Detection of six soil-transmitted helminths in human stool by qPCR- a systematic workflow

蛔虫 美国内贾特酒店 十二指肠钩虫 生物 多路复用 三叉毛螨 DNA提取 荧光染料 实时聚合酶链反应 多重聚合酶链反应 粪圆线虫 聚合酶链反应 微生物学 蠕虫 兽医学 医学 免疫学 遗传学 基因
作者
Kristy Azzopardi,Myra Hardy,Ciara Baker,Rhian Bonnici,Stacey Llewellyn,James McCarthy,Rebecca J. Traub,Andrew C. Steer
出处
期刊:PLOS ONE [Public Library of Science]
卷期号:16 (9): e0258039-e0258039 被引量:21
标识
DOI:10.1371/journal.pone.0258039
摘要

Soil-transmitted helminths (STH) infect up to one-quarter of the global population, with a significant associated disease burden. The main human STH are: Ancylostoma spp. and Necator americanus (hookworms); Ascaris lumbricoides, Trichuris trichiura, and Strongyloides stercoralis. The aim of this study was to establish a scalable system for stool STH multiplex quantitative real-time polymerase chain reactions (qPCR). Stool samples collected in Fiji and preserved in potassium dichromate were transferred to Melbourne at ambient temperature. Samples were washed to remove potassium dichromate and DNA was extracted with the Mini-Beadbeater-24 and a column-based kit. A SYBR green qPCR to detect the vertebrate mitochondrial gene was used as a DNA extraction control. Samples were tested using a probe-based multiplex qPCR targeting A. lumbricoides, T. trichiura and S. stercoralis, and in a second multiplex reaction to detect hookworms to the species level (A. duodenale, A. ceylanicum, N. americanus). An internal amplification control in both multiplex assays was included to prevent false-negative results due to PCR inhibitors. Samples were homogenised for a single cycle of 40 seconds to release STH DNA and washed stool was stored for up to 15 weeks at -30°C without compromising DNA. Our multiplex qPCR detected multiple species of STH without reduced sensitivity compared to singleplex. qPCR data from 40 stools was validated against STH-positive stools determined by microscopy. We have developed and validated an efficient and staged system for detecting six clinically important STH affecting humans that could be easily implemented without advanced automation in any qPCR-capable laboratory.
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