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首页> 外文期刊>Human vaccines & immunotherapeutics. >Population density profiles of nasopharyngeal carriage of 5 bacterial species in pre-school children measured using quantitative PCR offer potential insights into the dynamics of transmission
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Population density profiles of nasopharyngeal carriage of 5 bacterial species in pre-school children measured using quantitative PCR offer potential insights into the dynamics of transmission

机译:使用定量PCR测量的学龄前儿童鼻咽运输5种细菌的种群密度概况为传播动力学提供了潜在的见解

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Bacterial vaccines can reduce carriage rates. Colonization is usually a binary endpoint. Real time quantitative PCR (qPCR) can quantify bacterial DNA in mucosal samples over a wide range. Using culture and single-gene species-specific qPCRs for Streptococcus pneumoniae (lytA), Streptococcus pyogenes (ntpC), Moraxella catarrhalis (ompJ), Haemophilus influenzae (hdp) and Staphylococcus aureus (nuc) and standard curves against log-phase reference strain broth cultures we described frequency and peak density distributions of carriage in nasopharyngeal swabs from 161 healthy 2-4 y old children collected into STGG broth. In general, detection by qPCR and culture was consistent. Discordance mostly occurred at lower detection thresholds of both methods, although PCR assays for S. pyogenes and S. aureus were less sensitive. Density varied across 5-7 orders of magnitude for the 5 species with the abundant species skewed toward high values (modes: S. pneumoniae log3-4, M. catarrhalis & H. influenzae log4-5 CFU/ml broth). Wide ranges of bacterial DNA concentrations in healthy children carrying these bacteria could mean that different individuals at different times vary greatly in infectiousness. Understanding the host, microbial and environmental determinants of colonization density will permit more accurate prediction of vaccine effectiveness.
机译:细菌疫苗可以降低运输速度。殖民化通常是一个二进制终点。实时定量PCR(qPCR)可以在很大范围内对粘膜样品中的细菌DNA进行定量。使用肺炎链球菌(lytA),化脓性链球菌(ntpC),卡他莫拉菌(ompJ),流感嗜血杆菌(hdp)和金黄色葡萄球菌(nuc)的培养物和单基因物种特异性qPCR和针对对数期参考菌株肉汤的标准曲线的文化,我们描述了收集到STGG肉汤中的161名2-4岁健康儿童的鼻咽拭子中运输的频率和峰值密度分布。通常,通过qPCR和培养物检测是一致的。尽管对于化脓性链球菌和金黄色葡萄球菌的PCR检测灵敏度较低,但两种方法的不一致大多在较低的检测阈值下发生。 5个物种的密度在5-7个数量级之间变化,丰富的物种偏向高值(模式:肺炎链球菌log3-4,卡他莫拉菌和流感嗜血杆菌log4-5 CFU / ml肉汤)。在携带这些细菌的健康儿童中,细菌DNA的浓度范围很广,这可能意味着不同个体在不同时间的传染性差异很大。了解宿主,微生物和环境的定植密度决定因素,将可以更准确地预测疫苗效力。

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