Comparing two commercial domestic dog (Canis familiaris) STR genotyping kits for forensic identity calculations in a mixed-breed dog population sample.

Almost half of all US households own a dog (Canis familiaris). Though these household pets can attack humans and other animals, they are also frequently victims of cruelty, neglect and theft. In human-oriented investigations, the tendency of domestic dogs to leave behind physical traces (such as hair) can serve as valuable links between crime scenes and suspects/victims. This demonstrated utility of canine biological evidence has created demand for genotyping marker sets for canine forensic genetic testing. Through research and casework, short tandem repeat (STR) panels have been shown to be very efficient for identity and parentage testing in dogs. However, there is an absence of comparative studies between different canine forensic identification kits. The Thermo Fisher Scientific Canine Genotypes ™ Panel 1.1 and 2.1 Kits were originally designed and developed for routine and forensic use respectively, although both kits can be used for either purpose. In this study, we evaluated both STR panels to determine how critical forensic genetic metrics are affected by panel-to-panel variation in marker composition and design. Our results show that although STR panel composition can influence estimates such as inbreeding, combined power of discrimination and combined probability of exclusion, greater average allele number values exhibited across all markers in Panel 2.1 facilitated significantly more precise estimates of random match probability (RMP) and combined probability of identity. Furthermore, we demonstrate that a theta (θ) correction of 0.09 can be used to conservatively adjust RMPs generated from a small reference database of fewer than 50 samples, confirming that Panel 2.1 is a more robust forensic genotyping system than is Panel 1.1. for domestic dogs. We also demonstrate that opportunistic local sampling of fewer than 50 mixed-breed dogs can produce sufficient discriminatory and exclusionary power with either genotyping kit.

Reconstructing full and partial STR profiles from severely burned human remains using comparative ancient and forensic DNA extraction techniques.

Thermal degeneration of the DNA molecule presents a special challenge to medico-legal investigations since low DNA yields, fragmented DNA molecules, and damaged nucleotide bases hinder accurate STR genotyping. As a consequence, fragments of severely burned human remains are often not amenable to standard DNA recovery. However, current ancient DNA (aDNA) extraction methods have proven highly effective at obtaining ultrashort DNA fragments (∼50 bp) from degraded palaeontological and archaeological specimens. In this study, we compare DNA yields and STR results obtained from two established aDNA and forensic DNA extraction protocols by sampling multiple skeletal elements recovered from victims (n = 23) involved in fire-related incidents. DNA yields and STR results suggest an inverse correlation between DNA yield and STR quality and increasing temperature. Despite the rapid thermal destruction of DNA at high temperatures, we generated higher quality full and partial STR profiles using the aDNA extraction protocol across all burn categories than the forensic total bone demineralization extraction method. Our analysis suggests adopting aDNA extraction methods as an alternative to current forensic practices to improve DNA yields from challenging human remains.

ABO blood group phenotype frequency estimation using molecular phenotyping in rhesus and cynomolgus macaques.

A much larger sample (N = 2369) was used to evaluate a previously reported distribution of the A, AB and B blood group phenotypes in rhesus and cynomolgus macaques from six different regional populations. These samples, acquired from 15 different breeding and research facilities in the United States, were analyzed using a real-time quantitative polymerase chain reaction (qPCR) assay that targets single nucleotide polymorphisms (SNPs) responsible for the macaque A, B and AB phenotypes. The frequency distributions of blood group phenotypes of the two species differ significantly from each other and significant regional differentiation within the geographic ranges of each species was also observed. The B blood group phenotype was prevalent in rhesus macaques, especially those from India, while the frequencies of the A, B and AB phenotypes varied significantly among cynomolgus macaques from different geographic regions. The Mauritian cynomolgus macaques, despite having originated in Indonesia, showed significant (P ≪ .01) divergence from the Indonesian animals at the ABO blood group locus. Most Mauritian animals belonged to the B blood group while the Indonesian animals were mostly A. The close similarity in blood group frequency distributions between the Chinese rhesus and Indochinese cynomolgus macaques demonstrates that the introgression between these two species extends beyond the zone of intergradation in Indochina. This study underscores the importance of ABO blood group phenotyping of the domestic supply of macaques and their biospecimens.