Repeat Citizens in Motor Vehicle Stops

ABSTRACT

This paper explores the possible existence of the repeat phenomenon and their impact on racial disparities in police motor vehicle stops. The repeat phenomenon is the existence of a small proportion of people or places that account for a much larger proportion of events. While this phenomenon has been identified and discussed in other areas of criminal justice and criminology, it has not been extended to motor vehicle stops. The current study examines the existence of repeat citizens in a population of motor vehicle stops (N = 4775) from a Mid-western city during 2001. A small, but significant, concentration of motor vehicle stops were discovered among a few citizens and significant predictors of citizen performance included citizen race, gender, age, residency, time of the stop, and reason for the stop.     

DNA profiling of disaster victim identification in Trenggalek shipwreck case

DNA analysis is one of the primary methods of identification in DVI practices. The external environment of a mass disaster often results in severe fragmentation, decomposition and intermixing of the remains. However, DNA profiling still can be achieved even on cases involving partial, severely decomposed remains. This report shows the DNA profile of shipwreck victims using identifiler plus marker from tissue sample exposed to environmental conditions.     

Multiplex high resolution melt (HRM) messenger RNA profiling assays for body fluid identification

Traditional body fluid identification methods use a variety of technologically diverse techniques that do not permit the identification of all body fluids. Definitive identification of the biological material present can be crucial to a fuller understanding of the circumstances pertaining to a crime. Thus definitive molecular based strategies for the conclusive identification of forensically relevant biological fluids need to be developed. Messenger (mRNA) profiling is an example of such a molecular based approach.Current mRNA body fluid identification assays typically involve either capillary electrophoresis (CE) or quantitative RT-PCR (qRT-PCR) platforms, each with its own limitations. Both platforms require the use of expensive fluorescently labeled primers or probes. CE-based assays require separate amplification and detection steps thus increasing the time required for analysis. For qRT-PCR assays, only 3 or 4 markers can be included in a single reaction since each requires a different fluorescent dye. To simplify mRNA profiling assays and to reduce the time and cost of analysis, we have developed multiplex high resolution melt (HRM) assays that provide an identification of all forensically relevant biological fluids and tissues.     

SNP genotyping of forensic casework samples using the 52 SNPforID markers

The analysis of degraded DNA is one of the biggest challenges in forensic casework. SNPs, which can be amplified using small amplicons, have previously been successfully applied to the profiling of forensic evidence that could not be analyzed using conventional STRs. Here we selected the 52 SNPforID SNP markers, with amplicons that ranged in size from 59 bp to 115 bp, and used them to profile a range of casework samples from Malaysia. DNA degradation is a common problem in Malaysia due to the high temperatures and humidity. To carry out the study we modified the 52 SNPforID markers into four 13-plex SNaPshot assays to enable easier interpretation of profiles on the ABI PRISM^® 310 and 3500.Fifty-one crime samples comprising bloodstains on cloth, swabs, and a mat and 2 swabs of trace DNA from 10 crime scenes in Malaysia were profiled after DNA extraction using a phenol–chloroform method. The samples were also subjected to STR analysis using the Powerplex^® 16 system (Promega), which resulted in only 17 full profiles and 9 partial profiles; using SNPs, 36 full profiles and 5 partial profiles could be generated.     

The Role of the Chemical Weapons Convention in Countering Chemical Terrorism

A series of incidents over the past two decades has indicated that some terrorist groups are interested in acquiring and using improvised chemical devices (ICDs). Although the 1993 Chemical Weapons Convention (CWC) is a disarmament treaty that is legally binding only on sovereign states that join it voluntarily, the Convention fortuitously includes several provisions that can help its members to prevent chemical terrorism or to manage the consequences of an attack. This article examines the articles of the CWC that are relevant to counterterrorism and discusses how their implementation could be improved at the national and international levels. The article also addresses the role that the CWC secretariat, the Organization for the Prohibition of Chemical Weapons (OPCW) in The Hague, currently plays in preventing and responding to incidents of chemical terrorism, and the political factors that constrain its activities in the counterterrorism field.     

Concordance Between the AmpFℓSTR® MiniFiler™ and AmpFℓSTR® Identifiler® PCR Amplification Kits in the Kuwaiti Population

Abstract:  The AmpFℓSTR^® MiniFiler™ polymerase chain reaction amplification kit, developed and supplied by Applied Biosystems, complements the AmpFℓSTR^® Identifiler^® polymerase chain reaction amplification kit (Applied Biosystems, Warrington, U.K.) by improving the success rate when profiling DNA that is degraded or contains inhibitors. Before applying the MiniFiler™ kit to casework, the profiles from 200 unrelated Kuwaitis were compared to Identifiler^® profiles. Concordance was observed for 99.875% (1598 of 1600) of the compared STR loci. The two discordant profiles displayed allelic dropout: one at the D13S317 locus due to nonamplification of allele 10 in the MiniFiler™ profile, and one at the D18S51 locus due to nonamplification of allele 18 in the Identifiler^® profile.     

A report of the 2002–2008 paternity testing workshops of the English speaking working group of the International Society for Forensic Genetics

The English Speaking Working Group (ESWG) of the International Society for Forensic Genetics (ISFG) offers an annual Paternity Testing Workshop open to all members of the group. Blood samples, a questionnaire and a paper challenge are sent to the participants. Here, we present the results of the 2002–2008 Paternity Testing Workshops with the objective to evaluate the uniformity of DNA-profiling and conclusions of the participating laboratories as well as to clarify tendencies in typing strategies and biostatistical evaluations of the laboratories. The numbers of participating laboratories increased from 46 in 2002 to 68 in 2008. The results showed an increasing degree of concordance concerning methods and DNA systems used and a high degree of uniformity in typing results with discrepancies in 0.1 and 0.3 % of all submitted PCR-based results. The paper challenges showed uniformity in the calculation of the weight of evidence for simple cases with straight-forward genetic constellations. However, a high degree of variation existed in complex scenarios with rare genetic constellations such as genetic inconsistencies/possible silent alleles, rare alleles and haplotypes.     

无碳复写字迹的化学消退特征初探

无碳复写消退变造文书案件近年呈增多趋势。采用多种常见有机溶剂对无碳复写字迹进行化学消退实验,并比较消退效果及消退特征,为化学消退无碳复写字迹的检验提供基础性研究数据,具有重要的现实意义。     

Characterization of 26 miniSTR loci for improved analysis of degraded DNA samples

An additional 20 novel mini-short tandem repeat (miniSTR) loci have been developed and characterized beyond the six previously developed by our laboratory for a total of 26 non-CODIS miniSTR markers. These new markers produce short PCR products in the target range of 50-150 base pairs (bp) by moving the primer sequences as close as possible-often directly next to the identified repeat region. These candidate loci were initially screened based on their small amplicon sizes and locations on chromosomes currently unoccupied by the 13 CODIS STR loci or at least 50 Mb away from them on the same chromosome. They were sequenced and evaluated across more than 600 samples, and their population statistics were determined. The heterozygosities of the new loci were compared with those of the 13 CODIS loci and all were found to be comparable. Only five of the new loci had lower values than the CODIS loci; however, all of these were much smaller in size. This data suggests that these 26 miniSTR loci will serve as useful complements to the CODIS loci to aid in the forensic analysis of degraded DNA, as well as missing persons work and parentage testing with limited next-of-kin reference samples.     

大白口蘑子实体的化学成分研究

目的 研究大白口蘑(Tricholoma giganteum Massee)子实体的化学成分。方法 大白口蘑子实体的乙酸乙酯部位经过硅胶、RP-18、Sephadex LH-20等多种材料进行分离纯化, 通过现代波谱技术进行结构鉴定。结果 分离鉴定了12个化合物,它们分别为：亚油酸甲酯（1）、亚油酸（2）、麦角甾-4, 6, 8 (14), 22-四烯-3-酮（3）、麦角甾-5, 7, 22-三烯-3β-醇（4）、过氧麦角甾醇（5）、麦角甾-7, 22-二烯-3β, 5α, 9α-三羟基-6酮（6）、麦角甾-7, 22-二烯-3β, 5α-二羟基-6酮（7）、麦角甾-7, 22-二烯-3β, 5α, 6α, 9α-四醇（8）、麦角甾-7, 22-二烯-3β, 5α, 6β, 9α-四醇（9）、麦角甾-7, 22-二烯-3β, 5α, 6β-三醇（10）、3β-O-glucopyranosyl-5α, 6β-dihydroxy-ergosta-7,22-diene（11）、脑苷脂D（12）。结论 化合物1-3、6-12均为首次从该种真菌中分离得到。