Department of Bacteriology, Animal and Plant Health Agency, Weybridge, Surrey, United Kingdom.
Veterinary Epidemiology, Economics and Public Health Group, Department of Pathobiology and Population Sciences, Royal Veterinary College, London, United Kingdom.
PLoS One. 2024 Apr 11;19(4):e0289190. doi: 10.1371/journal.pone.0289190. eCollection 2024.
The emergence and spread of β-lactamase-producing Enterobacteriaceae poses a significant threat to public health, necessitating the rapid detection and investigation of the molecular epidemiology of these pathogens. We modified a multiplex real-time (RT)-PCR to concurrently detect β-lactamase genes (blaCTX-M, blaTEM, and blaSHV) and Enterobacteriaceae 16S ribosomal RNA. qPCR probes and primers were validated using control isolates, and the sensitivity and specificity assessed. The optimised multiplex qPCR was used to screen 220 non-clinical Enterobacteriaceae from food animals and in-contact humans in Southeast Nigeria selected on cefotaxime-supplemented agar plates. Binary logistic regression was used to explore factors associated with the presence of the blaTEM and blaSHV genes in these isolates, and a subset of isolates from matched sampling sites and host species were whole genome sequenced, and their antimicrobial resistance (AMR) and plasmid profiles determined. The sensitivity and specificity of the qPCR assay was 100%. All isolates (220/220) were positive for Enterobacteriaceae ribosomal 16S rRNA and blaCTX-M, while 66.4% (146/220) and 9% (20/220) were positive for blaTEM and blaSHV, respectively. The prevalence of blaTEM and blaSHV varied across different sampling sites (farm, animal market and abattoirs). Isolates from Abia state were more likely to harbour blaTEM (OR = 2.3, p = 0.04) and blaSHV (OR = 5.12,p = 0.01) than isolates from Ebonyi state; blaTEM was more likely to be detected in isolates from food animals than humans (OR = 2.34, p = 0.03), whereas the reverse was seen for blaSHV (OR = 7.23, p = 0.02). Furthermore, Klebsiella and Enterobacter isolates harboured more AMR genes than Escherichia coli, even though they were isolated from the same sample. We also identified pan resistant Klebsiella harbouring resistance to ten classes of antimicrobials and disinfectant. Therefore, we recommend ESKAPE pathogens are included in AMR surveillance in future and suggest qPCRs be utilised for rapid screening of Enterobacteriaceae from human and animal sources.
产β-内酰胺酶肠杆菌科的出现和传播对公共健康构成了重大威胁,因此需要快速检测和研究这些病原体的分子流行病学。我们修改了一种多重实时(RT)-PCR 方法,以同时检测β-内酰胺酶基因(blaCTX-M、blaTEM 和 blaSHV)和肠杆菌科 16S 核糖体 RNA。使用对照分离株验证了 qPCR 探针和引物,并评估了其灵敏度和特异性。优化后的多重 qPCR 用于筛选 220 株来自尼日利亚东南部食品动物和接触人群的非临床肠杆菌科,这些分离株是在头孢噻肟补充琼脂平板上选择的。使用二元逻辑回归探讨了这些分离株中 blaTEM 和 blaSHV 基因存在的相关因素,并对来自匹配采样点和宿主物种的分离株进行了全基因组测序,并确定了其抗生素耐药性(AMR)和质粒图谱。qPCR 检测方法的灵敏度和特异性均为 100%。所有分离株(220/220)均为肠杆菌科核糖体 16S rRNA 和 blaCTX-M 阳性,而 blaTEM 和 blaSHV 的阳性率分别为 66.4%(146/220)和 9%(20/220)。不同采样地点(农场、动物市场和屠宰场)的 blaTEM 和 blaSHV 流行率不同。来自阿比亚州的分离株比来自埃博尼州的分离株更有可能携带 blaTEM(OR = 2.3,p = 0.04)和 blaSHV(OR = 5.12,p = 0.01);blaTEM 更有可能在食品动物来源的分离株中检测到,而不是在人类来源的分离株中(OR = 2.34,p = 0.03),而 blaSHV 则相反(OR = 7.23,p = 0.02)。此外,与大肠埃希菌相比,克雷伯菌和肠杆菌属分离株携带更多的 AMR 基因,尽管它们是从同一样本中分离出来的。我们还发现了耐十种类抗生素和消毒剂的泛耐药性克雷伯菌。因此,我们建议在未来的抗生素耐药性监测中纳入 ESKAPE 病原体,并建议使用 qPCR 快速筛选来自人类和动物来源的肠杆菌科。
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