Department of Epidemiology and Infection Prevention, Regional Public Health Laboratory Kennemerland, Haarlem, The Netherlands.
Laboratory for Microbiology and Infection Control, Amphia Hospital, Breda, The Netherlands.
J Antimicrob Chemother. 2017 Sep 1;72(9):2512-2518. doi: 10.1093/jac/dkx189.
To determine the diagnostic accuracy of the Check-Direct ESBL Screen for BD MAX (ESBL qPCR) and an ESBL culture method to identify ESBLs directly from rectal swabs.
Rectal swabs were obtained from clinical patients by performing cross-sectional (point)prevalence measurements in three regional hospitals. Rectal swabs were analysed by direct culture (ChromID ESBL agar) and with the ESBL qPCR. Suspected ESBL-producing isolates were confirmed with the combination disc method and analysed by WGS.
Out of 354 rectal swabs and 351 patients, 21 rectal swabs and 20 patients were positive for ESBL-producing isolates, resulting in a regional ESBL colonization prevalence of 5.7%. One rectal swab was false negative with the ESBL qPCR (blaTEM-12) and not covered by the ESBL qPCR. Eight ESBL qPCR-positive rectal swabs could not be confirmed by culture and were classified as false ESBL qPCR positive. The sensitivity and specificity of the ESBL qPCR were 95.2% (n = 20) and 97.6% (n = 323), respectively. When an optimal cycle threshold cut-off value of 37 was used, the ESBL qPCR displayed a sensitivity and specificity of 95.2% (n = 20) and 98.8% (n = 327), respectively (AUC = 0.975, 95% CI = 0.922-1).
This ESBL qPCR offers rapid direct detection of the most prevalent ESBL types (blaCTX-M group and blaSHV group) from rectal swabs. The relatively high false-positive rate renders this test the most suitable as a screening test in high-prevalence regions or in an outbreak setting where a fast result is essential.
确定 BD MAX(ESBL qPCR)Check-Direct ESBL 筛查试验和一种从直肠拭子中直接鉴定 ESBL 的 ESBL 培养方法对 ESBL 的诊断准确性。
在 3 家地区医院进行横断面(点)患病率测量,从临床患者中采集直肠拭子。直肠拭子直接通过培养(ChromID ESBL 琼脂)和 ESBL qPCR 进行分析。通过联合药敏纸片法和 WGS 分析疑似产 ESBL 分离株。
在 354 份直肠拭子和 351 例患者中,21 份直肠拭子和 20 例患者的 ESBL 产分离株阳性,导致区域 ESBL 定植率为 5.7%。1 份直肠拭子的 ESBL qPCR(blaTEM-12)结果为假阴性,且不在 ESBL qPCR 检测范围内。8 份 ESBL qPCR 阳性的直肠拭子不能通过培养确认,被归类为假 ESBL qPCR 阳性。ESBL qPCR 的灵敏度和特异性分别为 95.2%(n=20)和 97.6%(n=323)。当使用最佳的循环阈值截止值 37 时,ESBL qPCR 的灵敏度和特异性分别为 95.2%(n=20)和 98.8%(n=327)(AUC=0.975,95%CI=0.922-1)。
这种 ESBL qPCR 可快速直接从直肠拭子中检测最常见的 ESBL 类型(blaCTX-M 组和 blaSHV 组)。相对较高的假阳性率使该试验最适合在高流行地区或在需要快速结果的暴发情况下作为筛查试验。
