Halse Tanya A, Musser Kimberlee A, Limberger Ronald J
New York State Department of Health, Wadsworth Center-David Axelrod Institute, 120 New Scotland Avenue, Albany, NY 12208, USA.
Mol Cell Probes. 2006 Oct;20(5):290-7. doi: 10.1016/j.mcp.2006.02.003. Epub 2006 Mar 6.
Lymphogranuloma venereum (LGV) is caused by a rare form of Chlamydia trachomatis that is difficult to diagnose, since culture is not readily available, and since other methods are not reliable or lack sensitivity. We report here a rapid, sensitive, and specific real-time multiplex polymerase chain reaction (PCR) assay capable of detecting C. trachomatis and identifying serovar L-2 in the same reaction, directly from rectal swabs. The analytical sensitivity of the assay was 25 genome copies for C. trachomatis, and 50 genome copies for L-2. The analytical specificity was 100%, as demonstrated with a diverse range of C. trachomatis serovars and other site-specific bacterial pathogens. With the use of a rapid DNA extraction method, a blinded validation of spiked rectal swabs correctly identified 30 samples containing C. trachomatis cells, L-2 DNA, or negative samples. The multiplexed PCR assay also identified serovar L-2 in 13 of 70 rectal swab samples taken from symptomatic patients. Twelve additional samples were positive for C. trachomatis only, and omp1 sequencing determined these samples as either serovar D, E, G, J, or K. This assay represents the first real-time PCR method capable of detecting C. trachomatis DNA, and of simultaneously identifying C. trachomatis infection as serovar L-2.
性病性淋巴肉芽肿(LGV)由沙眼衣原体的一种罕见类型引起,难以诊断,因为难以进行培养,且其他方法不可靠或缺乏敏感性。我们在此报告一种快速、灵敏且特异的实时多重聚合酶链反应(PCR)检测方法,该方法能够直接从直肠拭子中在同一反应中检测沙眼衣原体并鉴定血清型L-2。该检测方法对沙眼衣原体的分析灵敏度为25个基因组拷贝,对L-2为50个基因组拷贝。分析特异性为100%,这在多种沙眼衣原体血清型和其他部位特异性细菌病原体中得到了证实。使用快速DNA提取方法,对加标的直肠拭子进行盲法验证,正确鉴定出30个含有沙眼衣原体细胞、L-2 DNA的样本或阴性样本。多重PCR检测方法还在从有症状患者采集的70份直肠拭子样本中的13份中鉴定出了血清型L-2。另外12份样本仅沙眼衣原体呈阳性,omp1测序确定这些样本为血清型D、E、G、J或K。该检测方法是第一种能够检测沙眼衣原体DNA并同时将沙眼衣原体感染鉴定为血清型L-2的实时PCR方法。
