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一种α受体阻滞剂尼麦角林的血浆结合——与血清白蛋白以及天然和修饰的α1-酸性糖蛋白的亲和力

Plasma binding of an alpha-blocking agent, nicergoline--affinity for serum albumin and native and modified alpha 1-acid glycoprotein.

作者信息

Robert L, Migne J, Santonja R, Zini R, Schmid K, Tillement J P

出版信息

Int J Clin Pharmacol Ther Toxicol. 1983 Jun;21(6):271-6.

PMID:6885199
Abstract

The binding of nicergoline, an alpha-blocking drug, by human plasma proteins was studied using gel filtration, polyacrylamide gel electrophoresis, and equilibrium dialysis techniques. 3H-labeled nicergoline added to plasma was eluted together with two major protein fractions, one containing mainly serum albumin, the other glycoproteins such as alpha 1-acid glycoprotein (alpha 1-AG). Equilibrium dialysis experiments with pure human serum albumin and alpha 1-AG as well as with its chemically modified forms, desialylated, carboxymethylated, and both desialylated and carboxymethylated alpha 1-AG gave the following results: nicergoline has about a 4-fold higher affinity for alpha 1-AG than for serum albumin. There are two binding sites per molecule on serum albumin and one on alpha 1-AG. The binding parameters of alpha 1-AG were not significantly modified by desialylation or carboxymethylation. Only desialylated and carboxymethylated alpha 1-AG showed a decreased binding for nicergoline, suggesting conformational modifications induced by these combined treatments. The fact that desialylated alpha 1-AG keeps its affinity for nicergoline suggests the possibility of a selective introduction of this drug in cells possessing the Ashwell-type specific receptor for desialylated alpha 1-AG, for instance hepatocytes. Increased serum alpha 1-AG concentration induced by inflammatory reactions will also modify the distribution of bound nicergoline between serum albumin and alpha 1-AG and as a consequence its half-life and cell distribution.

摘要

采用凝胶过滤、聚丙烯酰胺凝胶电泳和平衡透析技术研究了α受体阻滞剂尼麦角林与人血浆蛋白的结合情况。添加到血浆中的3H标记尼麦角林与两个主要蛋白组分一起被洗脱,一个主要包含血清白蛋白,另一个包含糖蛋白,如α1-酸性糖蛋白(α1-AG)。用纯人血清白蛋白和α1-AG及其化学修饰形式(去唾液酸化、羧甲基化以及去唾液酸化和羧甲基化的α1-AG)进行的平衡透析实验得出以下结果:尼麦角林对α1-AG的亲和力比对血清白蛋白高约4倍。血清白蛋白分子上有两个结合位点,α1-AG上有一个结合位点。去唾液酸化或羧甲基化对α1-AG的结合参数没有显著影响。只有去唾液酸化和羧甲基化的α1-AG对尼麦角林的结合力降低,表明这些联合处理诱导了构象改变。去唾液酸化的α1-AG对尼麦角林仍保持亲和力这一事实表明,有可能将这种药物选择性地引入具有去唾液酸化α1-AG的阿什韦尔型特异性受体的细胞中,例如肝细胞。炎症反应引起的血清α1-AG浓度升高也会改变结合型尼麦角林在血清白蛋白和α1-AG之间的分布,从而改变其半衰期和细胞分布。

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Interindividual differences in the binding of antidepressives to plasma proteins: the role of the variants of alpha 1-acid glycoprotein.
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