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用于测量3',5'-环磷酸腺苷的放射免疫测定法。

Radioimmunoassay for the measurement of adenosine 3',5'-cyclic phosphate.

作者信息

Steiner A L, Kipnis D M, Utiger R, Parker C

出版信息

Proc Natl Acad Sci U S A. 1969 Sep;64(1):367-73. doi: 10.1073/pnas.64.1.367.

Abstract

A sensitive and specific radioimmunoassay for adenosine 3',5'-cyclic phosphate (cyclic AMP) has been developed which allows measurement of the nucleotide in extracts of 5-10 mg of tissue. The radioimmunoassay is sufficiently specific for cyclic AMP to eliminate the need for prior chromatographic separation of the cyclic nucleotide from other tissue nucleotides. The radioimmunoassay system is based upon competition of cyclic AMP with a labeled cyclic AMP derivative of high specific activity for binding sites on an antibody specific for the cyclic nucleotide. Antibody to cyclic AMP was obtained by immunizing rabbits with an antigen prepared by conjugating succinyl cyclic AMP with human serum albumin. A high specific activity derivative of cyclic AMP was prepared by synthesizing succinyl cyclic AMP tyrosine methyl ester (SCAMP-TME) and iodinating the phenolic hydroxyl group of the tyrosine moiety with (125)I. Free and antibody-bound (125)I-SCAMP-TME were separated by precipitation of the antibody-bound fraction with a second antibody (goat anti-rabbit gamma globulin). Displacement of (125)I-SCAMP-TME by unlabeled cyclic AMP when plotted as a semilogarithmic function was linear over a concentration range of 2-100 picomoles. The specificity of the antibody was tested against structurally related nucleotides, nucleosides, and purine bases. All had less than 0.005 per cent of the potency of cyclic AMP in inhibiting (125)I-SCAMP-TME binding. The marked differences in affinity of the various cyclic nucleotides to cyclic AMP antibody would suggest that antibodies can be developed for each of the cyclic nucleotides by the principles used in this work.

摘要

已开发出一种用于测定3',5'-环磷酸腺苷(环磷酸腺苷)的灵敏且特异的放射免疫分析法,该方法可测定5-10毫克组织提取物中的核苷酸。该放射免疫分析法对环磷酸腺苷具有足够的特异性,无需事先从其他组织核苷酸中对环核苷酸进行色谱分离。放射免疫分析系统基于环磷酸腺苷与高比活性的标记环磷酸腺苷衍生物竞争结合环核苷酸特异性抗体上的结合位点。通过用琥珀酰环磷酸腺苷与人血清白蛋白偶联制备的抗原免疫兔,获得了抗环磷酸腺苷抗体。通过合成琥珀酰环磷酸腺苷酪氨酸甲酯(SCAMP-TME)并用(125)I碘化酪氨酸部分的酚羟基,制备了高比活性的环磷酸腺苷衍生物。通过用第二抗体(山羊抗兔γ球蛋白)沉淀抗体结合部分,分离游离的和抗体结合的(125)I-SCAMP-TME。当以半对数函数绘制时,未标记的环磷酸腺苷对(125)I-SCAMP-TME的置换在2-100皮摩尔的浓度范围内呈线性。针对结构相关的核苷酸、核苷和嘌呤碱测试了抗体的特异性。所有这些在抑制(125)I-SCAMP-TME结合方面的效力均低于环磷酸腺苷的0.005%。各种环核苷酸与环磷酸腺苷抗体亲和力的显著差异表明,可根据本研究中使用的原理为每种环核苷酸开发抗体。

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