Morissette C, Goulet J, Lamoureux G
Centre de Recherche en Immunologie, Institut Armand-Frappier, Laval, Québec, Canada.
Appl Environ Microbiol. 1991 Mar;57(3):836-42. doi: 10.1128/aem.57.3.836-842.1991.
A rapid and sensitive screening sandwich enzyme-linked immunosorbent assay (ELISA) was developed for the detection of staphylococcal enterotoxin B (SEB) in cheese by using a highly avid anti-SEB antibody (Ab) as the capture Ab (CAb) and as the biotinylated Ab conjugate. The glutaraldehyde fixation method for the immobilization of CAb on polystyrene dipsticks was superior to the adsorption fixation and the adsorption-glutaraldehyde fixation methods. The glutaraldehyde fixation method resulted in a higher surface-saturating CAb concentration as evaluated by the peroxidase saturation technique and by the ability of the CAb-coated dipstick to discriminate between positive and negative controls (index of discrimination). Of nine blocking agents used alone or in pairs, lysine-human serum albumin, bovine serum albumin, human serum albumin, and gelatin effectively saturated available sites on the CAb-coated dipsticks without causing interference with the antigen-Ab reactions. The addition of 1% polyethylene glycol to the diluent of the biotinylated anti-SEB Ab conjugate improved the detection of SEB. A concentration of 4% polyethylene glycol allowed a 5-min reaction time for the streptavidin-biotin-horseradish peroxidase conjugate. Cheddar cheese homogenate reduced the sensitivity of the SEB assay; however, the sensitivity was restored when 1.6% (wt/vol) of either a nonionic detergent (Mega-9) or two zwitterionic detergents (Zwittergent 3-10 and 3-12 detergent) was added to the diluent. By using the rapid sandwich ELISA, a minimum of 0.5 to 1.0 ng of SEB per ml was detected within 45 min. The whole procedure for the analysis of the cheddar cheese samples was completed within 1 h.(ABSTRACT TRUNCATED AT 250 WORDS)
开发了一种快速灵敏的夹心酶联免疫吸附测定(ELISA)法,用于检测奶酪中的葡萄球菌肠毒素B(SEB)。该方法使用高亲和力的抗SEB抗体(Ab)作为捕获抗体(CAb)和生物素化抗体缀合物。将CAb固定在聚苯乙烯试纸条上的戊二醛固定法优于吸附固定法和吸附-戊二醛固定法。通过过氧化物酶饱和技术以及CAb包被试纸条区分阳性和阴性对照的能力(鉴别指数)评估,戊二醛固定法导致更高的表面饱和CAb浓度。单独或成对使用的九种封闭剂中,赖氨酸-人血清白蛋白、牛血清白蛋白、人血清白蛋白和明胶有效地饱和了CAb包被试纸条上的可用位点,而不会干扰抗原-抗体反应。向生物素化抗SEB抗体缀合物的稀释剂中添加1%聚乙二醇可提高SEB的检测效果。4%聚乙二醇的浓度允许链霉亲和素-生物素-辣根过氧化物酶缀合物有5分钟的反应时间。切达干酪匀浆降低了SEB检测的灵敏度;然而,当向稀释剂中添加1.6%(重量/体积)的非离子去污剂(Mega-9)或两种两性离子去污剂(Zwittergent 3-10和3-12去污剂)时,灵敏度得以恢复。通过使用快速夹心ELISA,在45分钟内可检测到每毫升至少0.5至1.0纳克的SEB。切达干酪样品的整个分析过程在1小时内完成。(摘要截短于250字)