens with 100% sensitivity; and serum and ear fluid specimens were also evaluated. Both the lytA-CDC and psaA assays, particularly the lytA-CDC assay, have improved specificities compared with those of currently available assays and should therefore be considered the assays of choice for the detection of pneumococcal DNA, particularly when upper respiratory P-LVS might be present in the clinical specimen.

机译：肺炎球菌疾病的准确诊断经常受到阻碍，不仅因为难以从患者标本中分离出病原体，而且由于将肺炎球菌样绿菌素类链球菌（P-LVS）误识别为肺炎链球菌 >。当标本来自呼吸道时，这一点尤其重要。在这项研究中，设计了用于检测 lytA ， ply 和 psaA 基因特定序列区域的三种新型实时PCR检测方法开发（分别是 lytA -CDC， ply -CDC和 psaA ）。这些测定法显示出高灵敏度（ lytA -CDC和 ply -CDC <10个拷贝，而 psaA 的敏感性低约两倍）。还评估了另外两个针对肺炎球菌DNA检测的 lytA 和 ply 实时荧光定量PCR检测方法。一组由67个 S组成的分离株。分别使用了44种不同的血清型和3种非包膜的结膜炎暴发性肺炎链球菌分离株和104种非肺炎球菌分离株。 67 S。肺炎分离株在所有五个测定中均具有反应性。针对 lytA 和 psaA 基因的新型实时检测方法对于检测被确认为 S的分离株而言是最特异性的。肺炎，其中 lytA -CDC表现出最大的特异性。两种 ply PCR均对所有 S分离株呈阳性。假性肺炎，以及其他13个其他P-LVS分离株的分离株，证实是非 S。 DNA-DNA重组产生肺炎。因此，在P-LVS存在下，使用 ply 基因检测肺炎链球菌会导致假阳性反应。这五个测定法以15％的敏感性应用于15个培养阳性的脑脊液标本。还评估了血清和耳液样本。与目前可用的测定法相比， lytA -CDC法和 psaA 法（尤其是 lytA -CDC法）均具有更高的特异性，因此，被认为是检测肺炎球菌DNA的首选检测方法，尤其是当临床标本中可能存在上呼吸道P-LVS时。 展开▼

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《Journal of Clinical Microbiology》 |2007年第8期|共7页

作者
Maria da Gloria S. Carvalho; Maria Lucia Tondella; Karen McCaustland; Luciana Weidlich; Lesley McGee; Leonard W. Mayer; Arnold Steigerwalt; Melissa Whaley; Richard R. Facklam; Barry Fields; George Carlone; Edwin W. Ades; Ron Dagan; Jacquelyn S. Sampson;
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中图分类医学微生物学（病原细菌学、病原微生物学）;

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Evaluation and Improvement of Real-Time PCR Assays Targeting lytA, ply, and psaA Genes for Detection of Pneumococcal DNA

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