A SNP panel for identification of DNA and RNA specimens

BIOS consortium

doi:https://doi.org/10.1186/s12864-018-4482-7

A SNP panel for identification of DNA and RNA specimens

BIOS consortium

Research output: Contribution to journal › Article › Academic › peer-review

30 Citations (Scopus)

Abstract

BACKGROUND: SNP panels that uniquely identify an individual are useful for genetic and forensic research. Previously recommended SNP panels are based on DNA profiles and mostly contain intragenic SNPs. With the increasing interest in RNA expression profiles, we aimed for establishing a SNP panel for both DNA and RNA-based genotyping.

RESULTS: To determine a small set of SNPs with maximally discriminative power, genotype calls were obtained from DNA and blood-derived RNA sequencing data belonging to healthy, geographically dispersed, Dutch individuals. SNPs were selected based on different criteria like genotype call rate, minor allele frequency, Hardy-Weinberg equilibrium and linkage disequilibrium. A panel of 50 SNPs was sufficient to identify an individual uniquely: the probability of identity was 6.9 × 10- 20 when assuming no family relations and 1.2 × 10- 10 when accounting for the presence of full sibs. The ability of the SNP panel to uniquely identify individuals on DNA and RNA level was validated in an independent population dataset. The panel is applicable to individuals from European descent, with slightly lower power in non-Europeans. Whereas most of the genes containing the 50 SNPs are expressed in various tissues, our SNP panel needs optimization for other tissues than blood.

CONCLUSIONS: This first DNA/RNA SNP panel will be useful to identify sample mix-ups in biomedical research and for assigning DNA and RNA stains in crime scenes to unique individuals.

Original language	English
Article number	90
Pages (from-to)	90
Journal	BMC Genomics
Volume	19
Issue number	1
DOIs	https://doi.org/10.1186/s12864-018-4482-7
Publication status	Published - 25 Jan 2018

Keywords

Biobanking
Forensics
Genetic variation
Journal Article
Mix up samples
Sample tracking

Cohort Studies

Netherlands Twin Register (NTR)

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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https://doi.org/10.1186/s12864-018-4482-7

Cite this

@article{0854127bfcee4855a18bb655670a920a,

title = "A SNP panel for identification of DNA and RNA specimens",

abstract = "BACKGROUND: SNP panels that uniquely identify an individual are useful for genetic and forensic research. Previously recommended SNP panels are based on DNA profiles and mostly contain intragenic SNPs. With the increasing interest in RNA expression profiles, we aimed for establishing a SNP panel for both DNA and RNA-based genotyping.RESULTS: To determine a small set of SNPs with maximally discriminative power, genotype calls were obtained from DNA and blood-derived RNA sequencing data belonging to healthy, geographically dispersed, Dutch individuals. SNPs were selected based on different criteria like genotype call rate, minor allele frequency, Hardy-Weinberg equilibrium and linkage disequilibrium. A panel of 50 SNPs was sufficient to identify an individual uniquely: the probability of identity was 6.9 × 10- 20 when assuming no family relations and 1.2 × 10- 10 when accounting for the presence of full sibs. The ability of the SNP panel to uniquely identify individuals on DNA and RNA level was validated in an independent population dataset. The panel is applicable to individuals from European descent, with slightly lower power in non-Europeans. Whereas most of the genes containing the 50 SNPs are expressed in various tissues, our SNP panel needs optimization for other tissues than blood.CONCLUSIONS: This first DNA/RNA SNP panel will be useful to identify sample mix-ups in biomedical research and for assigning DNA and RNA stains in crime scenes to unique individuals.",

keywords = "Biobanking, Forensics, Genetic variation, Journal Article, Mix up samples, Sample tracking",

author = "Soheil Yousefi and Tooba Abbassi-Daloii and Thirsa Kraaijenbrink and Martijn Vermaat and Hailiang Mei and {van 't Hof}, Peter and {van Iterson}, Maarten and Zhernakova, {Daria V} and Annique Claringbould and Lude Franke and {'t Hart}, {Leen M} and Slieker, {Roderick C} and {van der Heijden}, Amber and {de Knijff}, Peter and {'t Hoen}, {Peter A C} and {BIOS consortium} and D.I. Boomsma and {van Dongen}, J. and J.J. Hottenga and R. Pool and R. Jansen and {van Meurs}, {J. B.} and Heijmans, {B. T.} and Slagboom, {P. E.} and Suchiman, {H. E.D.} and {van Zwet}, {E. W.} and {van Greevenbroek}, {M. M.} and Stehouwer, {C. D.} and {van der Kallen}, {C. J.} and Schalkwijk, {C. G.} and C. Wijmenga and A. Zhernakova and Tigchelaar, {E. F.} and M. Beekman and J. Deelen and {van Heemst}, D. and Veldink, {J. H.} and {van den Berg}, {L. H.} and {van Duijn}, {C. M.} and Hofman, {B. A.} and Uitterlinden, {A. G.} and Jhamai, {P. M.} and M. Verbiest and M. Verkerk and {van der Breggen}, R. and {van Rooij}, J. and N. Lakenberg and J. Bot and P. Deelen and {van Dijk}, F.",

year = "2018",

month = jan,

day = "25",

doi = "https://doi.org/10.1186/s12864-018-4482-7",

language = "English",

volume = "19",

pages = "90",

journal = "BMC Genomics",

issn = "1471-2164",

publisher = "BioMed Central",

number = "1",

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TY - JOUR

T1 - A SNP panel for identification of DNA and RNA specimens

AU - Yousefi, Soheil

AU - Abbassi-Daloii, Tooba

AU - Kraaijenbrink, Thirsa

AU - Vermaat, Martijn

AU - Mei, Hailiang

AU - van 't Hof, Peter

AU - van Iterson, Maarten

AU - Zhernakova, Daria V

AU - Claringbould, Annique

AU - Franke, Lude

AU - 't Hart, Leen M

AU - Slieker, Roderick C

AU - van der Heijden, Amber

AU - de Knijff, Peter

AU - 't Hoen, Peter A C

AU - BIOS consortium

AU - Boomsma, D.I.

AU - van Dongen, J.

AU - Hottenga, J.J.

AU - Pool, R.

AU - Jansen, R.

AU - van Meurs, J. B.

AU - Heijmans, B. T.

AU - Slagboom, P. E.

AU - Suchiman, H. E.D.

AU - van Zwet, E. W.

AU - van Greevenbroek, M. M.

AU - Stehouwer, C. D.

AU - van der Kallen, C. J.

AU - Schalkwijk, C. G.

AU - Wijmenga, C.

AU - Zhernakova, A.

AU - Tigchelaar, E. F.

AU - Beekman, M.

AU - Deelen, J.

AU - van Heemst, D.

AU - Veldink, J. H.

AU - van den Berg, L. H.

AU - van Duijn, C. M.

AU - Hofman, B. A.

AU - Uitterlinden, A. G.

AU - Jhamai, P. M.

AU - Verbiest, M.

AU - Verkerk, M.

AU - van der Breggen, R.

AU - van Rooij, J.

AU - Lakenberg, N.

AU - Bot, J.

AU - Deelen, P.

AU - van Dijk, F.

PY - 2018/1/25

Y1 - 2018/1/25

N2 - BACKGROUND: SNP panels that uniquely identify an individual are useful for genetic and forensic research. Previously recommended SNP panels are based on DNA profiles and mostly contain intragenic SNPs. With the increasing interest in RNA expression profiles, we aimed for establishing a SNP panel for both DNA and RNA-based genotyping.RESULTS: To determine a small set of SNPs with maximally discriminative power, genotype calls were obtained from DNA and blood-derived RNA sequencing data belonging to healthy, geographically dispersed, Dutch individuals. SNPs were selected based on different criteria like genotype call rate, minor allele frequency, Hardy-Weinberg equilibrium and linkage disequilibrium. A panel of 50 SNPs was sufficient to identify an individual uniquely: the probability of identity was 6.9 × 10- 20 when assuming no family relations and 1.2 × 10- 10 when accounting for the presence of full sibs. The ability of the SNP panel to uniquely identify individuals on DNA and RNA level was validated in an independent population dataset. The panel is applicable to individuals from European descent, with slightly lower power in non-Europeans. Whereas most of the genes containing the 50 SNPs are expressed in various tissues, our SNP panel needs optimization for other tissues than blood.CONCLUSIONS: This first DNA/RNA SNP panel will be useful to identify sample mix-ups in biomedical research and for assigning DNA and RNA stains in crime scenes to unique individuals.

AB - BACKGROUND: SNP panels that uniquely identify an individual are useful for genetic and forensic research. Previously recommended SNP panels are based on DNA profiles and mostly contain intragenic SNPs. With the increasing interest in RNA expression profiles, we aimed for establishing a SNP panel for both DNA and RNA-based genotyping.RESULTS: To determine a small set of SNPs with maximally discriminative power, genotype calls were obtained from DNA and blood-derived RNA sequencing data belonging to healthy, geographically dispersed, Dutch individuals. SNPs were selected based on different criteria like genotype call rate, minor allele frequency, Hardy-Weinberg equilibrium and linkage disequilibrium. A panel of 50 SNPs was sufficient to identify an individual uniquely: the probability of identity was 6.9 × 10- 20 when assuming no family relations and 1.2 × 10- 10 when accounting for the presence of full sibs. The ability of the SNP panel to uniquely identify individuals on DNA and RNA level was validated in an independent population dataset. The panel is applicable to individuals from European descent, with slightly lower power in non-Europeans. Whereas most of the genes containing the 50 SNPs are expressed in various tissues, our SNP panel needs optimization for other tissues than blood.CONCLUSIONS: This first DNA/RNA SNP panel will be useful to identify sample mix-ups in biomedical research and for assigning DNA and RNA stains in crime scenes to unique individuals.

KW - Biobanking

KW - Forensics

KW - Genetic variation

KW - Journal Article

KW - Mix up samples

KW - Sample tracking

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UR - http://www.scopus.com/inward/citedby.url?scp=85041448036&partnerID=8YFLogxK

U2 - https://doi.org/10.1186/s12864-018-4482-7

DO - https://doi.org/10.1186/s12864-018-4482-7

M3 - Article

C2 - 29370748

SN - 1471-2164

VL - 19

SP - 90

JO - BMC Genomics

JF - BMC Genomics

IS - 1

M1 - 90

ER -

A SNP panel for identification of DNA and RNA specimens

Abstract

Keywords

Cohort Studies

UN SDGs

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