使用实时 PCR(RT-PCR)比较健康儿童和有呼吸道症状儿童的肺炎链球菌定植密度。
Comparison of pneumococcal colonization density among healthy children and children with respiratory symptoms using real time PCR (RT-PCR).
机构信息
Faculty of Medicine, University of Peradeniya, Kandy, Sri Lanka.
Department of Microbiology, Faculty of Medicine, University of Peradeniya, Kandy, Sri Lanka.
出版信息
BMC Microbiol. 2022 Jan 20;22(1):31. doi: 10.1186/s12866-022-02442-z.
BACKGROUND
Nasopharyngeal colonization is considered a necessary step in the initiation of pneumococcal diseases. Real time PCR (RT-PCR) is an alternative approach for the identification and quantification of pneumococci directly from samples.
OBJECTIVES
To compare pneumococcal detection rates using culture-based method versus RT-PCR direct detection and to quantify pneumococcal colonization in two study cohorts (healthy children and hospitalized children with respiratory symptoms) using quantitation through RT-PCR.
METHODOLOGY
A total of 101 nasopharyngeal swabs (NPS) from healthy children and 183 NPSs from hospitalized children with respiratory symptoms were included in the study. None of the children were vaccinated. All children were between 2 months to 2 years. In parallel to routine culture and identification, a RT-PCR assay targeting the lytA gene was done.
RESULTS
Considering all 284 samples tested, colonization rate by conventional culture was 41.2% (n = 117) while positive colonization using RT-PCR was 43.7% (n = 124). The colonization rate detected by RT-PCR in the healthy cohort was 33.7% (n = 34) and it was 49.2% (n = 90) in the hospitalized cohort. It was 37.6% (n = 38) and 43.2% (n = 79) for the two cohorts by culture. The mean Cq value for the healthy cohort is 29.61 (SD 2.85) and 28.93 (SD 3.62) for the hospitalized cohort. With the standard curve obtained from amplifying a dilution series of control DNA, the mean amount of genomic DNA copy numbers detected in children with respiratory symptoms was log10 7.49 (SD 1.07) while it was log10 7.30 (SD 0.23) in healthy children and the difference was not statistically significant.
CONCLUSIONS
The overall colonization rate was higher when detected using RT-PCR compared to culture. However, it was lower in the healthy group when detected with RT-PCR compared to culture. Even though there was a higher detection of pneumococcal colonization density in children with respiratory symptoms, this was not significantly higher unlike many previous studies. Therefore, the use of RT-PCR to detect pneumococcal colonization needs further evaluation with careful analysis of interpretation and confounders.
背景
鼻咽定植被认为是引发肺炎球菌病的必要步骤。实时 PCR(RT-PCR)是一种替代方法,可以直接从样本中鉴定和定量肺炎球菌。
目的
比较基于培养的方法与 RT-PCR 直接检测的肺炎球菌检出率,并使用 RT-PCR 定量法对两个研究队列(健康儿童和住院有呼吸道症状的儿童)进行肺炎球菌定植的定量。
方法
本研究共纳入 101 例健康儿童鼻咽拭子(NPS)和 183 例住院有呼吸道症状儿童的 NPS。所有儿童均未接种疫苗,年龄均在 2 个月至 2 岁之间。除常规培养和鉴定外,还进行了针对 lytA 基因的 RT-PCR 检测。
结果
考虑到所有 284 个测试样本,常规培养的定植率为 41.2%(n=117),而 RT-PCR 检测的阳性定植率为 43.7%(n=124)。健康队列中通过 RT-PCR 检测到的定植率为 33.7%(n=34),住院队列中的定植率为 49.2%(n=90)。培养的两个队列的定植率分别为 37.6%(n=38)和 43.2%(n=79)。健康队列的平均 Cq 值为 29.61(SD 2.85),住院队列的平均 Cq 值为 28.93(SD 3.62)。使用从扩增系列稀释对照 DNA 获得的标准曲线,患有呼吸道症状的儿童中检测到的基因组 DNA 拷贝数的平均量为 log10 7.49(SD 1.07),而健康儿童的平均量为 log10 7.30(SD 0.23),差异无统计学意义。
结论
与培养法相比,使用 RT-PCR 检测的总体定植率更高。然而,与培养法相比,RT-PCR 检测在健康组中的定植率较低。尽管患有呼吸道症状的儿童中肺炎球菌定植密度的检测较高,但与许多先前的研究不同,这并没有显著更高。因此,使用 RT-PCR 检测肺炎球菌定植需要进一步评估,并仔细分析解释和混杂因素。
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