Validation of highly polymorphic fluorescent multiplex short tandem repeat systems using two generations of DNA sequencers

被引:0
作者
Frégeau, CJ [1 ]
Bowen, KL [1 ]
Fourney, RM [1 ]
机构
[1] Royal Canadian Mounted Police, Cent Forens Lab, DNA Methods & Data Base, Ottawa, ON K1G 3M8, Canada
关键词
forensic science; short tandem repeat; validation; multiplex; fluorescence; polymerase chain reaction; sequencer;
D O I
暂无
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
Validation studies are a crucial requirement before implementation of new genetic typing systems for clinical diagnostics or forensic identity. Two different fluorescence-based multiplex DNA profiling systems composed of amelogenin, HumD21S11 and HumFGA (referred to as multiplex 1A)? and HumD3S1358, HumD21S11: and HumFGA (multiplex 1B) have been evaluated for use in forensic identification using the Applied Biosystems Model 373A and Prism(TM) 377 DNA Sequencers, respectively. Experiments were aimed at defining the limit of target DNA required for reliable profiling, the level of degradation that would still permit amplification of the short tandem repeat (STR) loci examined, and the robustness of each locus in the multiplexes after samples were exposed to environmental insults. In addition, the specificity of the multiplexes was demonstrated using nonhuman DNAs. Forensically relevant samples such as cigarette butts. chewing gum, fingernails and envelope flaps were processed using both an organic extraction procedure and a QIAamp protocol. DNAs and resultant multiplex STR profiles were compared. The validation of the tripler STR systems was extended to include over 140 nonprobative casework specimens and was followed with a close monitoring of initial casework (over 300 exhibits). Our results document the robustness:of these multiplex STR profiling systems which, when combined with other multiplex systems, could provide a power of discrimination of approximately 0.9999.
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页码:133 / 166
页数:34
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