Joban Quesada, Paula Alfaro-Segura, Carlos Mata-Somarribas, Jackeline Alger, Mazlova Toledo, Jucicleide Ramos de Souza, Javier Mora, Carlos Graeff-Teixeira, Alberto Solano-Barquero, Alicia Rojas
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The present assay successfully amplified DNA of A. costaricensis obtained from different hosts and identified slight sequence differences through the HRM analysis. The detection limit of the HRM-qPCR was 0.00036 ng/µL, 1.0 ng/µL, and 0.1 ng/µL when A. costaricensis DNA was diluted in nuclease-free water, whole blood, and sera, respectively, which highlights its potential use for cell-free DNA detection. Moreover, the reaction did not cross-amplify DNA of Angiostrongylus cantonensis, Strongyloides stercoralis, and other nematodes, thus emphasizing its specificity. Additionally, the assay tested positive in formalin-fixed paraffin embedded biopsies with visible A. costaricensis adults or eggs, but not in samples without evident parasites or a low number of larvae, which suggests that the reaction is useful for confirming the presence of the nematode in clinical samples. Finally, DNA of sera from patients with AA was evaluated with the HRM-qPCR but none tested positive, possibly due to long storage periods of the samples which could have led to cfDNA degradation. 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引用次数: 0
摘要
腹腔角弓反张症(AA)是由腹腔角弓反张蚤(Angiostrongylus costaricensis)引起的人畜共患的严重寄生虫病。目前,AA 的诊断方法是在活组织切片中观察到与 A. costaricensis 相符的结构,或在血清检验中检测到抗体。因此,我们开发了一种 HRM 偶联 qPCR 方法来检测寄生虫的内部转录间隔 1(ITS1)。本检测方法成功地扩增了从不同宿主处获得的 A. costaricensis DNA,并通过 HRM 分析确定了轻微的序列差异。当 A. costaricensis DNA 被稀释在无核酸水、全血和血清中时,HRM-qPCR 的检测限分别为 0.00036 ng/µL、1.0 ng/µL 和 0.1 ng/µL,这突显了其用于无细胞 DNA 检测的潜力。此外,该反应不会交叉扩增坎顿角弓形虫、盘尾丝虫和其他线虫的 DNA,因此强调了其特异性。此外,在福尔马林固定的石蜡包埋活检样本中,该检测方法对可见的库氏安氏线虫成虫或虫卵检测呈阳性,而对无明显寄生虫或幼虫数量较少的样本检测呈阳性,这表明该反应可用于确认临床样本中是否存在线虫。最后,用 HRM-qPCR 对 AA 患者血清中的 DNA 进行了评估,但检测结果均为阳性,这可能是由于样本储存时间过长导致 cfDNA 降解所致。这些结果表明,该检测方法可用于 AA 的确诊,并有望用于无细胞 DNA 检测方案。
Real-time qPCR coupled with high-resolution melting curve analysis for the detection of the internal transcribed spacer 1 of Angiostrongylus costaricensis.
Abdominal angiostrongyliasis (AA) is a zoonotic and severe parasitic infection caused by Angiostrongylus costaricensis. AA is currently diagnosed by the observation of A. costaricensis-compatible structures in biopsies or the detection of antibodies in serological tests. However, molecular methods targeting homologous sequences of A. costaricensis have not been designed before, and therefore, an HRM-coupled qPCR was developed to detect the internal transcribed spacer 1 (ITS1) of the parasite. The present assay successfully amplified DNA of A. costaricensis obtained from different hosts and identified slight sequence differences through the HRM analysis. The detection limit of the HRM-qPCR was 0.00036 ng/µL, 1.0 ng/µL, and 0.1 ng/µL when A. costaricensis DNA was diluted in nuclease-free water, whole blood, and sera, respectively, which highlights its potential use for cell-free DNA detection. Moreover, the reaction did not cross-amplify DNA of Angiostrongylus cantonensis, Strongyloides stercoralis, and other nematodes, thus emphasizing its specificity. Additionally, the assay tested positive in formalin-fixed paraffin embedded biopsies with visible A. costaricensis adults or eggs, but not in samples without evident parasites or a low number of larvae, which suggests that the reaction is useful for confirming the presence of the nematode in clinical samples. Finally, DNA of sera from patients with AA was evaluated with the HRM-qPCR but none tested positive, possibly due to long storage periods of the samples which could have led to cfDNA degradation. These results indicate that this assay may be useful in the confirmation of AA and its prospection for cell-free DNA detection protocols.
期刊介绍:
The journal Parasitology Research covers the latest developments in parasitology across a variety of disciplines, including biology, medicine and veterinary medicine. Among many topics discussed are chemotherapy and control of parasitic disease, and the relationship of host and parasite.
Other coverage includes: Protozoology, Helminthology, Entomology; Morphology (incl. Pathomorphology, Ultrastructure); Biochemistry, Physiology including Pathophysiology;
Parasite-Host-Relationships including Immunology and Host Specificity; life history, ecology and epidemiology; and Diagnosis, Chemotherapy and Control of Parasitic Diseases.