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免疫印迹条上免疫球蛋白的定量分析作为人类免疫缺陷病毒血清学诊断的一种工具。

Quantification of immunoglobulin on electrophoretic immunoblot strips as a tool for human immunodeficiency virus serodiagnosis.

作者信息

Blomberg J, Klasse P J

机构信息

Department of Medical Microbiology, University of Lund, Sweden.

出版信息

J Clin Microbiol. 1988 Jan;26(1):111-5. doi: 10.1128/jcm.26.1.111-115.1988.

Abstract

Electrophoretic immunoblotting (EIB [Western blotting]), the main method for verification of human immunodeficiency virus (HIV) seropositivity, needs thorough characterization and standardization. We explored the possibilities of quantifying immunoglobulin G (IgG) bound to EIB strips both by densitometry of the peroxidase-stained bands and by measurement of radioactivity with labeled anti-HIV IgG. The radioactivity method is inherently more exact but was more cumbersome. However, despite saturation phenomena at high IgG densities, the densitometric method was more convenient and yielded reproducible estimates of the amount of bound IgG. We found it useful primarily for documentation of changes in the relative abundance of antibodies to different HIV proteins from individual patients over time. To explore the potential usefulness of the method, we studied a small set of HIV-seropositive persons. The average p24/gp41 color yield ratios and standard deviations in 3 persons with recent seroconversion, 15 healthy subjects, and 6 diseased HIV-seropositive persons were 6.6 +/- 0.9, 2.3 +/- 1.9, and 1.3 +/- 0.5, respectively. These data are in accord with previous qualitative or semiquantitative observations but are too limited for any conclusions regarding the use of quantitative EIB for prognostic use with individual patients. Quantitative EIB is a valuable tool for comparative methodological studies and for research on the protective role of anti-HIV antibodies in acquired immunodeficiency syndrome pathogenesis. Its possible use in prognostication for individual patients must be evaluated in long-term studies.

摘要

电泳免疫印迹法(EIB[蛋白质印迹法])是验证人类免疫缺陷病毒(HIV)血清阳性的主要方法,需要进行全面的特性描述和标准化。我们探索了通过过氧化物酶染色条带的光密度测定以及用标记的抗HIV IgG测量放射性来定量与EIB条带结合的免疫球蛋白G(IgG)的可能性。放射性方法本质上更精确,但操作更繁琐。然而,尽管在高IgG密度下存在饱和现象,但光密度测定法更方便,并且能对结合的IgG量进行可重复的估计。我们发现它主要有助于记录个体患者随时间推移针对不同HIV蛋白的抗体相对丰度的变化。为了探索该方法的潜在用途,我们研究了一小群HIV血清阳性者。近期血清转化的3人、15名健康受试者和6名患病的HIV血清阳性者的平均p24/gp41颜色产率比及标准差分别为6.6±0.9、2.3±1.9和1.3±0.5。这些数据与先前的定性或半定量观察结果一致,但对于关于使用定量EIB对个体患者进行预后评估的任何结论而言,数据过于有限。定量EIB是比较方法学研究以及研究抗HIV抗体在获得性免疫缺陷综合征发病机制中保护作用的有价值工具。其在个体患者预后评估中的可能用途必须在长期研究中进行评估。

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