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首页> 外文期刊>Journal of Clinical Microbiology >Development of a biotin-streptavidin-enhanced enzyme-linked immunosorbent assay which uses monoclonal antibodies for detection of group C rotaviruses.
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Development of a biotin-streptavidin-enhanced enzyme-linked immunosorbent assay which uses monoclonal antibodies for detection of group C rotaviruses.

机译:开发生物素 - 链霉蛋白增强的酶联免疫吸附测定法,其使用单克隆抗体进行C组旋流孔。

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A biotin-streptavidin-enhanced enzyme-linked immunosorbent assay (ELISA) which uses monoclonal antibodies (MAbs) for the detection of group C rotaviruses was developed. An assay in which plates were coated with three pooled MAbs and biotinylated polyclonal immunoglobulin G (IgG) (polyclonal antibody [PAb]) was used as the detector (MAb capture-PAb detector) was found to be the most sensitive and specific of the assays when it was compared with assays in which plates were coated with polyclonal antiserum and detection was done with either biotinylated polyclonal antiserum (PAb capture-PAb detector) or biotinylated pooled MAbs (PAb capture-MAb detector). The MAb capture-PAb detector ELISA detected 83% of samples confirmed to be positive for group C rotaviruses, whereas the PAb capture-PAb detector assay detected 63% of positive samples and the PAb capture-MAb detector assay detected 65% of positive samples. All three procedures detected both of the bovine and the two human group C rotaviruses, but none of the three procedures detected fecal samples containing group A and B rotaviruses or fecal samples negative for group C rotaviruses used in this study. The sensitivity of the MAb capture-PAb detector ELISA was determined by serially diluting fecal group C rotaviruses; antigens were detected in maximal positive dilution ranges of 1:1,000 to 1:3,000 for the samples tested. On the basis of the cell culture immunofluorescence assay infectivity titer of semipurified cell culture-passaged Cowden group C rotavirus, the sensitivity of the MAb capture-PAb detection ELISA for detection of homologous group C rotavirus was 53 fluorescent focus units per ml. Epitope mapping by use of the biotinylated MAbs in competition assay suggested that our MAbs may bind to three different but overlapping epitopes. These results suggest that the MAb capture-PAb detector ELISA can be used to study the epidemiology of group C rotaviruses in humans and animals.
机译:开发了一种使用单克隆抗体(MAb)用于检测C组旋流孔的生物素 - 链霉抗生物素蛋白增强的酶联免疫吸附测定(ELISA)。用三种合并的mAb涂覆板和生物素化的多克隆免疫球蛋白G(IgG)(多克隆抗体[PAB])作为检测器(MAB捕获 - PAB检测器)是最敏感的和特异性的测定的测定当与将板涂覆有多克隆抗血管的测定进行比较时,用生物素化的多克隆抗血清(PAB捕获 - PAB检测器)或生物素化的合并的MAb(PAB捕获-mAb检测器)进行检测。 MAB捕获-Pab检测器ELISA检测了83%的样品,证实是C组旋泻的阳性,而PAB捕获-PAB检测器测定检测63%的阳性样品,并且PAB捕获-MAb检测器测定检测65%的阳性样品。所有三种程序都检测到这两个人组旋泻,但这三种方法都没有检测到含有A组和B旋泻或粪便样品的粪便样品对本研究中使用的C组旋泻的阴性。通过连续稀释粪便基团COTAVIRUS来确定MAB捕获-PAB检测器ELISA的敏感性;对于测试的样品,在最大阳性稀释范围内检测到抗原,其为1:1,000至1:3,000。在基于细胞培养免疫荧光测定滴度滴度滴度的半润泽细胞培养型牛犊组C轮状病毒,MAB捕获-PAB检测ELISA检测同源CORAVIRUS的敏感性为每mL 53荧光焦点单元。通过在竞争测定中使用生物素化的mAbs的表位映射表明我们的mAb可以结合三种不同但重叠的表位。这些结果表明,MAB捕获 - PAB探测器ELISA可用于研究人类和动物群旋流病毒的流行病学。

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