评估雅培LCx连接酶链反应检测法用于检测性传播疾病门诊人群尿液和生殖器拭子标本中的沙眼衣原体和淋病奈瑟菌。
Evaluation of the Abbott LCx ligase chain reaction assay for detection of Chlamydia trachomatis and Neisseria gonorrhoeae in urine and genital swab specimens from a sexually transmitted disease clinic population.
作者信息
Carroll K C, Aldeen W E, Morrison M, Anderson R, Lee D, Mottice S
机构信息
Department of Pathology, University of Utah Health Sciences Center, Salt Lake City 84132, USA.
出版信息
J Clin Microbiol. 1998 Jun;36(6):1630-3. doi: 10.1128/JCM.36.6.1630-1633.1998.
The Abbott LCx ligase chain reaction (LCR) assay for the simultaneous detection of Chlamydia trachomatis and Neisseria gonorrhoeae was evaluated by using swab and urine specimens from 562 patients. C. trachomatis results by LCR were compared to those by the Gen-Probe PACE 2 assay, whereas N. gonorrhoeae results by LCR were compared to those by culture. The Gen-Probe and LCR assays were performed according to the manufacturers' instructions. Gram-negative diplococci growing on modified Thayer-Martin medium were confirmed as N. gonorrhoeae by the GonoGen II assay. Supplemental data analysis was performed by major outer membrane protein PCR for C. trachomatis and probes for pilin gene detection for N. gonorrhoeae. A true-positive result for each pathogen was defined as a positive result for all three or two of three assays. Overall agreement among the six assays was 94.8%. C. trachomatis prevalence was 16.2%; N. gonorrhoeae prevalence was 5.5%. The overall sensitivity and specificity, respectively, for each test (after supplemental data analysis) were as follows: for C. trachomatis, Gen-Probe, 65.9 and 100%; LCR on urine, 90.1 and 100%; LCR on swab specimens, 96.7 and 100%; and for N. gonorrhoeae, culture, 80.6 and 100%; LCR on urine, 93.5 and 99.8%; and LCR on swab specimens, 96.8 and 100%. For women, the N. gonorrhoeae culture was very insensitive compared to its performance in men (58.3 versus 94.7%, respectively). For C. trachomatis, the Gen-Probe assay's sensitivity was lower for men than for women (62.3 versus 71.1%, respectively). The sensitivity for C. trachomatis detection by LCR on urethral and cervical swab specimens was 96.2 and 97.4% for men and women, respectively. For men, swab results were slightly better than urine results for both pathogens (sensitivity for C. trachomatis in swab and urine specimens, 96.2 and 92.5%, respectively; sensitivity for N. gonorrhoeae in swab and urine specimens, 100 and 94.7%, respectively), while for women, cervical swabs were superior in sensitivity to urine samples for detecting C. trachomatis (swab, 97.4%; urine, 81.6%) and equivalent for N. gonorrhoeae (swab, 92.3%; urine, 91.6%). The LCx LCR appears to be both sensitive and specific for the detection of C. trachomatis and N. gonorrhoeae when performed on urine or genital swab samples. Swab samples had better sensitivity than urine samples for the detection of both pathogens.
采用雅培LCx连接酶链反应(LCR)检测法对562例患者的拭子和尿液标本同时进行沙眼衣原体和淋病奈瑟菌检测,并进行评估。将LCR检测沙眼衣原体的结果与Gen-Probe PACE 2检测法的结果进行比较,而将LCR检测淋病奈瑟菌的结果与培养法的结果进行比较。Gen-Probe和LCR检测均按照制造商的说明进行。在改良的Thayer-Martin培养基上生长的革兰阴性双球菌通过GonoGen II检测法确认为淋病奈瑟菌。采用沙眼衣原体主要外膜蛋白PCR和淋病奈瑟菌菌毛基因检测探针进行补充数据分析。每种病原体的真阳性结果定义为三种检测中的三种或两种呈阳性结果。六种检测方法的总体一致性为94.8%。沙眼衣原体患病率为16.2%;淋病奈瑟菌患病率为5.5%。每项检测(补充数据分析后)的总体敏感性和特异性分别如下:对于沙眼衣原体,Gen-Probe检测法为65.9%和100%;尿液LCR检测法为90.1%和100%;拭子标本LCR检测法为96.7%和100%;对于淋病奈瑟菌,培养法为80.6%和100%;尿液LCR检测法为93.5%和99.8%;拭子标本LCR检测法为96.8%和100%。对于女性,淋病奈瑟菌培养法与其在男性中的表现相比非常不敏感(分别为58.3%和94.7%)。对于沙眼衣原体,Gen-Probe检测法在男性中的敏感性低于女性(分别为62.3%和71.1%)。LCR检测尿道和宫颈拭子标本中沙眼衣原体的敏感性,男性和女性分别为96.2%和97.4%。对于男性,两种病原体的拭子检测结果均略优于尿液检测结果(沙眼衣原体拭子和尿液标本的敏感性分别为96.2%和92.5%;淋病奈瑟菌拭子和尿液标本的敏感性分别为100%和94.7%),而对于女性,宫颈拭子在检测沙眼衣原体方面的敏感性优于尿液样本(拭子为97.4%;尿液为81.6%),在检测淋病奈瑟菌方面两者相当(拭子为92.3%;尿液为91.6%)。当对尿液或生殖器拭子样本进行检测时,LCx LCR检测法对于沙眼衣原体和淋病奈瑟菌的检测似乎既敏感又特异。在检测两种病原体时,拭子样本的敏感性优于尿液样本。
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