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作 者:朱其芳[1] 吴耀生[1] 邓勇[1] 周素芳[1]
机构地区:[1]广西医科大学生物化学教研室
出 处:《广西医科大学学报》1999年第5期593-595,共3页Journal of Guangxi Medical University
摘 要:目的:建立白桂木凝集素-HRP夹心法检测唾液中分泌型IgA(SIgA)。方法:制备AHL-HRP作为酶标凝集素,AHL为包被物,确定最适包被浓度及AHL-HRP工作稀释度,夹心酶联检测SIgA,进行检出限、精密度、准确性等实验并制备标准曲线,初步测定71例正常人唾液SIgA含量。结果:AHL-HRP夹心法检测SIgA标准曲线线性检测范围5~337mg/L。本法测定71例健康人唾液SIgA含量为(509.15±296.75)mg/L。其中5份标本批内平均变异7.4%,批间变异10.56%,回收率平均94%。结论:AHL-HRP夹心法测定SIgA的作用模式为AHL→SIgA→AHL-HRP,可用于唾液中的SIgA含量的测定。方法简便、准确、便于推广。Objective:AHL HRP Sandwich assay was developed for the measurement of SIgA Methods:AHL HRP was prepared, and optimum concentration of the coating AHL and working dilution degree of AHL HRP was determined for the measure ment of SIgA with Sandwich enzyme linked assay The working rang of the standard curves,precision and accuracy was performed The standard curves were prepared for SIgA Results:The working range of the standard curves were 5 ̄337mg/L for SIgA respectively The value of SIgA in the saliva of 71 healthy persons was(509 15±296 75) mg/L with the assay Intra assay cv 7 4% Inter assay cv 10 56% Reclamation was 94% Conclusion:The sandwich enzyme linked assay with AHL HRP is simple and precise,and be used in wide range
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