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基于新型重组抗原(NIE/SsIR)的粪类圆线虫免疫层析快速检测方法的评估:一项准确性研究。

Evaluation of novel recombinant antigen-based (NIE/SsIR) immunochromatographic rapid tests for Strongyloides stercoralis: an accuracy study.

作者信息

Scarso Salvatore, Tamarozzi Francesca, Mazzi Cristina, Degani Monica, Rizzi Eleonora, Tais Stefano, Buonfrate Dora

机构信息

Department of Infectious Tropical Diseases and Microbiology, IRCCS Sacro Cuore Don Calabria Hospital, Negrar, Verona, Italy.

Clinical Research Unit, IRCCS Sacro Cuore Don Calabria Hospital, Negrar, Verona, Italy.

出版信息

Parasit Vectors. 2024 Dec 23;17(1):535. doi: 10.1186/s13071-024-06569-y.

Abstract

BACKGROUND

Strongyloidiasis is a chronic parasitic disease that results in relevant human morbidity, caused by the nematode Strongyloides stercoralis. This nematode has a unique and complex life-cycle. There is so far no perfect test for this helminthiasis. Rapid immunochromatographic tests (RDTs) are of interest, specifically due to their feasibility for use in the field, where public health control of strongyloidiasis is recommended. The aim of this study was to evaluate two novel RDTs, one detecting immunoglobulin (Ig) G and the other detecting IgG4, based on a combination of recombinant antigens. The primary objective was to estimate the sensitivity and specificity of these RDTs, and the secondary objective was to assess ease of interpretation.

METHODS

Serum samples stored in our biobank with available matched results for at least one fecal (i.e. agar plate culture or PCR) and one serology test (i.e. enzyme-linked immunosorbent assay [ELISA] or indirect immunofluorescent antibody test [IFAT]) for S. stercoralis, were selected for this study. Those with at least one positive result for the fecal test were considered to be true positives (irrespective of the serology), while true negatives were those with negative results for both the fecal and serology tests. The results of the RDTs were read independently by two laboratory technicians. When disagreement over the results occurred, a third reader was involved, and the final result for each test was based on consistent results from two readers. Estimates were reported along with the 95% confidence intervals (CI). Regarding the secondary objective, agreement between two independent readers was calculated with Cohen's kappa statistic (κ).

RESULTS

A total of 90 serum samples were tested. Sensitivity of the IgG- and the IgG4-RDTs was 91.1% (95% CI 78.8-97.5) and 77.3% (95% CI 62.2-88.5), respectively. Specificity was 91.1% (95% CI 78.8-97.5) for the IgG-RDT and 100% (95% CI 92.1-100) for the IgG4-RDT. Agreement between readers was excellent (Cohen's κ = 0.96, 95% CI 0.86-1.08%).

CONCLUSIONS

The IgG-RDT demonstrated higher sensitivity and could hence be preferred for individual diagnosis, whereas the excellent specificity of the IgG4-RDT could be preferred for prevalence surveys in endemic areas. The results of both RDTs were easy to interpret based on excellent agreement between readers. Large prospective studies should follow to confirm these findings and to validate the use of either RDT for specific purposes/contexts.

摘要

背景

类圆线虫病是一种由粪类圆线虫引起的慢性寄生虫病,可导致相关的人类发病。这种线虫具有独特而复杂的生命周期。迄今为止,尚无针对这种蠕虫病的完美检测方法。快速免疫层析试验(RDT)备受关注,特别是因其适用于现场使用,而在现场推荐对类圆线虫病进行公共卫生控制。本研究的目的是评估两种新型RDT,一种检测免疫球蛋白(Ig)G,另一种检测IgG4,基于重组抗原的组合。主要目标是估计这些RDT的敏感性和特异性,次要目标是评估解读的简易程度。

方法

从我们的生物样本库中选取储存的血清样本,这些样本至少有一项粪检(即琼脂平板培养或PCR)和一项血清学检测(即酶联免疫吸附测定[ELISA]或间接免疫荧光抗体试验[IFAT])针对粪类圆线虫的匹配结果,用于本研究。粪检至少有一项阳性结果的被视为真阳性(无论血清学结果如何),而真阴性是指粪检和血清学检测结果均为阴性的样本。RDT的结果由两名实验室技术人员独立读取。当对结果出现分歧时,引入第三名读取人员,每项检测的最终结果基于两名读取人员一致的结果。报告估计值以及95%置信区间(CI)。关于次要目标,使用科恩kappa统计量(κ)计算两名独立读取人员之间的一致性。

结果

共检测了90份血清样本。IgG - RDT和IgG4 - RDT的敏感性分别为91.1%(95%CI 78.8 - 97.5)和77.3%(95%CI 62.2 - 88.5)。IgG - RDT的特异性为91.1%(95%CI 78.8 - 97.5),IgG4 - RDT的特异性为100%(95%CI 92.1 - 100)。读取人员之间的一致性极佳(科恩κ = 0.96,95%CI 0.86 - 1.08%)。

结论

IgG - RDT显示出更高的敏感性,因此可能更适合个体诊断,而IgG4 - RDT的出色特异性可能更适合在流行地区进行患病率调查。基于读取人员之间的极佳一致性,两种RDT的结果都易于解读。应开展大型前瞻性研究以证实这些发现,并验证任一RDT在特定目的/背景下的使用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/84d9/11668118/04954f97ef81/13071_2024_6569_Fig1_HTML.jpg

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