3 allele. The only other example of an apparent
true discordance due to an allele dropout occurred in sample 13-011549R-02-1. This was a single source sample and was called as a 16 homozygote in Ferroptosis inhibitor drugs D10S1248 by the Investigator® ESSplex Plus Kit and a 14, 16 heterozygote by both PowerPlex® ESX Fast Systems. Genotypes were obtained from 1392 samples for the PowerPlex® ESI 17 Fast System and 1387 samples for the PowerPlex® ESX 17 Fast System. There was no discordance between the fast cycling and standard cycling chemistries. Thus, the genotype and allele frequencies recently reported for loci present in the PowerPlex® ESI Fast and ESX Fast Systems may be used click here with these systems [28]. Stutter percentages were calculated from the 656 unrelated individuals used in the concordance study. Percentage stutter was determined for products that were
both one repeat unit smaller (N − 4/N − 3) and larger (N + 4/N + 3) in length than the true allele at all autosomal loci and for products that are two bases (N − 2) smaller than the true allele at D1S1656 and SE33. The plus one repeat unit stutter is low for all tetranucleotide repeats, but higher for the trinucleotide repeat D22S1045. The mean, standard deviation of the mean (SD), and maximum stutter observed Cobimetinib manufacturer across all alleles at each locus in both multiplex configurations are shown in Table 1 and Table 2. The mean plus three SD values in each table are used as the recommended stutter filter in the GeneMapper®ID panel file and the GeneMapper®ID-X stutter file. The PowerPlex® ESI Fast and ESX Fast Systems allow for rapid amplification on a variety of thermal cyclers from both purified DNA and direct amplification samples using the
same autosomal primer pairs incorporated in the original standard cycling systems [4], [5] and [6]. By using the same autosomal primer pairs (and only minor changes to the 5′ end of the amelogenin primers), concordance and species specificity was maintained under the faster cycling conditions. Despite a 4-fold reduction in cycling time there is no significant reduction in performance in the presence of PCR inhibitors, overall sensitivity, ability to detect minor contributors in two person mixtures or in stutter when compared to the original standard cycling systems [4], [5], [6] and [28]. The ability to perform direct amplification on a variety of single source reference sample types is conferred by the incorporation of AmpSolution™ Reagent into the reaction with concordant genotypes obtained across diverse direct amplification sample types, both within and between labs.