The experimental spectra are compared with theoretical spectra calculated by PF-736 using density functional theory for GMP and the other purine-containing nucleotides, adenosine 5′-monophosphate,
and adenosine 5′-triphosphate. The N K-edge XANES spectra for all of these nucleotides are classified by the numbers of N atoms with particular chemical bonding characteristics in the purine moiety. (C) 2014 AIP Publishing LLC.”
“Raloxifene is an antiestrogen marketed for the treatment of osteoporosis. The major metabolic pathway of raloxifene is glucuronidation at 6- and/or 4′-positions, which is mainly catalyzed by UDP-glucuronosyltransferase 1A8 (UGT1A8) expressed in extrahepatic tissues such as the small intestine and colon. Two non-synonymous allelic variants, termed UGT1A8(*)2 (518C > G, A173G)
and UGT1A8(*)3 (830G>A, C277Y), have been found in Caucasian, African-American and Asian populations. In this study, the effect of amino acid substitutions in UGT1A8 on raloxifene glucuronidation was studied using recombinant UGT1A8 enzymes of wild-type (UGT1A8.1) and variant UGT1A8 (UGT1A8.2 and UGT1A8.3) expressed in Sf9 cells. Raloxifene 6- and 4′-glucuronidation by UGT1A8.1 exhibited negative allosteric kinetics. The K-m and V-max values of UGT1A8.1 were 15.0 mu M and 111 pmol/min/mg protein for 6-glucuronidation, and 9.35 mu M and 232 pmol/min/mg BI-2536 protein for 4′-glucuronidation, respectively. The kinetics
of raloxifene 6-glucuronidation by UGT1A8.2 was positive allosteric, whereas the kinetics of raloxifene 4′-glucuronidation was negative allosteric. The S-50 value of raloxifene 6-glucuronidation was markedly low (1.2%) compared with the K-m value of UGT1A8.1, and the K-m value for raloxifene 4′-glucuronidation was 29% that of UGT1A8.1. The V-max value for raloxifene 6-glucuronidation by UGT1A8.2 was comparable to that of UGT1A8.1, whereas the V-max value for raloxifene 4′-glucuronidation was significantly lower (54%) than that of UGT1A8.1. The activities of raloxifene 6- and 4′-glucuronidation in UGT1A8.3 were markedly lower than those of UGT1A8.1. In mycopthenolic acid glucuronidation, the kinetics by wild-type and variant UGT1A8s fitted the Michaelis-Menten model. The K-m and V-max values of UGT1A8.1 JQ-EZ-05 were 123 mu M and 4820 pmol/min/mg protein, respectively. The K-m and V-max values of UGT1A8.2 were comparable to those of UGT1A8.1. The K-m value of UGT1A8.3 was similar to that of UGT1A8.1, whereas the V-max value was reduced to 2.4% of UGT1A8.1. These findings suggest that A173G and C277Y substitutions of UGT1A8 change the metabolic ability toward raloxifene, and that the polymorphic alleles of UGT1A8 may influence the clinical response and bioavailability of medicines metabolized mainly by UGT1A8. (C) 2013 Elsevier B.V. All rights reserved.”
“The PmPR10-1.