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Ferutinin stability in human plasma and interaction with human serum albumin.

作者信息

Greige-Gerges H, Diab Y, Farah J, Magdalou J, Haddad C, Ouaini N

机构信息

Holy Spirit University of Kaslik, Faculty of Sciences and Computer Engineering, B.P. 446 Jounieh, Lebanon.

出版信息

Biopharm Drug Dispos. 2008 Mar;29(2):83-9. doi: 10.1002/bdd.589.

DOI:10.1002/bdd.589
PMID:18050264
Abstract

Ferutinin is a potent phytoestrogen extracted from plants of the genus Ferula. The biological activity of this sesquiterpene is associated with the esterification of p-hydroxybenzoic acid with the daucane alcohol, jaeschkeanadiol. A HPLC method was developed to investigate the stability of ferutinin in acidic and basic solutions (pH 1.5 and 9.0, respectively), in buffer (pH 7.4) as well as in serial dilutions of albumin and in human plasma. The degradation of ferutinin was relatively slow at physiological pH 7.4 compared with low or high pH. Ferutinin was fully stable in human plasma as well as in albumin solution and the stability increased with albumin concentration. The binding of ferutinin to albumin was investigated by fluorescence spectroscopy. Ferutinin decreased the fluorescence of HSA and that of the only tryptophan residue located in domain IIA. As a result of the interaction between ferutinin and albumin, the binding of bilirubin decreased. The stability of ferutinin in plasma is attributable to ferutinin-albumin binding.

摘要

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