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Dennis Y. Wang Chien-Wei Chang Nicola J. Oldroyd Lori K. Hennessy 《Forensic Science International: Genetics Supplement Series》2009,2(1):113-114
Forensic databasing laboratories routinely analyze blood or buccal cell samples deposited on FTA® paper. Prior to PCR amplification of the STRs, the FTA® samples must undergo multi-step sample purification protocols to remove the PCR inhibitors present within the sample and from the FTA® paper. The multi-step sample purification protocols are laborious, time-consuming and increase the potential for sample cross-contamination.To eliminate the need for DNA purification, we conducted studies to optimize the PCR buffer and thermal cycling parameters to allow for direct amplification of STRs from blood or buccal samples on FTA® paper. We evaluated the effect of various factors on the DNA profile including: FTA® disc size, blood sample load variation, and buffer formulation. The new STR assay enables the direct amplification of DNA from single source samples on FTA® discs without sample purification. The new STR assay improves the workflow by eliminating tedious steps and minimizing sample handling. Furthermore, the new STR assay reduces cost by eliminating the need for purification reagents and expensive robots. 相似文献
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Julio J. Mulero Nicola J. Oldroyd Michael T. Malicdem Lori K. Hennessy 《Forensic Science International: Genetics Supplement Series》2008,1(1):121-122
Since its introduction in 2002, the AmpF?STR® SEfiler™ kit has provided a highly discriminating DNA profiling option to German forensic laboratories by combining the widely used SGM Plus® Kit loci with the SE-33 locus required for the German DNA Database. Whilst proving successful on database samples, laboratories using the SEfiler™ kit have reported the need for chemistry better able to handle the ever-increasing number of casework samples.The new AmpF?STR® SEfiler Plus™ kit contains the same loci and primer sequences as the SEfiler™ kit but uses improved synthesis and purification processes to minimize the presence of dye-labeled artifacts. Other improvements include modified PCR cycling conditions for enhanced sensitivity and a new buffer formulation that improves performance with inhibited samples when compared to the original SEfiler™ kit.Validation studies demonstrating the effectiveness of the multiplex are presented with emphasis on the models of inhibition and casework samples. 相似文献
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Stine Frisk Fredslund Helle Smidt Mogensen Niels Morling 《Forensic Science International: Genetics Supplement Series》2009,2(1):27-28
Validation of the AmpF?STR® SEfiler Plus™ PCR Amplification kit with 29 and 30 PCR cycles for forensic STR analysis demonstrated that the kit had fewer artefacts than the AmpF?STR® SGM Plus™ kit (28 PCR cycles). The SEfiler Plus kit was more sensitive and devoid of colour artefacts, but showed more stutters, drop-ins, drop-outs and allelic imbalances. 相似文献
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