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用于检测亚皮克级布鲁氏菌抗原量的尼龙珠酶联免疫吸附测定法。

Nylon bead enzyme-linked immunosorbent assay for detection of sub-picogram quantities of Brucella antigens.

作者信息

Perera V Y, Creasy M T, Winter A J

出版信息

J Clin Microbiol. 1983 Sep;18(3):601-8. doi: 10.1128/jcm.18.3.601-608.1983.

Abstract

An indirect sandwich enzyme-linked immunosorbent assay, using antibody covalently coupled to nylon beads, has been adapted for the detection of Brucella antigens. Optimum conditions were achieved by incubation of 1 ml of reaction mixture with a single bead, and by minimizing nonspecific interactions through the use of beads coated with purified bovine antibodies, preabsorption of third layer rabbit antibodies with normal bovine serum, and treatment of beads with normal goat serum before addition of the goat anti-rabbit enzyme conjugate. Beta-galactosidase was selected for use with clinical samples primarily because of low levels of endogenous enzyme in bovine leukocytes. Use of a fluorogenic substrate enhanced sensitivity 20-fold. Under these conditions, 100 fg of solubilized crude lipopolysaccharide or 8 to 10 Brucella cells was detectable in a fixed volume of 1 ml. A system was also devised for concentrating antigen which permitted ready detection of 2 pg of lipopolysaccharide in a volume of 50 ml (40 fg/ml). Attempts to detect lipopolysaccharide in the presence of concentrated serum or plasma were unsuccessful, but 10 brucellae added to a suspension of leukocytes from 100 ml of normal bovine blood were easily measured.

摘要

一种采用与尼龙珠共价偶联抗体的间接夹心酶联免疫吸附测定法已被用于检测布鲁氏菌抗原。通过将1毫升反应混合物与单个珠子一起孵育,并通过使用包被有纯化牛抗体的珠子、用正常牛血清预吸收第三层兔抗体以及在加入山羊抗兔酶结合物之前用正常山羊血清处理珠子来最小化非特异性相互作用,从而实现了最佳条件。选择β-半乳糖苷酶用于临床样本主要是因为牛白细胞中内源性酶水平较低。使用荧光底物使灵敏度提高了20倍。在这些条件下,在1毫升固定体积中可检测到100飞克溶解的粗脂多糖或8至10个布鲁氏菌细胞。还设计了一种浓缩抗原的系统,该系统能够在50毫升体积(40飞克/毫升)中轻松检测到2皮克脂多糖。在存在浓缩血清或血浆的情况下检测脂多糖的尝试未成功,但向来自100毫升正常牛血的白细胞悬液中加入10个布鲁氏菌很容易被检测到。

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