Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise

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Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise. / Sanchez, Juan Jose; Børsting, C; Balogh, K; Berger, B; Bogus, M; Butler, J M; Carracedo, A; Court, D Syndercombe; Dixon, L A; Filipovic, B; Fondevila, M; Gill, P; Harrison, C D; Hohoff, C; Huel, R; Ludes, B; Parson, W; Parsons, T J; Petkovski, E; Phillips, C; Schmitter, H; Schneider, Peter M; Vallone, P M; Morling, N.

I: Forensic Science International: Genetics, Bind 2, Nr. 3, 2008, s. 176-83.

Publikation: Bidrag til tidsskriftTidsskriftartikelForskningfagfællebedømt

Harvard

Sanchez, JJ, Børsting, C, Balogh, K, Berger, B, Bogus, M, Butler, JM, Carracedo, A, Court, DS, Dixon, LA, Filipovic, B, Fondevila, M, Gill, P, Harrison, CD, Hohoff, C, Huel, R, Ludes, B, Parson, W, Parsons, TJ, Petkovski, E, Phillips, C, Schmitter, H, Schneider, PM, Vallone, PM & Morling, N 2008, 'Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise', Forensic Science International: Genetics, bind 2, nr. 3, s. 176-83. https://doi.org/10.1016/j.fsigen.2007.12.002

APA

Sanchez, J. J., Børsting, C., Balogh, K., Berger, B., Bogus, M., Butler, J. M., Carracedo, A., Court, D. S., Dixon, L. A., Filipovic, B., Fondevila, M., Gill, P., Harrison, C. D., Hohoff, C., Huel, R., Ludes, B., Parson, W., Parsons, T. J., Petkovski, E., ... Morling, N. (2008). Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise. Forensic Science International: Genetics, 2(3), 176-83. https://doi.org/10.1016/j.fsigen.2007.12.002

Vancouver

Sanchez JJ, Børsting C, Balogh K, Berger B, Bogus M, Butler JM o.a. Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise. Forensic Science International: Genetics. 2008;2(3):176-83. https://doi.org/10.1016/j.fsigen.2007.12.002

Author

Sanchez, Juan Jose ; Børsting, C ; Balogh, K ; Berger, B ; Bogus, M ; Butler, J M ; Carracedo, A ; Court, D Syndercombe ; Dixon, L A ; Filipovic, B ; Fondevila, M ; Gill, P ; Harrison, C D ; Hohoff, C ; Huel, R ; Ludes, B ; Parson, W ; Parsons, T J ; Petkovski, E ; Phillips, C ; Schmitter, H ; Schneider, Peter M ; Vallone, P M ; Morling, N. / Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise. I: Forensic Science International: Genetics. 2008 ; Bind 2, Nr. 3. s. 176-83.

Bibtex

@article{411d28808b2e11de8bc9000ea68e967b,
title = "Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise",
abstract = "We report the results of an inter-laboratory exercise on typing of autosomal single nucleotide polymorphisms (SNP) for forensic genetic investigations in crime cases. The European DNA Profiling Group (EDNAP), a working group under the International Society for Forensic Genetics (ISFG), organised the exercise. A total of 11 European and one US forensic genetic laboratories tested a subset of a 52 SNP-multiplex PCR kit developed by the SNPforID consortium. The 52 SNP-multiplex kit amplifies 52 DNA fragments with 52 autosomal SNP loci in one multiplex PCR. The 52 SNPs are detected in two separate single base extension (SBE) multiplex reactions with 29 and 23 SNPs, respectively, using SNaPshot kit, capillary electrophoresis and multicolour fluorescence detection. For practical reasons, only the 29 SBE multiplex reaction was carried out by the participating laboratories. A total of 11 bloodstains on FTA cards including a sample of poor quality and a negative control were sent to the laboratories together with the essential reagents for the initial multiplex PCR and the multiplex SBE reaction. The total SNP locus dropout rate was 2.8% and more than 50% of the dropouts were observed with the poor quality sample. The overall rate of discrepant SNP allele assignments was 2.0%. Two laboratories reported 60% of all the discrepancies. Two laboratories reported all 29 SNP alleles in all 10 positive samples correctly. The results of the collaborative exercise were surprisingly good and demonstrate that SNP typing with SBE, capillary electrophoresis and multicolour detection methods can be developed for forensic genetics.",
author = "Sanchez, {Juan Jose} and C B{\o}rsting and K Balogh and B Berger and M Bogus and Butler, {J M} and A Carracedo and Court, {D Syndercombe} and Dixon, {L A} and B Filipovic and M Fondevila and P Gill and Harrison, {C D} and C Hohoff and R Huel and B Ludes and W Parson and Parsons, {T J} and E Petkovski and C Phillips and H Schmitter and Schneider, {Peter M} and Vallone, {P M} and N Morling",
note = "Keywords: Alleles; Blood Stains; DNA Fingerprinting; Electrophoresis, Capillary; Europe; Forensic Genetics; Genotype; Humans; Laboratories; Polymerase Chain Reaction; Polymorphism, Single Nucleotide; Repetitive Sequences, Nucleic Acid; United States",
year = "2008",
doi = "10.1016/j.fsigen.2007.12.002",
language = "English",
volume = "2",
pages = "176--83",
journal = "Forensic Science International: Genetics",
issn = "1872-4973",
publisher = "Elsevier",
number = "3",

}

RIS

TY - JOUR

T1 - Forensic typing of autosomal SNPs with a 29 SNP-multiplex--results of a collaborative EDNAP exercise

AU - Sanchez, Juan Jose

AU - Børsting, C

AU - Balogh, K

AU - Berger, B

AU - Bogus, M

AU - Butler, J M

AU - Carracedo, A

AU - Court, D Syndercombe

AU - Dixon, L A

AU - Filipovic, B

AU - Fondevila, M

AU - Gill, P

AU - Harrison, C D

AU - Hohoff, C

AU - Huel, R

AU - Ludes, B

AU - Parson, W

AU - Parsons, T J

AU - Petkovski, E

AU - Phillips, C

AU - Schmitter, H

AU - Schneider, Peter M

AU - Vallone, P M

AU - Morling, N

N1 - Keywords: Alleles; Blood Stains; DNA Fingerprinting; Electrophoresis, Capillary; Europe; Forensic Genetics; Genotype; Humans; Laboratories; Polymerase Chain Reaction; Polymorphism, Single Nucleotide; Repetitive Sequences, Nucleic Acid; United States

PY - 2008

Y1 - 2008

N2 - We report the results of an inter-laboratory exercise on typing of autosomal single nucleotide polymorphisms (SNP) for forensic genetic investigations in crime cases. The European DNA Profiling Group (EDNAP), a working group under the International Society for Forensic Genetics (ISFG), organised the exercise. A total of 11 European and one US forensic genetic laboratories tested a subset of a 52 SNP-multiplex PCR kit developed by the SNPforID consortium. The 52 SNP-multiplex kit amplifies 52 DNA fragments with 52 autosomal SNP loci in one multiplex PCR. The 52 SNPs are detected in two separate single base extension (SBE) multiplex reactions with 29 and 23 SNPs, respectively, using SNaPshot kit, capillary electrophoresis and multicolour fluorescence detection. For practical reasons, only the 29 SBE multiplex reaction was carried out by the participating laboratories. A total of 11 bloodstains on FTA cards including a sample of poor quality and a negative control were sent to the laboratories together with the essential reagents for the initial multiplex PCR and the multiplex SBE reaction. The total SNP locus dropout rate was 2.8% and more than 50% of the dropouts were observed with the poor quality sample. The overall rate of discrepant SNP allele assignments was 2.0%. Two laboratories reported 60% of all the discrepancies. Two laboratories reported all 29 SNP alleles in all 10 positive samples correctly. The results of the collaborative exercise were surprisingly good and demonstrate that SNP typing with SBE, capillary electrophoresis and multicolour detection methods can be developed for forensic genetics.

AB - We report the results of an inter-laboratory exercise on typing of autosomal single nucleotide polymorphisms (SNP) for forensic genetic investigations in crime cases. The European DNA Profiling Group (EDNAP), a working group under the International Society for Forensic Genetics (ISFG), organised the exercise. A total of 11 European and one US forensic genetic laboratories tested a subset of a 52 SNP-multiplex PCR kit developed by the SNPforID consortium. The 52 SNP-multiplex kit amplifies 52 DNA fragments with 52 autosomal SNP loci in one multiplex PCR. The 52 SNPs are detected in two separate single base extension (SBE) multiplex reactions with 29 and 23 SNPs, respectively, using SNaPshot kit, capillary electrophoresis and multicolour fluorescence detection. For practical reasons, only the 29 SBE multiplex reaction was carried out by the participating laboratories. A total of 11 bloodstains on FTA cards including a sample of poor quality and a negative control were sent to the laboratories together with the essential reagents for the initial multiplex PCR and the multiplex SBE reaction. The total SNP locus dropout rate was 2.8% and more than 50% of the dropouts were observed with the poor quality sample. The overall rate of discrepant SNP allele assignments was 2.0%. Two laboratories reported 60% of all the discrepancies. Two laboratories reported all 29 SNP alleles in all 10 positive samples correctly. The results of the collaborative exercise were surprisingly good and demonstrate that SNP typing with SBE, capillary electrophoresis and multicolour detection methods can be developed for forensic genetics.

U2 - 10.1016/j.fsigen.2007.12.002

DO - 10.1016/j.fsigen.2007.12.002

M3 - Journal article

C2 - 19083818

VL - 2

SP - 176

EP - 183

JO - Forensic Science International: Genetics

JF - Forensic Science International: Genetics

SN - 1872-4973

IS - 3

ER -

ID: 13835702