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马拉维沿马拉维湖南岸地区感染曼氏血吸虫的学龄儿童的曼氏血吸虫分子流行病学和种群遗传学。

Molecular epidemiology and population genetics of Schistosoma mansoni infecting school-aged children situated along the southern shoreline of Lake Malawi, Malawi.

机构信息

Department of Tropical Disease Biology, Liverpool School of Tropical Medicine, Liverpool, United Kingdom.

Wolfson Wellcome Biomedical Laboratories, Department of Zoology, Natural History Museum, Cromwell Road, London, United Kingdom.

出版信息

PLoS Negl Trop Dis. 2024 Oct 7;18(10):e0012504. doi: 10.1371/journal.pntd.0012504. eCollection 2024 Oct.

Abstract

BACKGROUND

In areas of low disease endemicity, highly sensitive diagnostic tools to identify, diagnose, and monitor intestinal schistosomiasis transmission are needed to reliably measure the burden and risk of infection. Here, we used highly sensitive molecular diagnostic methods to investigate Schistosoma mansoni prevalence and transmission along the southern shoreline of Lake Malawi, five years post-disease outbreak.

METHODOLOGY AND PRINCIPAL FINDINGS

Faecal and urine samples were provided by school-aged children situated along the southern shoreline of Lake Malawi. Kato-Katz faecal-egg microscopy and point-of-care circulating cathodic antigen (POC-CCA) rapid diagnostic tests were then performed to diagnose infection with S. mansoni. Urine-egg microscopy was also used to diagnose infection with Schistosoma haematobium. In addition, Schistosoma miracidia were isolated from faecal material using a standard miracidium hatching technique. A two-step real-time PCR approach was then used to diagnose infection with S. mansoni using DNA isolated from faecal samples. Furthermore, isolated miracidia were genotyped to species level through PCR and Sanger sequencing. Phylogenetic analyses were then carried out to identify which previously defined S. mansoni cox1 lineage group S. mansoni miracidia were most closely related to. The measured prevalence of S. mansoni infection varied considerably depending on which diagnostic assay was used. When compared to real-time PCR, faecal-egg microscopy had a sensitivity of 9% and a specificity of 100%. When POC-CCA 'trace' results were considered positive, POC-CCA had a sensitivity of 73% and a specificity of 81% when compared to real-time PCR. However, when considered negative, POC-CCA sensitivity was reduced to 56%, whereas specificity was increased to 90%. In addition, a high degree of S. haematobium DNA was detected in DNA isolated from faecal samples and motile S. haematobium miracidia were recovered from faecal samples. Schistosoma mansoni miracidia were closely related to two independent cox1 lineage groups, suggesting multiple recent introduction and colonisation events originating from surrounding east African countries.

CONCLUSIONS AND SIGNIFICANCE

Intestinal schistosomiasis is now highly prevalent along the southern shoreline of Lake Malawi just five years post-disease outbreak. In addition, a high prevalence of urogenital schistosomiasis persists. The revision of ongoing schistosomiasis control programmes in this area is therefore recommended. Our study also highlights the need for reliable diagnostic assays capable of distinguishing between Schistosoma species in multispecies co-endemic areas.

摘要

背景

在疾病低流行地区,需要高度敏感的诊断工具来识别、诊断和监测肠道血吸虫病传播,以便可靠地衡量感染负担和风险。在这里,我们使用高度敏感的分子诊断方法来调查马拉维湖南部沿湖地区五年后血吸虫病爆发后的曼氏血吸虫病的流行率和传播情况。

方法和主要发现

采集了位于马拉维湖南部沿湖地区的学龄儿童的粪便和尿液样本。然后进行加藤厚涂片粪便虫卵镜检和即时检测循环阴离子抗原(POC-CCA)快速诊断检测,以诊断曼氏血吸虫感染。尿液虫卵镜检也用于诊断埃及血吸虫感染。此外,使用标准的毛蚴孵化技术从粪便材料中分离毛蚴。然后使用两步实时 PCR 方法从粪便样本中提取的 DNA 诊断曼氏血吸虫感染。此外,通过 PCR 和 Sanger 测序对分离的毛蚴进行种系水平基因分型。然后进行系统发育分析,以确定与分离的曼氏血吸虫毛蚴最密切相关的先前定义的曼氏血吸虫 cox1 谱系群。曼氏血吸虫感染的测量流行率因使用的诊断检测方法而异。与实时 PCR 相比,粪便虫卵镜检的灵敏度为 9%,特异性为 100%。当将 POC-CCA“痕迹”结果视为阳性时,与实时 PCR 相比,POC-CCA 的灵敏度为 73%,特异性为 81%。然而,当被认为是阴性时,POC-CCA 的灵敏度降低到 56%,而特异性增加到 90%。此外,从粪便样本中提取的 DNA 中检测到大量的埃及血吸虫 DNA,并且从粪便样本中回收了活动的埃及血吸虫毛蚴。曼氏血吸虫毛蚴与两个独立的 cox1 谱系群密切相关,这表明多个最近来自周边东非国家的传入和定植事件。

结论和意义

曼氏血吸虫病在马拉维湖南部沿湖地区的流行率很高,这是疾病爆发五年后的情况。此外,泌尿生殖道血吸虫病的高患病率仍然存在。因此,建议修订该地区正在进行的血吸虫病控制方案。我们的研究还强调了在多物种流行地区需要可靠的诊断检测方法,能够区分血吸虫种。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7005/11458004/124774acd288/pntd.0012504.g001.jpg

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