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Detection of Severe Acute Respiratory Syndrome (SARS) Coronavirus Nucleocapsid Protein in SARS Patients by Enzyme-Linked Immunosorbent Assay

机译:酶联免疫吸附法检测SARS患者严重急性呼吸系统综合症(SARS)冠状病毒核蛋白

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摘要

We report the development of an enzyme-linked immunosorbent assay (ELISA) for the detection of severe acute respiratory syndrome (SARS) coronavirus (CoV) nucleocapsid protein. The assay was carried out with hyperimmune polyclonal nucleocapsid-specific antibodies from guinea pigs and rabbits immunized with recombinant His6-tagged SARS CoV nucleocapsid protein. The assay was used for the detection of SARS CoV nucleocapsid protein in nasopharyngeal aspirate, urine, and fecal samples collected from patients with confirmed SARS between days 2 and 33 after the onset of illness. The ELISA was capable of detecting this protein in SARS CoV cell culture lysates at 15 50% tissue culture infective doses/ml but did not produce positive signals when tested with cell culture lysates of human coronaviruses OC43 and 229E. When tested with 120 nasopharyngeal aspirate, 100 urine, and 100 fecal specimens from hospitalized patients without SARS, the assay was shown to have high specificities—96.7, 99, and 96%, respectively. In an evaluation of clinical specimens from SARS patients, 34 (52%) of 66 nasopharyngeal aspirate samples from 50 patients, 5 (5%) of 94 urine samples from 94 patients, and 36 (55%) of 65 fecal samples from 65 patients tested positive for SARS CoV nucleocapsid protein. Nucleocapsid protein could be detected from days 6 to 24 in nasopharyngeal aspirate specimens, from days 11 to 31 in urine specimens, and from days 8 to 32 in fecal specimens after the onset of illness. Moreover, the protein could be detected in 25 (83%) of 30 nasopharyngeal aspirate specimens obtained from days 11 to 15 and in all 7 fecal specimens obtained from days 21 to 32. Since the present ELISA is more convenient and economical than reverse transcription-PCR, it may serve as an alternative tool for the early diagnosis of SARS CoV infection in laboratories with limited resources and expertise and for mass screening for the reservoir of SARS CoV. Further studies on serial clinical specimens should reveal the duration of nucleocapsid protein shedding and may reveal a higher detection rate in SARS patients.
机译:我们报告发展用于检测严重急性呼吸系统综合症(SARS)冠状病毒(CoV)核衣壳蛋白的酶联免疫吸附测定(ELISA)的发展。用重组His6标签的SARS CoV核衣壳蛋白免疫的豚鼠和家兔的超免疫多克隆核衣壳特异性抗体进行测定。该检测方法用于在疾病发作后第2天至第33天之间从确诊为SARS的患者中收集的鼻咽抽吸物,尿液和粪便中检测SARS CoV核衣壳蛋白。 ELISA能够以15 50%组织培养物感染剂量/ ml在SARS CoV细胞培养物裂解物中检测到该蛋白质,但在用人冠状病毒OC43和229E的细胞培养物裂解物进行测试时,则不会产生阳性信号。当对120例无SARS住院患者的鼻咽抽吸物,100尿液和100粪便标本进行测试时,该方法具有很高的特异性-分别为96.7%,99%和96%。在对SARS患者的临床标本进行评估时,来自50位患者的66份鼻咽抽吸物样本中有34张(52%),来自94位患者的94份尿样中有5张(5%)和来自65位患者的65份粪便样本中有36张(55%)检测出SARS CoV核衣壳蛋白呈阳性。在发病后的鼻咽抽吸物标本中,从第6至24天,尿液标本中的第11至31天,以及粪便标本中的第8至32天都可以检测到核蛋白。此外,在11到15天获得的30份鼻咽抽吸物标本和21到32天获得的所有7份粪便标本中,有25份(83%)可以检测到这种蛋白质。 PCR,它可以作为资源和专业知识有限的实验室中早期诊断SARS CoV感染的替代工具,以及大规模筛选SARS CoV储库的工具。对系列临床标本的进一步研究应揭示核衣壳蛋白脱落的持续时间,并可能显示出SARS患者的检出率更高。

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