Identification of a D8S1179 primer binding site mutation and the validation of a primer designed to recover null alleles

被引:63
作者
Leibelt, C
Budowle, B
Collins, P
Daoudi, Y
Moretti, T
Nunn, G
Reeder, D
Roby, R
机构
[1] Appl Biosyst Inc, Foster City, CA 94404 USA
[2] FBI, Lab Div, Washington, DC 20535 USA
[3] Fed Bur Invest Acad, Lab Div, Quantico, VA 22135 USA
关键词
D8S1179; primer binding site mutation; AmpFlSTR (R); multiplex; PCR; STR; validation;
D O I
10.1016/S0379-0738(03)00035-5
中图分类号
DF [法律]; D9 [法律]; R [医药、卫生];
学科分类号
0301 ; 10 ;
摘要
A population study of Chamorros and Filipinos using short tandem repeat (STR) loci amplified with the AmpFlSTR(R) Profiler Plus(TM) PCR amplification kit demonstrated an excess of observed homozygosity at the D8S1179 locus. Use of a different set of D8S1179 primers to type the same samples did not demonstrate an excess of homozygosity and showed discordant genotypes at the D8S1179 locus. A single point mutation, G-to-A transition, 16 nucleotides from the 3' end of the reverse primer, was identified to cause allele dropout when using the AmpFlSTR(R) Profiler Plus(TM) primer set. An additional D8S 1179 reverse primer specific for the variant was constructed resulting in the recovery of the null allele. The primer was included in the newly developed AmpFlSTR(R) Identifiler(TM)PCR amplification kit. No deleterious effects or non-specific peaks were observed in validation experiments evaluating primer concentration, Mg2+ concentration, annealing temperature and population samples. (C) 2003 Elsevier Science Ireland Ltd. All rights reserved.
引用
收藏
页码:220 / 227
页数:8
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