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Refining Diagnosis of Schistosoma haematobium Infections: Antigen and Antibody Detection in Urine

机译:精制诊断血吸虫血吸虫沸腾感染:尿树和抗体检测尿液

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摘要

Background: Traditional microscopic examination of urine or stool for schistosome eggs lacks sensitivity compared to measurement of schistosome worm-derived circulating antigens in serum or urine. The ease and non-invasiveness of urine collection makes urine an ideal sample for schistosome antigen detection. In this study several user-friendly, lateral-flow (LF) based urine assays were evaluated against a composite reference that defined infection as detection of either eggs in urine or anodic antigen in serum.Method: In a Tanzanian population with a S. haematobium prevalence of 40–50% (S. mansoni prevalence <2%), clinical samples from 44 women aged 18 to 35 years were analyzed for Schistosoma infection. Urine and stool samples were examined microscopically for eggs, and serum samples were analyzed for the presence of the anodic antigen. Urines were further subjected to a set of LF assays detecting (circulating) anodic (CAA) and cathodic antigen (CCA) as well as antibodies against soluble egg antigens (SEA) and crude cercarial antigen preparation (SCAP).Results: The urine LF anodic antigen assay utilizing luminescent upconverting reporter particles (UCP) confirmed its increased sensitivity when performed with larger sample volume. Qualitatively, the anodic antigen assay performed on 250 μL urine matched the performance of the standard anodic antigen assay performed on 20 μL serum. However, the ratio of anodic antigen levels in urine vs. serum of individual patients varied with absolute levels always higher in serum. The 10 μL urine UCP-LF cathodic antigen assay correlated with the commercially available urine POC-CCA (40 μL) test, while conferring better sensitivity with a quantitative result. Urinary antibodies against SEA and SCAP overlap and correlate with the presence of urinary egg and serum anodic antigen levels.Conclusions: The UCP-LF anodic antigen assay using 250 μL of urine is an expedient user-friendly assay and a suitable non-invasive alternative to serum-based antigen testing and urinary egg detection. Individual biological differences in the clearance process of the circulating antigens are thought to explain the observed high variation in the type and level of antigen (anodic or cathodic) measured in urine or serum. Simultaneous detection of anodic and cathodic antigen may be considered to further increase accuracy.
机译:背景:与血清或尿液中的血吸虫蠕虫衍生的循环抗原的测量相比,血吸虫卵的传统显微镜检查缺乏敏感性。尿液收集的缓解和非侵袭性使尿液成为血吸虫抗原检测的理想样本。在该研究中,评估了几种用户友好的横向流动(LF)的尿法测定,该综合参考评估了定义的感染作为血清中尿液或阳极抗原的卵子中的卵子的检测。在坦桑尼人群中,用S. haematobium分析了44岁至35岁女性的40-50%(S.Mansoni Prevaliency <2%)的患病率分析了44至35岁的临床样本进行血吸虫瘤感染。检查尿液和粪便样品用于卵子,分析血清样品用于阳极抗原的存在。尿液进一步进行一组LF测定检测(循环)阳极(CAA)和阴极抗原(CCA)以及针对可溶性蛋抗原(海)和粗胰抗原制剂(SCAP)的抗体。结果:尿液LF阳极利用发光的抗原测定,使用发光上变化报告器颗粒(UCP)确认在用较大样品体积进行时的敏感性增加。定性地,在250μl尿液中进行的阳极抗原测定匹配在20μL血清上进行的标准阳极抗原测定的性能。然而,血清中尿液与血清血清血清血清的比例随绝对水平而变化。 10μl尿液UCP-LF阴极抗原测定与市售的尿POC-CCA(40μL)试验相关,同时赋予具有定量结果的更好的敏感性。尿抗体与海和湿湿重叠并与尿液和血清阳极抗原水平的存在相关。结论:使用250μl尿液的UCP-LF阳极抗原测定是有利的用户友好的测定和合适的非侵入性替代品基于血清的抗原测试和尿液检测。循环抗原的间隙过程中的个体生物差异被认为解释在尿液或血清中测量的抗原(阳极或阴极或阴极)的类型和水平的观察到的高变化。可以认为阳极和阴极抗原的同时检测进一步提高精度。

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