Detection of human strongyloidiasis among patients with a high risk of complications attending selected tertiary care hospitals in Colombo, Sri Lanka using molecular and serological diagnostic tools.

IF 3 2区医学 Q1 PARASITOLOGY

Parasites & Vectors Pub Date : 2024-10-12 DOI:10.1186/s13071-024-06508-x

Chamarika Jayanetti Weerasekera, Nayana Gunathilaka, Chandrani Menike, Philip Anpahalan, Nilanka Perera, Nilanthi Renuka de Silva, Renu Wickremasinghe

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Abstract

Background: Strongyloidiasis a neglected tropical disease is known to cause severe disease among immunosuppressed and has not been studied extensively in Sri Lanka. Parasitological diagnostic approaches based on faecal microscopy and culture often fail to detect low-intensity infections. This study investigates the presence of strongyloidiasis among selected immunocompromised individuals using parasitological, molecular and serological techniques.

Methods: Adult patients with immunocompromising conditions admitted to three tertiary care hospitals in Sri Lanka were recruited. A faecal sample and 2 ml of venous blood were collected. The faecal samples were subjected to direct faecal smear and cultures (agar plate, charcoal and Harada-Mori) and polymerase chain reaction (PCR) using species specific primers designed for Strongyloides stercoralis. The presence of Strongyloides IgG antibodies was tested in the collected serum samples using DRG Strongyloides IgG enzyme-linked immunosorbent assay (ELISA) kits. The PCR products of the positive samples were sequenced using Sanger sequencing method.

Results: A total of 260 patients were recruited to this study, out of which 160 provided faecal samples and 122 provided blood samples. Out of the 160 faecal samples, none were positive for strongyloidiasis by direct smear, charcoal and Harada-Mori cultures. Only one sample (0.6%) was positive by agar plate culture. Out of the 123 samples subjected to PCR, 14 (11.4%), including the culture positive patient, were positive for S. stercoralis. Sequencing results of the PCR products indicated 100% similarity to S. stercoralis. Out of the 122 serum samples subjected to ELISA, 20 (16.4%), including the culture positive patient, were positive for Strongyloides IgG antibodies. However, sociodemographic, exposure factors, clinical features were not significantly associated with the presence of strongyloidiasis infection.

Conclusions: Strongyloidiasis is present among the immunocompromised population in Sri Lanka, even in the absence of a significant relationship with associated factors. It is advisable to screen such patients with highly sensitive tests such as PCR for early diagnosis and treatment.

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利用分子和血清学诊断工具在斯里兰卡科伦坡选定的三级医院就诊的高并发症风险患者中检测人类强直性脊柱炎。

背景：已知软下疳是一种被忽视的热带疾病，可在免疫抑制人群中引发严重疾病，但斯里兰卡尚未对其进行广泛研究。基于粪便显微镜和培养的寄生虫学诊断方法往往无法检测到低强度感染。本研究采用寄生虫学、分子学和血清学技术，调查了部分免疫力低下患者中是否存在强直性脊髓炎：方法：研究人员招募了在斯里兰卡三家三级医院住院的免疫力低下的成年患者。采集粪便样本和 2 毫升静脉血。粪便样本直接进行粪便涂片和培养（琼脂平板、木炭和 Harada-Mori），并使用针对盘尾丝虫设计的物种特异性引物进行聚合酶链反应（PCR）。使用 DRG 盘尾丝虫 IgG 酶联免疫吸附试验（ELISA）试剂盒检测采集的血清样本中是否存在盘尾丝虫 IgG 抗体。采用桑格测序法对阳性样本的 PCR 产物进行测序：本研究共招募了 260 名患者，其中 160 人提供了粪便样本，122 人提供了血液样本。在 160 份粪便样本中，经直接涂片、木炭和 Harada-Mori 培养，无一强直性包虫病阳性。只有一个样本（0.6%）在琼脂平板培养中呈阳性。在进行 PCR 检测的 123 个样本中，有 14 个样本（11.4%）（包括培养呈阳性的病人）对带状孢子虫呈阳性。聚合酶链反应产物的测序结果表明其与带状孢子虫的相似度为 100%。在进行ELISA检测的122份血清样本中，20份（16.4%）（包括培养阳性患者）的盘尾丝虫IgG抗体呈阳性。然而，社会人口学因素、接触因素和临床特征与强直丝虫感染并无明显关联：结论：斯里兰卡免疫力低下人群中存在强直丝虫感染，即使与相关因素没有明显关系。建议使用 PCR 等高灵敏度检测方法筛查此类患者，以便及早诊断和治疗。

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来源期刊

Parasites & Vectors 医学-寄生虫学

CiteScore

6.30

自引率

9.40%

发文量

433

审稿时长

1.4 months

期刊介绍： Parasites & Vectors is an open access, peer-reviewed online journal dealing with the biology of parasites, parasitic diseases, intermediate hosts, vectors and vector-borne pathogens. Manuscripts published in this journal will be available to all worldwide, with no barriers to access, immediately following acceptance. However, authors retain the copyright of their material and may use it, or distribute it, as they wish. Manuscripts on all aspects of the basic and applied biology of parasites, intermediate hosts, vectors and vector-borne pathogens will be considered. In addition to the traditional and well-established areas of science in these fields, we also aim to provide a vehicle for publication of the rapidly developing resources and technology in parasite, intermediate host and vector genomics and their impacts on biological research. We are able to publish large datasets and extensive results, frequently associated with genomic and post-genomic technologies, which are not readily accommodated in traditional journals. Manuscripts addressing broader issues, for example economics, social sciences and global climate change in relation to parasites, vectors and disease control, are also welcomed.