棘球蚴抗原在血清学诊断中的应用评价。

Q2 Medicine Medical Journal of the Islamic Republic of Iran Pub Date : 2023-08-14 eCollection Date: 2023-01-01 DOI:10.47176/mjiri.37.87
Fatemeh Maleki, Lame Akhlaghi, Fatemeh Tabatabaie
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引用次数: 0

摘要

背景:棘球蚴病是一种慢性人畜共患疾病,在世界范围内均有分布,由棘球蚴蠕虫幼虫期引起。Dot-ELISA能快速准确地诊断棘球蚴病。此外,与目前使用的其他棘球蚴病检测不同,这种快速且价格合理的酶免疫测定法非常保守血清和抗原,只需要纳米级的寄生虫抗原。方法:采用CIEP法、ELISA法和Dot-ELISA法,从棘球蚴囊液中提取粗抗原和B抗原,对人棘球蚴病进行诊断。从德黑兰的屠宰场采集感染了棘球蚴的肝脏,以制备不同阶段的囊肿液。在提取和纯化半胱氨酸后,将其在4ºc下离心,然后准备浓缩。本研究还包括棘球蚴病(n=60)血清、蠕虫寄生虫(n=55)、筋膜炎(n=35)、弓线虫病(n=20)和阴性对照(n=35。所有统计分析均使用Windows 25.0版社会科学统计软件包(SPSS股份有限公司,Chicago,IL,USA)进行。结果:使用ELISA方法,棘球蚴粗抗原的特异性为76.7%,敏感度为93.3%,使用相同方法,B抗原的特异性为96.7%,敏感率为88.3%。用CIEP检测棘球蚴粗抗原的特异性为68.9%,敏感性为86.7%。使用相同的方法,B抗原显示出87.8%的特异性和83.3%的敏感性。用Dot-ELISA法测定血清稀释度为1:800的棘球蚴粗抗原的特异性为83.3%,灵敏度为100%,用同样的方法测定血清稀释率为1:800血清的B抗原的特异性为100%,灵敏度为98.3%。结果表明,B抗原对Dot-ELISA法诊断棘球蚴病具有最大的特异性。结论:棘球蚴的症状多种多样。可能不存在接触受感染动物的历史。诊断它需要高度的临床怀疑,结合细致的病史和实验室调查支持的临床检查。具有天然抗原B的Dot-ELISA系统是一种可行的免疫诊断人类棘球蚴病的方法,该方法优于感染。
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Evaluation of Hydatid Cyst Antigen for Serological Diagnosis.

Background: Hydatidosis, a chronic zoonotic disease, has a distribution worldwide and is caused by the larval stage of the Echinococcus helminth. The Dot-ELISA test can diagnose hydatidosis quickly and accurately. Additionally, unlike other hydatid disease tests now used, this quick and affordable enzyme immunoassay is very serum-conservative and antigen-conservative, needing just nanogram levels of parasite antigen.

Methods: In the present cross-sectional study, crude and B antigens of hydatid cyst fluid were obtained to diagnose human hydatidosis using CIEP (Counter Immunoelectrophoresis), ELISA (Enzyme-linked Immuno Sorbent assay), and Dot- ELISA (Dot Enzyme linked Immuno Sorbent Assay) methods. Infected liver with a hydatid cyst was collected from Tehran's slaughterhouses to prepare cyst fluid in different stages. After extracting and purifying the Cyst fluid, it is centrifuged at 4ºc, then prepared to concentrate. The study also included sera from hydatidosis (n=60), samples of helminth parasites (n=55), fascioliasis (n=35), toxocariasis (n=20) and negative control (n=35) were tested by CIEP (Counter Immunoelectrophoresis), ELISA (Enzyme-linked Immune Sorbent assay), and Dot- ELISA (Dot Enzyme linked Immuno Sorbent Assay) methods. All statistical analyses were performed using Statistical Package for the Social Sciences (SPSS) for Windows release 25.0 (SPSS Inc., Chicago, IL, USA).

Results: Crude antigen of hydatid cyst showed a specificity of 76.7%, a sensitivity of 93.3% using the ELISA method, and B antigen showed a specificity of 96.7% and sensitivity of 88.3% using the same method. The crude antigen of the hydatid cyst exhibited a specificity of 68.9% and a sensitivity of 86.7% using CIEP. The B antigen showed a specificity of 87.8% and sensitivity of 83.3% using the same method.The crude antigen of hydatid cyst having serum dilution at 1:800 exhibited a specificity of 83.3% and sensitivity of 100% using the Dot-ELISA method and B antigen having serum dilution at 1:800 serum showed a specificity of 100% and sensitivity of 98.3% using the same method. The results of this finding showed that B antigen has the maximum specificity to diagnose hydatid test using the Dot- ELISA method.

Conclusion: Hydatid cysts present with varied symptomatology. History of exposure to infected animals may not be present. A high degree of clinical suspicion combined with meticulous history and clinical examination supported by laboratory investigations are required for its diagnosis. The Dot-ELISA system with native antigen B is a viable approach for the immunodiagnosis of human hydatidosis that is preferred to infection.

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CiteScore
2.40
自引率
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发文量
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审稿时长
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