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Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants

Polymorphic expression of CYP2D6 contributes to the wide range of activity observed for this clinically important drug metabolizing enzyme. In this report we describe novel CYP2D7/2D6 hybrid genes encoding non-functional and functional CYP2D6 protein and a CYP2D7 variant that mimics a CYP2D7/2D6 hyb...

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Autores principales: Gaedigk, Andrea, Jaime, Lazara Karelia Montane, Bertino, Joseph S., Bérard, Anick, Pratt, Victoria M., Bradfordand, L. DiAnne, Leeder, J. Steven
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Research Foundation 2010
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3153001/
https://www.ncbi.nlm.nih.gov/pubmed/21833166
http://dx.doi.org/10.3389/fphar.2010.00121
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author Gaedigk, Andrea
Jaime, Lazara Karelia Montane
Bertino, Joseph S.
Bérard, Anick
Pratt, Victoria M.
Bradfordand, L. DiAnne
Leeder, J. Steven
author_facet Gaedigk, Andrea
Jaime, Lazara Karelia Montane
Bertino, Joseph S.
Bérard, Anick
Pratt, Victoria M.
Bradfordand, L. DiAnne
Leeder, J. Steven
author_sort Gaedigk, Andrea
collection PubMed
description Polymorphic expression of CYP2D6 contributes to the wide range of activity observed for this clinically important drug metabolizing enzyme. In this report we describe novel CYP2D7/2D6 hybrid genes encoding non-functional and functional CYP2D6 protein and a CYP2D7 variant that mimics a CYP2D7/2D6 hybrid gene. Five-kilobyte-long PCR products encompassing the novel genes were entirely sequenced. A quantitative assay probing in different gene regions was employed to determine CYP2D6 and 2D7 copy number variations and the relative position of the hybrid genes within the locus was assessed by long-range PCR. In addition to the previously known CYP2D6*13 and *66 hybrids, we describe three novel non-functional CYP2D7-2D6 hybrids with gene switching in exon 2 (CYP2D6*79), intron 2 (CYP2D6*80), and intron 5 (CYP2D6*67). A CYP2D7-specific T-ins in exon 1 causes a detrimental frame shift. One subject revealed a CYP2D7 conversion in the 5′-flanking region of a CYP2D6*35 allele, was otherwise unaffected (designated CYP2D6*35B). Finally, three DNAs revealed a CYP2D7 gene with a CYP2D6-like region downstream of exon 9 (designated CYP2D7[REP6]). Quantitative copy number determination, sequence analyses, and long-range PCR mapping were in agreement and excluded the presence of additional gene units. Undetected hybrid genes may cause over-estimation of CYP2D6 activity (CYP2D6*1/*1 vs *1/hybrid, etc), but may also cause results that may interfere with the genotype determination. Detection of hybrid events, “single” and tandem, will contribute to more accurate phenotype prediction from genotype data.
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spelling pubmed-31530012011-08-10 Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants Gaedigk, Andrea Jaime, Lazara Karelia Montane Bertino, Joseph S. Bérard, Anick Pratt, Victoria M. Bradfordand, L. DiAnne Leeder, J. Steven Front Pharmacol Pharmacology Polymorphic expression of CYP2D6 contributes to the wide range of activity observed for this clinically important drug metabolizing enzyme. In this report we describe novel CYP2D7/2D6 hybrid genes encoding non-functional and functional CYP2D6 protein and a CYP2D7 variant that mimics a CYP2D7/2D6 hybrid gene. Five-kilobyte-long PCR products encompassing the novel genes were entirely sequenced. A quantitative assay probing in different gene regions was employed to determine CYP2D6 and 2D7 copy number variations and the relative position of the hybrid genes within the locus was assessed by long-range PCR. In addition to the previously known CYP2D6*13 and *66 hybrids, we describe three novel non-functional CYP2D7-2D6 hybrids with gene switching in exon 2 (CYP2D6*79), intron 2 (CYP2D6*80), and intron 5 (CYP2D6*67). A CYP2D7-specific T-ins in exon 1 causes a detrimental frame shift. One subject revealed a CYP2D7 conversion in the 5′-flanking region of a CYP2D6*35 allele, was otherwise unaffected (designated CYP2D6*35B). Finally, three DNAs revealed a CYP2D7 gene with a CYP2D6-like region downstream of exon 9 (designated CYP2D7[REP6]). Quantitative copy number determination, sequence analyses, and long-range PCR mapping were in agreement and excluded the presence of additional gene units. Undetected hybrid genes may cause over-estimation of CYP2D6 activity (CYP2D6*1/*1 vs *1/hybrid, etc), but may also cause results that may interfere with the genotype determination. Detection of hybrid events, “single” and tandem, will contribute to more accurate phenotype prediction from genotype data. Frontiers Research Foundation 2010-10-04 /pmc/articles/PMC3153001/ /pubmed/21833166 http://dx.doi.org/10.3389/fphar.2010.00121 Text en Copyright © 2010 Gaedigk, Jaime, Bertino, Jr., Bérard, Pratt, Bradford and Leeder. http://www.frontiersin.org/licenseagreement This is an open-access article subject to an exclusive license agreement between the authors and the Frontiers Research Foundation, which permits unrestricted use, distribution, and reproduction in any medium, provided the original authors and source are credited.
spellingShingle Pharmacology
Gaedigk, Andrea
Jaime, Lazara Karelia Montane
Bertino, Joseph S.
Bérard, Anick
Pratt, Victoria M.
Bradfordand, L. DiAnne
Leeder, J. Steven
Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title_full Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title_fullStr Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title_full_unstemmed Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title_short Identification of Novel CYP2D7-2D6 Hybrids: Non-Functional and Functional Variants
title_sort identification of novel cyp2d7-2d6 hybrids: non-functional and functional variants
topic Pharmacology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3153001/
https://www.ncbi.nlm.nih.gov/pubmed/21833166
http://dx.doi.org/10.3389/fphar.2010.00121
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