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非同位素和同位素免疫分析中针对可替宁的单克隆抗体和多克隆抗体的比较。

Comparison of monoclonal and polyclonal antibodies to cotinine in nonisotopic and isotopic immunoassays.

作者信息

Bjercke R J, Cook G, Langone J J

出版信息

J Immunol Methods. 1987 Feb 11;96(2):239-46. doi: 10.1016/0022-1759(87)90320-6.

Abstract

Monoclonal antibodies (McAb) were used to develop nonisotopic and radioimmunoassays (RIA) for quantitative determination of the major nicotine metabolite, cotinine, in physiological fluids. ELISAs and fluorescence immunoassays were carried out in microtiter plate wells coated with a conjugate of cotinine 4'-carboxylic acid bound covalently to poly-L-lysine. The detection systems were horseradish peroxidase (HRP)-labeled staphylococcal protein A, HRP-streptavidin-biotin, and biotinylated alkaline phosphatase-4-methylumbelliferyl phosphate. With the three McAb tested, I50 values ranged between 0.024-0.063 ng cotinine and as little as 0.005-0.015 ng gave 15% inhibition. These assays were 5-20 times more sensitive than similar assays using six rabbit antisera. With McAb the standard inhibition curves were steeper and complete inhibition of immune binding was achieved with approximately 1 ng cotinine. In contrast, 100-500 ng cotinine failed to give greater than 80-90% inhibition with rabbit antibodies either in the plate assays or in RIA using a 125I-labeled tyramine derivative of cotinine as the tracer. In this RIA, the sensitivity with McAb (mean I50 of 0.55 ng cotinine) was over three-fold greater than with rabbit antisera (mean I50 of 1.84 ng). The presence of antibodies directed to the amide linkage group common to the polylysine conjugate. 125I-tyramine derivative and the immunogen likely accounts for the inferior quality of assays using rabbit antisera. Consistent with this conclusion, superimposable inhibition curves were obtained in the RIA when monoclonal or rabbit antibodies were used with [3H]cotinine. Cotinine levels in saliva, serum and plasma from smokers and non-smokers determined with McAb-based assays showed a strong correlation with values obtained by RIA using rabbit antisera or by gas chromatography. Properly selected McAb offer distinct advantages over conventional antisera in nonisotopic immunoassays and RIAs for cotinine as a biochemical marker of active or passive smoking.

摘要

单克隆抗体(McAb)被用于开发非同位素免疫分析和放射免疫分析(RIA),以定量测定生理体液中主要的尼古丁代谢物可替宁。酶联免疫吸附测定(ELISA)和荧光免疫测定在包被有与聚-L-赖氨酸共价结合的可替宁4'-羧酸缀合物的微量滴定板孔中进行。检测系统为辣根过氧化物酶(HRP)标记的葡萄球菌蛋白A、HRP-链霉亲和素-生物素以及生物素化碱性磷酸酶-4-甲基伞形酮磷酸酯。在所测试的三种单克隆抗体中,半数抑制浓度(I50)值在0.024 - 0.063 ng可替宁之间,低至0.005 - 0.015 ng可产生15%的抑制率。这些分析比使用六种兔抗血清的类似分析灵敏5 - 20倍。使用单克隆抗体时,标准抑制曲线更陡峭,用约1 ng可替宁可实现免疫结合的完全抑制。相比之下,无论是在平板分析中还是在以125I标记的可替宁酪胺衍生物作为示踪剂的放射免疫分析中,100 - 500 ng可替宁用兔抗体都无法产生大于80 - 90%的抑制率。在这种放射免疫分析中,单克隆抗体的灵敏度(可替宁的平均I50为0.55 ng)比兔抗血清(平均I50为1.84 ng)高逾三倍。针对聚赖氨酸缀合物、125I - 酪胺衍生物和免疫原共有的酰胺连接基团的抗体的存在,可能是使用兔抗血清的分析质量较差的原因。与此结论一致的是,当单克隆抗体或兔抗体与[3H]可替宁一起用于放射免疫分析时,可获得重叠的抑制曲线。用基于单克隆抗体的分析方法测定的吸烟者和非吸烟者唾液、血清和血浆中的可替宁水平,与使用兔抗血清的放射免疫分析或气相色谱法获得的值显示出很强的相关性。在作为主动或被动吸烟生化标志物的可替宁的非同位素免疫分析和放射免疫分析中,正确选择的单克隆抗体比传统抗血清具有明显优势。

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