首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Enzyme-Linked Immunosorbent Assay for Detection of Hepatitis A Antigen in Stool and Antibody to Hepatitis A Antigen in Sera: Comparison with Solid-Phase Radioimmunoassay Immune Electron Microscopy and Immune Adherence Hemagglutination Assay
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Enzyme-Linked Immunosorbent Assay for Detection of Hepatitis A Antigen in Stool and Antibody to Hepatitis A Antigen in Sera: Comparison with Solid-Phase Radioimmunoassay Immune Electron Microscopy and Immune Adherence Hemagglutination Assay

机译:酶联免疫吸附法检测粪便中的甲型肝炎抗原和血清中甲型肝炎抗原的抗体:与固相放射免疫测定免疫电子显微镜和免疫粘附血凝测定的比较

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摘要

Previously described techniques for detection of hepatitis A antigen (HA Ag) and antibody (anti-HA) have required purified HA Ag and expensive equipment. Herein is described an enzyme-linked immunosorbent assay (ELISA) for specific detection of HA Ag in human stool filtrates and of anti-HA in sera by using selected HA Ag-containing human stool filtrates as the antigen source. Because human stools often react nonspecifically in serological tests for HA Ag, blocking with preexposure and hyperimmune anti-HA sera from a chimpanzee inoculated with hepatitis A virus was used to confirm specific detection of HA Ag. The sensitivity of ELISA was found to be comparable to that of solid-phase radioimmunoassay (SPRIA) and immune electron microscopy (IEM). Of 37 acute-phase stools collected from nine patients, 16 were positive for HA Ag by ELISA. In 13 of these, HA Ag particles were found by IEM, and an additional 3 stools negative by ELISA contained HA Ag particles by IEM. Eight control stools were negative by both ELISA and IEM. Anti-HA was measured in sera by demonstrating its ability to block binding of the enzyme conjugate to HA Ag in a stool without detectable nonspecificity. This test (blocking ELISA) was as sensitive and specific as blocking SPIRA, IEM, and immune adherence hemagglutination and, like SPRIA and IEM, detected early-developing antibody. The ELISA is simple to perform and requires only a minimum of equipment. It is useful for screening stools for HA Ag and for monitoring HA Ag during purification, as well as for detecting early and late anti-HA in sera.
机译:先前描述的用于检测甲型肝炎抗原(HA Ag)和抗体(抗HA)的技术需要纯化的HA Ag和昂贵的设备。本文描述了一种酶联免疫吸附测定(ELISA),其通过使用选择的含HA Ag的人粪便滤液作为抗原源来特异性检测人粪便滤液中的HA Ag和血清中的抗HA。由于人类粪便在针对HA Ag的血清学测试中通常会发生非特异性反应,因此可以使用预先暴露的疫苗和来自接种甲型肝炎病毒的黑猩猩的超免疫抗HA血清进行阻断,以确认对HA Ag的特异性检测。发现ELISA的灵敏度与固相放射免疫测定(SPRIA)和免疫电子显微镜(IEM)相当。从9名患者收集的37份急性期大便中,有16份通过ELISA检测出HA Ag阳性。在其中的13个中,通过IEM发现了HA Ag颗粒,另外3个通过ELISA呈阴性的粪便通过IEM发现了HA Ag颗粒。 ELISA和IEM对8个对照粪便均呈阴性。通过证明其在粪便中阻止酶偶联物与HA Ag结合的能力而无可检测的非特异性,来测定血清中的抗HA。该测试(阻断ELISA)与阻断SPIRA,IEM和免疫粘附血凝反应一样灵敏,特异,并且像SPRIA和IEM一样,检测到了早期抗体。 ELISA操作简单,只需要最少的设备。它可用于筛查粪便中的HA Ag,并在纯化过程中监测HA Ag,以及检测血清中的早期和晚期抗HA。

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