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采用同位素稀释-放射免疫分析法对舒林酸及其代谢产物进行分析。

Analysis of sulindac and metabolites by combined isotope dilution-radioimmunoassay.

作者信息

Hare L E, Ditzler C A, Hichens M, Rosegay A, Duggan D E

出版信息

J Pharm Sci. 1977 Mar;66(3):414-7. doi: 10.1002/jps.2600660324.

Abstract

Sulindac, a new anti-inflammatory agent, and its sulfone and sulfide metabolites were conjugated to bovine serum albumin by the N-hydroxysuccinimide active ester procedure. Antiserum from rabbits immunized with each of these haptens exhibited extensive cross-reactivity, precluding differential analyses of the three species by displacement assay without prior separation. Therefore, an analytical method based on a combination of isotope dilution and radioimmunoassay was devised. A known mixture of the three chemical species, each labeled with tritium, was equilibrated with plasma or urine samples, reisolated chromatographically, and quantitated by binding to an appropriate immunoglobulin. The radiolabeled materials thus served as recovery standards as well as labeled antigens for each displacement assay. Sulindac and each of its metabolites in plasma or urine at concentrations as low as 500 ng/sample were differentially determined by this procedure. However, since an extraction is required, several milliliters of plasma can be used for each sample, thus increasing the actual sensitivity of the assay.

摘要

舒林酸是一种新型抗炎药,其砜和硫化物代谢产物通过N-羟基琥珀酰亚胺活性酯法与牛血清白蛋白偶联。用这些半抗原中的每一种免疫的兔抗血清表现出广泛的交叉反应性,这使得在没有事先分离的情况下通过置换分析对这三种物质进行差异分析变得不可能。因此,设计了一种基于同位素稀释和放射免疫分析相结合的分析方法。将三种化学物质的已知混合物,每种都用氚标记,与血浆或尿液样品平衡,通过色谱法重新分离,并通过与适当的免疫球蛋白结合进行定量。因此,放射性标记的物质既作为回收标准,也作为每次置换分析的标记抗原。通过该方法可以差异测定血浆或尿液中低至500 ng/样品浓度的舒林酸及其每种代谢产物。然而,由于需要进行萃取,每个样品可以使用几毫升血浆,从而提高了测定的实际灵敏度。

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