山东汉族人群19个STR基因座的遗传多态性

目的调查山东汉族人群19个STR基因座的群体遗传学资料,为亲权鉴定提供遗传学数据。方法采用GoldeneyeTM20A试剂盒对山东汉族人群中205例无关个体进行基因分型,得到19个STR基因座的等位基因频率及群体遗传学参数。对Identifile一、SinoFilerTM、PowerPlex16和GoldeneyeTM20A4个试剂盒进行比较,并对l例特殊的亲子鉴定案件进行分析。结果获得山东汉族人群19个STR基因座的群体遗传学参数。累积个体识别率（CDP）及累积非父排除率（CPE）从高到低分别为GoldeneyeTM20A、SinoFilerTM、PowerPlex16、IdentifilerTM试剂盒。对实际案件进行分析．作为二联体,IdentifilerTM试剂盒无被排除基因座,而SinoFilerTM、PowerPlex16和GoldeneyeTM20A试剂盒均不能排除父子关系。结论与IdentifilerTM、SinoFilerYn和PowerPlex163种试剂盒进行比较．GoldeneyeTM20A试剂盒效能更高．但不能完全满足二联体鉴定的要求。     

Genetic Polymorphisms of 15 STR Loci in Gansu Hui Population

The short tandem repeat （STR） markers are widely used in human identification and paternity testing in the field of forensic geneticsm. Recent re- searches on polymorphic STRs have led to their applications to population genetics, forensic DNA database, human individual identification, paternity testing, genetic mapping, disease linkage analysis, archaeology and potential inference of the ethnic o- rigin of an individual.     

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.     

Application of direct PCR in forensic casework

Direct PCR is fast becoming a popular method in forensic science due to the advantages of saving time and money in the lab while increasing the probability of obtaining substantial results has a positive rippling effect. A laboratory is able to reduce the time spent on processing trace DNA samples, which can lead to investigators receiving important information in a timely manner that may not have been possible using standard methods. This study highlights the benefits of direct PCR in forensic casework by analysing trace and touch DNA on a range of substrates and exploring the loss of initial DNA due to extraction.     

Analysis of 15 autosomal STR loci in the population of the State of Acre,Brazilian Amazonia

Acre was the last state of Brazil to be inhabited by non-indigenous individuals. The aim of this study was to calculate the allele frequencies of 15 STR loci in 503 unrelated individuals living in Acre, as well as to estimate statistical parameters of forensic interest. The Hardy–Weinberg equilibrium test performed in the overall sample, as well as population comparisons between sub-samples from the five regions in Acre did not reveal the presence of population substructure. This is the first report of STR data in this population and the results showed that a single database is suitable for all the regions analyzed.     

Developmental validation of 15 X chromosomal short tandem repeat markers

The use of X chromosomal short tandem repeat (STR) markers has been greatly increasing in the forensic setting. Using guidelines set forth previously for the validation of autosomal and Y STRs, aspects of the feasibility of routine X chromosomal STR use were evaluated. Two mini-X chromosomal STR multiplexes capable of amplifying 15 total markers were developed and utilized to determine allele nomenclature, allele/genotype frequencies, mutation rates, and linkage between markers. Additionally, a concordance study between these multiplexes and a commercially available kit was performed. Here, the authors present an overview of this extensive developmental validation study.     

Ultrafast Amplification of DNA on Plastic Microdevices for Forensic Short Tandem Repeat Analysis

The majority of microfluidic devices used as a platform for low‐cost, rapid DNA analysis are glass devices; however, microchip fabrication in glass is costly and laborious, enhancing the interest in polymeric substrates, such as poly (methyl methacrylate) (PMMA), as an inexpensive alternative. Here, we report amplification in PMMA polymerase chain reaction (PCR) microchips providing full short tandem repeat profiles (16 of 16 loci) in 30–40 min, with peak height ratios and stutter percentages that meet literature threshold requirements. In addition, partial profiles (15 of 16 loci) were generated using an ultrafast PCR method in 17.1 min, representing a ~10‐fold reduction in reaction time as compared to current amplification methods. Finally, a multichamber device was demonstrated to simultaneously amplify one positive, one negative, and five individual samples in 39 min. Although there were instances of loci dropout, this device represents a first step toward a microfluidic system capable of amplifying more than one sample simultaneously.     

High‐Throughput STR Analysis for DNA Database Using Direct PCR,

Since the Korean criminal DNA database was launched in 2010, we have focused on establishing an automated DNA database profiling system that analyzes short tandem repeat loci in a high‐throughput and cost‐effective manner. We established a DNA database profiling system without DNA purification using a direct PCR buffer system. The quality of direct PCR procedures was compared with that of conventional PCR system under their respective optimized conditions. The results revealed not only perfect concordance but also an excellent PCR success rate, good electropherogram quality, and an optimal intra/inter‐loci peak height ratio. In particular, the proportion of DNA extraction required due to direct PCR failure could be minimized to <3%. In conclusion, the newly developed direct PCR system can be adopted for automated DNA database profiling systems to replace or supplement conventional PCR system in a time‐ and cost‐saving manner.     

中国成都地区汉族群体5个STR基因座的遗传多态性

采用PCR扩增,聚丙烯酰胺凝胶电泳分析技术,调查中国成都汉族群体DIS1656、D851179、D9S302、D185535及D195253等5个STR基因座的等位基因频率分布。D1S1656检出11个等位基因,35种基因型;DSS1179检出9个等位基因,32种基因型;D95302检出12个等位基因,50种基因型;D185535检出7个等位基因,20种基因型;D195253检出8个等位基因,28种基因型。5个STR基因座基因型频率分布符合Hardy-weinberg平衡（P＞0．05）。个人识别机率（DP）为0．92～0．98。分析了二代3口之家的遗传模式,证明5个STR基因座均符合孟德尔遗传规律。5个STR基因座PCR扩增采用同一条件,方法简单、快速、灵敏、重复性好,可用于法科学亲子鉴定和个人识别。     

青岛地区汉族人群13个STR基因座的频率分布及法医学应用

目的　调查青岛地区汉族人群无关个体的 13个STR基因座 (D3S135 8、VWA、FGA、D8S1179、D2 1S11、D18S5 1、D5S818、D13S317、D7S82 0、D16S5 39、TH0 1、TPOX、CSFIPO)的基因频率分布 ,研究其遗传多态性及其在法医学个体识别及亲子鉴定中的应用价值。　方法　用美国ABI - 310型遗传分析仪对ProfilerPlus和Cofiler两个系统的 13个STR基因座的复合扩增产物进行毛细管电泳及四色荧光自动分析检测 ,基因分型软件为GeneScanv3.1和Genotyperv2 .5 .2。　 结果　获得 13个STR基因座在青岛地区汉族人群的基因频率分布数据 ,13个STR基因座的PIC >0 .5 ,DP >0 .71,CCE =0 .999999,TDP值接近 1,TPm =1.2× 10 -14 ,家系调查符合孟德尔遗传规律。　结论　ProfilerPlus和Cofiler两个系统的 13个STR基因座在法医学个体识别及亲子鉴定中具有较高的应用价值。