Use of Recombinant CP2 and CP23 Antigens of Cryptosporidium parvum for Serodiagnosis of Human Cryptosporidiosis

Q2 Biochemistry, Genetics and Molecular Biology
G. Barzegar, E. Ahmadpour, B. Shahriari, R. Solgi, M. Motazedian
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Abstract

Background: Cryptosporidium parvum is an important coccidian parasite infecting many mammals, including human. This parasite can manifest as chronic severe diarrhea in immunocompromised individuals, especially those with AIDS. The present study reports the recombinant production of rP2 and rP23 antigens of C. parvum as antigens for detecting human cryptosporidiosis using indirect ELISA tests. Methods: The coding sequences of rP2 and rP23 proteins were codon-optimized, commercially synthesized and sub-cloned in the pET28a expression vector. The expressed proteins were purified by Ni-NTA column chromatography and confirmed by Western blotting. The efficacy of rP2/rP23 proteins for serodiagnosis was evaluated by positive (n = 20) and negative (n = 20) human sera, confirmed by the Ziehl-Neelsen staining as the gold standard test. Results: In ELISA test, the sera from C. parvum-infected patients reacted strongly to rP2/rP23. The sensitivity and specificity related to the diagnostic potential of rP2/rP23 in the ELISA assay were 100%. Conclusion: Our results showed that combination of rP23 and rP2 antigens in ELISA significantly increases the performance of C. parvum serodiagnosis in human cryptosporidiosis.
重组小隐孢子虫CP2和CP23抗原在人隐孢子虫病血清诊断中的应用
背景:微小隐孢子虫是一种重要的球虫寄生虫,感染包括人类在内的许多哺乳动物。这种寄生虫在免疫功能低下的个体中表现为慢性严重腹泻,尤其是艾滋病患者。本研究报道了用间接ELISA法检测人隐孢子虫病的重组细小隐孢子虫rP2和rP23抗原。方法:对rP2和rP23蛋白的编码序列进行密码子优化,商业合成并亚克隆到pET28a表达载体中。表达的蛋白质通过Ni-NTA柱色谱法纯化并通过蛋白质印迹法确认。rP2/rP23蛋白用于血清诊断的效力通过阳性(n=20)和阴性(n=20。结果:在ELISA检测中,细小念珠菌感染者血清对rP2/rP23反应强烈。与rP2/rP23在ELISA检测中的诊断潜力相关的敏感性和特异性为100%。结论:rP23和rP2抗原联合应用能显著提高细小隐孢子虫病的血清学诊断效果。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Iranian Biomedical Journal
Iranian Biomedical Journal Biochemistry, Genetics and Molecular Biology-Biochemistry, Genetics and Molecular Biology (all)
CiteScore
3.20
自引率
0.00%
发文量
42
审稿时长
8 weeks
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