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使用链霉亲和素 - 生物素化聚糖作为表征凝集素寡糖结合特异性的工具。

The use of streptavidin-biotinylglycans as a tool for characterization of oligosaccharide-binding specificity of lectin.

作者信息

Shao M C

机构信息

Department of Biochemistry, Shanghai Medical University, People's Republic of China.

出版信息

Anal Biochem. 1992 Aug 15;205(1):77-82. doi: 10.1016/0003-2697(92)90581-q.

DOI:10.1016/0003-2697(92)90581-q
PMID:1443561
Abstract

A new rapid and sensitive method for characterizing lectin specificity using streptavidin-biotinylglycans as a tool is presented. This assay is analogous to enzyme immunoassay and takes advantage of the strong, irreversible adsorption of streptavidin to the wells of the chambers of titer plates. A series of streptavidin-biotinylglycans was first coated on a microtiter plate, and then one of six lectins, concanavalin A, wheat germ agglutinin, Phaseolus vulgaris (red kidney bean) erythro-agglutinin, Lens culinaris (lentil) agglutinin, Datura stramoniun agglutinin, or Sambucus nigra (elderberry bark) agglutinin coupled to horseradish peroxidase, was added. After incubation and thorough washing, only the lectin bound to a complementary glycan remained and could be detected and quantified by the peroxidase reaction. It was established that the lectins retained their oligosaccharide-binding specificities after coupling to the peroxidase, that the binding was inhibited by addition of the corresponding sugar inhibitors, and that the color intensity produced by the enzyme reaction is proportional to the amount of lectin-peroxidase bound to biotinylglycan complexed with streptavidin immobilized on the plate. As an example, it was found that the peroxidase-D. stramoniun agglutinin conjugate strongly bound biotinylglycans, GlcNAc3-Man5-R, GalGlcNAc3Man5-R, and GlcNAc3-4Man3-R (R = GlcNAc2-[6-(biotinamido)hexanoyl]-Asn). As little as 10 pmol/ml of lectin was detected. With the growing availability of biotinylglycans, the method should represent a reliable and simple procedure for screening lectin-oligosaccharide recognition qualitatively and quantitatively.

摘要

本文介绍了一种使用链霉亲和素 - 生物素化聚糖作为工具来表征凝集素特异性的快速灵敏新方法。该检测方法类似于酶免疫测定法,利用了链霉亲和素对滴定板孔的强不可逆吸附。首先将一系列链霉亲和素 - 生物素化聚糖包被在微量滴定板上,然后加入六种凝集素之一,即与辣根过氧化物酶偶联的伴刀豆球蛋白A、麦胚凝集素、菜豆(红芸豆)红细胞凝集素、小扁豆凝集素、曼陀罗凝集素或接骨木(接骨木树皮)凝集素。孵育并彻底洗涤后,仅与互补聚糖结合的凝集素留存下来,可通过过氧化物酶反应进行检测和定量。结果表明,凝集素与过氧化物酶偶联后仍保留其寡糖结合特异性,加入相应的糖抑制剂可抑制结合,并且酶反应产生的颜色强度与结合到固定在板上的与链霉亲和素复合的生物素化聚糖上的凝集素 - 过氧化物酶量成正比。例如,发现过氧化物酶 - 曼陀罗凝集素缀合物能强烈结合生物素化聚糖GlcNAc3 - Man5 - R、GalGlcNAc3Man5 - R和GlcNAc3 - 4Man3 - R(R = GlcNAc2 - [6 - (生物素酰胺基)己酰基] - Asn)。检测到的凝集素浓度低至10 pmol/ml。随着生物素化聚糖的可得性不断增加,该方法应代表一种可靠且简单的程序,用于定性和定量筛选凝集素 - 寡糖识别。

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