Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions

Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions

BackgroundThe CYP2D6 gene locus has been extensively studied over decades, yet a portion of variability in CYP2D6 activity cannot be explained by known sequence variations within the gene, copy number variation, or structural rearrangements. It was proposed that rs5758550, located 116 kb downstream...

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Main Authors: Erin C. Boone, Wendy Y. Wang, Roger Gaedigk, Mariana Cherner, Anick Bérard, J. Steven Leeder, Neil A. Miller, Andrea Gaedigk
Format: Article
Language:English
Published: Frontiers Media S.A. 2020-05-01
Series:Frontiers in Pharmacology
Subjects:
CYP2D6
allele definition
enhancer SNP
ddPCR = droplet digital PCR
phasing
Online Access:https://www.frontiersin.org/article/10.3389/fphar.2020.00486/full
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language English
format Article
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author Erin C. Boone
Wendy Y. Wang
Roger Gaedigk
Roger Gaedigk
Mariana Cherner
Anick Bérard
Anick Bérard
J. Steven Leeder
J. Steven Leeder
Neil A. Miller
Neil A. Miller
Andrea Gaedigk
Andrea Gaedigk
spellingShingle Erin C. Boone
Wendy Y. Wang
Roger Gaedigk
Roger Gaedigk
Mariana Cherner
Anick Bérard
Anick Bérard
J. Steven Leeder
J. Steven Leeder
Neil A. Miller
Neil A. Miller
Andrea Gaedigk
Andrea Gaedigk
Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
Frontiers in Pharmacology
CYP2D6
allele definition
enhancer SNP
ddPCR = droplet digital PCR
phasing
author_facet Erin C. Boone
Wendy Y. Wang
Roger Gaedigk
Roger Gaedigk
Mariana Cherner
Anick Bérard
Anick Bérard
J. Steven Leeder
J. Steven Leeder
Neil A. Miller
Neil A. Miller
Andrea Gaedigk
Andrea Gaedigk
author_sort Erin C. Boone
title Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
title_short Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
title_full Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
title_fullStr Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
title_full_unstemmed Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele Definitions
title_sort long-distance phasing of a tentative “enhancer” single-nucleotide polymorphism with cyp2d6 star allele definitions
publisher Frontiers Media S.A.
series Frontiers in Pharmacology
issn 1663-9812
publishDate 2020-05-01
description BackgroundThe CYP2D6 gene locus has been extensively studied over decades, yet a portion of variability in CYP2D6 activity cannot be explained by known sequence variations within the gene, copy number variation, or structural rearrangements. It was proposed that rs5758550, located 116 kb downstream of the CYP2D6 gene locus, increases gene expression and thus contributes to variability in CYP2D6 activity. This finding has, however, not been validated. The purpose of the study was to address a major technological barrier, i.e., experimentally linking rs5758550, also referred to as the “enhancer” single-nucleotide polymorphism (SNP), to CYP2D6 haplotypes >100 kb away. To overcome this challenge is essential to ultimately determine the contribution of the “enhancer” SNP to interindividual variability in CYP2D6 activity.MethodsA large ethnically mixed population sample (n=3,162) was computationally phased to determine linkage between the “enhancer” SNP and CYP2D6 haplotypes (or star alleles). To experimentally validate predicted linkages, DropPhase2D6, a digital droplet PCR (ddPCR)-based method was developed. 10X Genomics Linked-Reads were utilized as a proof of concept.ResultsPhasing predicted that the “enhancer” SNP can occur on numerous CYP2D6 haplotypes including CYP2D6*1, *2, *5, and *41 and suggested that linkage is incomplete, i.e., a portion of these alleles do not have the “enhancer” SNP. Phasing also revealed differences among the European and African ancestry data sets regarding the proportion of alleles with and without the “enhancer” SNP. DropPhase2D6 was utilized to confirm or refute the predicted “enhancer” SNP location for individual samples, e.g., of n=3 samples genotyped as *1/*41, rs5758550 was on the *41 allele of two samples and on the *1 allele of one sample. Our findings highlight that the location of the “enhancer” SNP must not be assigned by “default.” Furthermore, linkage between the “enhancer” SNP and CYP2D6 star allele haplotypes was confirmed with 10X Genomics technology.ConclusionsSince the “enhancer” SNP can be present on a portion of normal, decreased, or no function alleles, the phase of the “enhancer” SNP must be considered when investigating the impact of the “enhancer” SNP on CYP2D6 activity.
topic CYP2D6
allele definition
enhancer SNP
ddPCR = droplet digital PCR
phasing
url https://www.frontiersin.org/article/10.3389/fphar.2020.00486/full
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spelling doaj-95c177f96d5a4f668bb3bb8c21f82b6c2020-11-25T02:40:21ZengFrontiers Media S.A.Frontiers in Pharmacology1663-98122020-05-011110.3389/fphar.2020.00486530539Long-Distance Phasing of a Tentative “Enhancer” Single-Nucleotide Polymorphism With CYP2D6 Star Allele DefinitionsErin C. Boone0Wendy Y. Wang1Roger Gaedigk2Roger Gaedigk3Mariana Cherner4Anick Bérard5Anick Bérard6J. Steven Leeder7J. Steven Leeder8Neil A. Miller9Neil A. Miller10Andrea Gaedigk11Andrea Gaedigk12Division of Clinical Pharmacology, Toxicology and Therapeutic Innovation, Children's Mercy Kansas City, Kansas City, MO, United StatesDivision of Clinical Pharmacology, Toxicology and Therapeutic Innovation, Children's Mercy Kansas City, Kansas City, MO, United StatesDivision of Clinical Pharmacology, Toxicology and Therapeutic Innovation, Children's Mercy Kansas City, Kansas City, MO, United StatesSchool of Medicine, University of Missouri-Kansas City, Kansas City, MO, United StatesDepartment of Psychiatry, University of California, San Diego, La Jolla, CA, United StatesFaculty of Pharmacy, University of Montreal, Montreal, QC, CanadaResearch Center, CHU Sainte-Justine, Montreal, QC, CanadaDivision of Clinical Pharmacology, Toxicology and Therapeutic Innovation, Children's Mercy Kansas City, Kansas City, MO, United StatesSchool of Medicine, University of Missouri-Kansas City, Kansas City, MO, United StatesSchool of Medicine, University of Missouri-Kansas City, Kansas City, MO, United StatesCenter for Pediatric Genomic Medicine, Children's Mercy Kansas City, Kansas City, MO, United StatesDivision of Clinical Pharmacology, Toxicology and Therapeutic Innovation, Children's Mercy Kansas City, Kansas City, MO, United StatesSchool of Medicine, University of Missouri-Kansas City, Kansas City, MO, United StatesBackgroundThe CYP2D6 gene locus has been extensively studied over decades, yet a portion of variability in CYP2D6 activity cannot be explained by known sequence variations within the gene, copy number variation, or structural rearrangements. It was proposed that rs5758550, located 116 kb downstream of the CYP2D6 gene locus, increases gene expression and thus contributes to variability in CYP2D6 activity. This finding has, however, not been validated. The purpose of the study was to address a major technological barrier, i.e., experimentally linking rs5758550, also referred to as the “enhancer” single-nucleotide polymorphism (SNP), to CYP2D6 haplotypes >100 kb away. To overcome this challenge is essential to ultimately determine the contribution of the “enhancer” SNP to interindividual variability in CYP2D6 activity.MethodsA large ethnically mixed population sample (n=3,162) was computationally phased to determine linkage between the “enhancer” SNP and CYP2D6 haplotypes (or star alleles). To experimentally validate predicted linkages, DropPhase2D6, a digital droplet PCR (ddPCR)-based method was developed. 10X Genomics Linked-Reads were utilized as a proof of concept.ResultsPhasing predicted that the “enhancer” SNP can occur on numerous CYP2D6 haplotypes including CYP2D6*1, *2, *5, and *41 and suggested that linkage is incomplete, i.e., a portion of these alleles do not have the “enhancer” SNP. Phasing also revealed differences among the European and African ancestry data sets regarding the proportion of alleles with and without the “enhancer” SNP. DropPhase2D6 was utilized to confirm or refute the predicted “enhancer” SNP location for individual samples, e.g., of n=3 samples genotyped as *1/*41, rs5758550 was on the *41 allele of two samples and on the *1 allele of one sample. Our findings highlight that the location of the “enhancer” SNP must not be assigned by “default.” Furthermore, linkage between the “enhancer” SNP and CYP2D6 star allele haplotypes was confirmed with 10X Genomics technology.ConclusionsSince the “enhancer” SNP can be present on a portion of normal, decreased, or no function alleles, the phase of the “enhancer” SNP must be considered when investigating the impact of the “enhancer” SNP on CYP2D6 activity.https://www.frontiersin.org/article/10.3389/fphar.2020.00486/fullCYP2D6allele definitionenhancer SNPddPCR = droplet digital PCRphasing

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