PT - JOURNAL ARTICLE AU - Girard-Bock, Camille AU - Benoit-Biancamano, Marie-Odile AU - Villeneuve, Lyne AU - Desjardins, Sylvie AU - Guillemette, Chantal TI - A Rare <em>UGT2B7</em> Variant Creates a Novel N-Glycosylation Site at Codon 121 with Impaired Enzyme Activity AID - 10.1124/dmd.116.071860 DP - 2016 Dec 01 TA - Drug Metabolism and Disposition PG - 1867--1871 VI - 44 IP - 12 4099 - http://dmd.aspetjournals.org/content/44/12/1867.short 4100 - http://dmd.aspetjournals.org/content/44/12/1867.full SO - Drug Metab Dispos2016 Dec 01; 44 AB - The UDP glucuronosyltransferase (UGT) superfamily comprises glycoproteins that reside in the endoplasmic reticulum membranes and that undergo post-translational modifications (PTMs). UGT2B7 is of particular interest because of its action on a wide variety of drugs. Most studies currently survey common variants and examine only a small fraction of the genetic diversity; however, rare variants (frequency &lt;1%) might have a significant effect because they are predicted to greatly outnumber common variants in the human genome. We discovered a rare single nucleotide UGT2B7 variant of potential pharmacogenetic relevance that encodes a nonconservative amino acid substitution at codon 121. This low-frequency variation, found in two individuals of a population of 305 healthy volunteers, leads to the translation of an asparagine instead of an aspartic acid (UGT2B7 p.D121N). This amino acid change was predicted to create a putative N-glycosylation motif NX(S/T) subsequently validated upon endoglycosidase H treatment of microsomal fractions and inhibition of N-glycosylation of endogenously produced UGT2B7 with tunicamycin in human embryonic kidney (HEK293) cells. The presence of an additional N-linked glycan on the UGT2B7 enzyme, likely affecting proper protein folding, resulted in a significant decrease of 49% and 40% in the formation of zidovudine and mycophenolic acid glucuronides, respectively. A systematic survey of the Short Genetic Variations database uncovered 32 rare, naturally occurring missense variations predicted to create or disrupt N-glycosylation sequence motifs in the other UGT2B enzymes. Collectively, these variants have the potential to increase the proportion of variance explained in the UGT pathway resulting from changes in PTMs, such as N-linked glycosylation with consequences on drug metabolism.