通过采用多种实时 PCR 检测方法,证实加纳感染艾滋病毒和未感染艾滋病毒的人的肠道微生物群中没有可测量数量的念珠菌和隐球菌。

Frieder Fuchs, Hagen Frickmann, Andreas Hahn, Carsten Balczun, Ralf Matthias Hagen, Torsten Feldt, Fred Stephen Sarfo, Veronica Di Cristanziano, Ulrike Loderstädt, Stephan Ehrhardt, Stefanie Schoppen, Harry Tagbor, Kirsten Alexandra Eberhardt
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引用次数: 0

摘要

导言。真菌感染是资源有限的热带地区获得性免疫缺陷患者的相关健康风险,但可用的监测数据却很少。对于白色念珠菌和隐球菌属来说,在气候变化和治疗方案有限的背景下,它们从环境贮藏体演变为人类病原体,导致危及生命的疾病,是目前讨论的一个公共卫生问题。发现胃肠道是真菌从环境中进入未确诊真菌感染者体内的流行病学生态位。通过分析加纳人的胃肠道样本,为西非加纳当地的阴沟球菌和隐球菌属流行病学数据做出贡献。对 875 名非年龄分层的加纳 HIV 感染者和 30 名未发现 HIV 感染的加纳对照者的粪便样本进行了分析,采用了四种针对球孢子菌的实时 PCR 检测方法和五种针对隐球菌的实时 PCR 检测方法。此外,还调查了 664 份 2 岁以下加纳儿童的样本。在实时 PCR 检测中,如果每个样本出现 1 个或更少的阳性信号,则认为目标微生物的真实丰度不太可能;如果出现 2 到 3 个阳性信号,则认为目标微生物的真实丰度很可能;如果出现 4 个或更多阳性信号,则认为目标微生物的真实丰度很可能。结果表明,结合应用灵敏的靶向特异性实时 PCR 检测方法,无论是否感染艾滋病毒,加纳人的肠道微生物群中都不存在隐球菌、新生隐球菌复合体和加特隐球菌复合体。尽管这些病原体对免疫抑制的加纳人造成了巨大的疾病负担,但从胃肠道样本中检测到这些病原体的可能性很小,因此在讨论这些与公共卫生有关的真菌的筛查策略时应考虑到这一点。相反,从这些样本中检测到的真菌不应被常规视为共生定植菌群。
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Absence of measurable quantities of Candida auris and Cryptococcus spp. in the gut microbiota of Ghanaian individuals with and without HIV infection as confirmed by applying multiple real-time PCR assays.

Introduction. Fungal infections are relevant health risks for individuals with acquired immunodeficiency in the resource-limited tropics, but available surveillance data are scarce. For Candida auris and Cryptococcus spp., the evolution from environmental reservoirs to human pathogens causing life-threatening diseases is currently discussed as a public health concern in the context of climate change and limited treatment options.Gap statement. Uncovering the gastrointestinal tract as an epidemiological niche of fungi emerging from the environment into individuals for whom fungal infections are not diagnosed.Aim. To contribute to data on the local epidemiology of C. auris and Cryptococcus spp. in Western African Ghana by analysing gastrointestinal samples of Ghanaian individuals.Methodology. Four real-time PCR assays targeting C. auris and five real-time PCR assays targeting Cryptococcus spp. were applied with stool samples of 875 non-age-stratified Ghanaian HIV patients and 30 Ghanaian control individuals without known HIV infection. Also, 664 samples from Ghanaian children under 2 years of age were investigated. The true abundance of the target micro-organism was considered as unlikely in the case of one or fewer positive signals, likely in the case of two to three positive signals and highly likely in the case of four or more positive signals per sample in the real-time PCR assays.Results. The combined application of sensitive, target-specific real-time PCR assays indicates that neither C. auris, Cryptococcus neoformans complex nor Cryptococcus gattii complex were part of the gut microbiota of Ghanaian individuals with or without HIV infection.Conclusion. Despite the significant disease burden from these pathogens in immunosuppressed Ghanaian individuals, detection from gastrointestinal samples was unlikely, which should be taken into account when discussing screening strategies for these fungi of public health concern. In contrast, the detection of these fungi from such samples should not routinely be considered as commensal colonization flora.

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