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新型非甾体抗炎药甲布芬在人体中的血浆蛋白结合情况。

Plasma protein binding of metbufen, a new non-steroid anti-inflammatory drug, in humans.

作者信息

Brunner F, Zini R, Tillement J P

出版信息

Int J Clin Pharmacol Ther Toxicol. 1984 Mar;22(3):134-9.

PMID:6201451
Abstract

The binding of 14C-metbufen to human serum albumin and to plasma of cirrhotic patients was measured by equilibrium dialysis at 37 degrees C, pH = 7.4. Between 0.37-373 microM, binding of metbufen to human serum is linear and 99% complete. HSA is the only binding protein with two classes of saturable binding sites. The binding parameters are n1 = 3-5; K1 = 40000 M-1; n2 = 5-8; K2 = 2000 M-1 and n1 = 2; K1 = 148000 M-1, n2 = 7.5; K2 = 2800 M-1 to serum (600 microM HSA) and HSA (600 microM), respectively. The higher affinity constants of pure commercial HSA than found in serum and the lower number of binding sites are thought to be due to albumin polymerization in commercial HSA. In plasma from cirrhotic patients (total bilirubin: 232 microM; HSA = 450 microM), at 7.5 and 30 microM, metbufen-free fractions increased from 1.4 to 2.4% and 1.3 to 3.6%, respectively. At 2 or 8 micrograms/ml, metbufen is not displaced by salicylic acid (300 micrograms/ml), CPIB (200 micrograms/ml), furosemide (2 micrograms/ml), itanoxone (20 micrograms/ml), tolbutamide (100 micrograms/ml), warfarin (3 micrograms/ml), or diazepam (0.75 micrograms/ml). Finally, metbufen interacts with both the diazepam and warfarin binding sites of HSA to some degree.

摘要

在37℃、pH = 7.4条件下,通过平衡透析法测定了14C-美布洛芬与人血清白蛋白及肝硬化患者血浆的结合情况。在0.37 - 373微摩尔之间,美布洛芬与人血清的结合呈线性,且99%完成结合。人血清白蛋白(HSA)是唯一具有两类可饱和结合位点的结合蛋白。结合参数分别为:血清(600微摩尔HSA)时,n1 = 3 - 5;K1 = 40000 M-1;n2 = 5 - 8;K2 = 2000 M-1;HSA(600微摩尔)时,n1 = 2;K1 = 148000 M-1,n2 = 7.5;K2 = 2800 M-1。纯商业HSA的亲和力常数高于血清中的,结合位点数却低于血清中的,这被认为是由于商业HSA中白蛋白发生了聚合。在肝硬化患者的血浆中(总胆红素:232微摩尔;HSA = 450微摩尔),在7.5微摩尔和30微摩尔时,美布洛芬的游离分数分别从1.4%增加到2.4%和从1.3%增加到3.6%。在2微克/毫升或8微克/毫升时,美布洛芬不会被水杨酸(300微克/毫升)、氯贝丁酯(200微克/毫升)、呋塞米(2微克/毫升)、伊他诺酮(20微克/毫升)、甲苯磺丁脲(100微克/毫升)、华法林(3微克/毫升)或地西泮(0.75微克/毫升)置换。最后,美布洛芬在一定程度上与HSA的地西泮和华法林结合位点相互作用。

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