4个Y-STR基因座遗传多态性及分子克隆技术制备分型标准物

目的研究Y染色体4个新发现的STR基因座在成都汉族群体中的遗传多态性,寻找适合于法医学应用的Y-STR基因座并用分子克隆法制备其等位基因分型标准物。方法用PCR扩增和非变性聚丙烯酰胺凝胶电泳技术,对105名成都地区汉族无血缘关系男性个体的4个Y-STR基因座进行分型。并通过分子克隆技术制备DYS643基因座的等位基因分型标准物。结果DYS632、DYS634、DYS642和DYS643四个STR基因座均具有Y染色体特异性,在成都汉族群体中等位基因个数分别为2、4、3和5,共检测出31种单倍型;DYS643基因座的等位基因分型标准物可以用于群体研究。结论DYS643基因座及其分子克隆法制备的等位基因分型标准物具有较高的法医学应用价值。     

DNATyper Y21试剂盒基因座在河南人群中的遗传多态性

本文采用DNA Typer Y21试剂盒对中国河南地区汉族604个健康无关个体进行19个Y-STR基因座和1个常染色体STR基因座遗传多态性进行调查。采用血卡样本进行直扩,用DNA Typer Y21试剂盒进行扩增及检测。结果在20个基因座共检出164个等位基因和601种单倍型,其分布符合Hardy-Weinberg平衡定律(P0.05)。所调查的河南人群20个STR基因座具有较好识别能力,该试剂盒与Yfiler Plus相同基因座遗传学数据比较无显著差异。     

新疆克州维吾尔族15个常染色体STR和10个Y-STR遗传多态性

本文应用ExpressMarker 16+10Y荧光检测试剂盒,对中国新疆克州地区维吾尔族人群239个无关个体15个常染色体STR、10个Y染色体STR基因座遗传多态性进行调查。结果在15个常染色体STR基因座共检出155种等位基因,其分布符合Hardy-Weinberg平衡定律(P>0.05)。累计个体识别率为1-3.3574×10-18,累计非父排除率达0.999 999 244。对所调查的维族人群,本文15个常染色体STR基因座具有较好的识别能力,10个Y染色体STR基因座做了很好的补充,适宜法庭科学DNA建库。     

荧光标记STR复合扩增检验系统的研究

本研究以化学合成的荧光标记引物建立了STR复合扩增体系,体系I包括4个STR基因座和牙釉蛋白基因,体系Ⅱ包括4个STR基因座,体系Ⅲ包括3个STR基因座.制备了体系I各基因座的等位基因标准对照,测定了各等位基因长度.对代表性等位基因进行了序列测定,确定了等位基因重复单位的重复数目及测量长度与等位基因命名的对应关系,对各基因座等位基因进行了标准命名.建立了复合扩增检验系统等位基因自动分析命名的模板.三个复合扩增检验体系的累积随机匹配概率为8.3×10-3,为遗传学分析建立了实用的检验系统.     

新疆克州维吾尔族15个常染色体STR和10个Y-STR遗传多态性

本文应用ExpressMarker 16+10Y荧光检测试剂盒,对中国新疆克州地区维吾尔族人群239个无关个体15个常染色体STR、10个Y染色体STR基因座遗传多态性进行调查。结果在15个常染色体STR基因座共检出155种等位基因,其分布符合Hardy-Weinberg平衡定律(P0.05)。累计个体识别率为1-3.3574×10-18,累计非父排除率达0.999 999 244。对所调查的维族人群,本文15个常染色体STR基因座具有较好的识别能力,10个Y染色体STR基因座做了很好的补充,适宜法庭科学DNA建库。     

15个常染色体和10个Y-STR基因座复合扩增试剂盒的研发

目的建立法医物证学常染色体和Y染色体综合检测的方法。方法选择常用的常染色体STR基因座和Y染色体STR基因座,设计复合扩增引物,形成五色荧光标记复合扩增试剂盒。结果开发出一个五色荧光标记复合扩增试剂盒,可同时对15个常染色体STR基因座、1个性别基因座和10个Y染色体STR基因座进行分型检测。结论 15个常染色体STR加10个Y染色体STR检测试剂盒结合毛细管电泳凝胶进行STR分型,结果准确可靠,在法医学案件检验及数据库建设等方面有良好的应用前景。     

7个Y-STR基因座单倍型及其法医学应用

目的调查7个Y-STR基因座单倍型及其法医学应用。方法利用二组复合扩增体系,(Ⅰ:DYS391、GATA-A4、GATA-A10和GATA-H4;Ⅱ:DYS439、DYS437和DYS434)检测7个Y染色体特异性的STR基因座,并用聚丙烯酰胺凝胶电泳和银染显色技术进行基因分型。结果在广东汉族372名无关男性个体中,二组7个基因座分别检出5、7、6、5和6、4、4个等位基因,共检出254种单倍型,其中201种为唯一的。单倍型基因多样性为0.9960。结论7个Y-STR基因座具有很高的识别能力,对建立Y染色体STR数据库,研究群体遗传学和进行法医学鉴定有重要意义。     

Y染色体STR基因座的研究进展

人类Y染色体STR基因座作为一个特殊的遗传标记以其独特的优势在法医学实践中发挥着重要作用。本文就Y染色体STR基因座的相关理论和研究动态等进行综合评述，为Y染色体STR基因座在法医学中的应用进行有益的探索。     

Y染色体STR基因座的研究进展

人类Y染色体STR基因座作为一个特殊的遗传标记以其独特的优势在法医学实践中发挥着重要作用。本文就Y染色体STR基因座的相关理论和研究动态等进行综合评述,为Y染色体STR基因座在法医学中的应用进行有益的探索。     

湖南汉族人群16个Y—STR基因座遗传多态性

Y染色体短串联重复序列（Y—STR）被广泛应用于父权鉴定、个体识别、人类学和遗传学研究,这些基因座基因频率分布调查是必要的。本文调查了湖南汉族人群174例无关男性个体16个Y—STR基因座的基因频率分布情况,以期为相关实践提供参考数据。     

DNA Commission of the International Society of Forensic Genetics (ISFG): an update of the recommendations on the use of Y-STRs in forensic analysis

The DNA Commission of the International Society of Forensic Genetics (ISFG) regularly publishes guidelines and recommendations concerning the application of DNA polymorphisms to the problems of human identification. A previous recommendation published in 2001 has already addressed Y-chromosome polymorphisms, with particular emphasis on short tandem repeats (STRs). Since then, the use of Y-STRs has become very popular, and a numerous new loci have been introduced. The current recommendations address important aspects to clarify problems regarding the nomenclature, the definition of loci and alleles, population genetics and reporting methods.     

Molecular characterization and Austrian Caucasian population data of the multi-copy Y-chromosomal STR DYS464

DYS464 is a multi-copy STR system with four positions on the Y-chromosome (DYS464a, b, c, and d) which was recently identified and characterized [Forensic Sci. Int. 130 (2002) 97]. The aims of our study were to perform a population study, to estimate the mutation rate and an extensive sequence analysis in order to confirm the nomenclature. Fourteen different alleles were found in an Austrian population sample with an allele length varying from 9 to 19 repeats. All alleles were cloned and sequenced. Alleles 9-19 showed the general repeat structure (CCTT)n...(CCTT)2...(CCTT)3...(CCTT)4...(CCTT)2...(CCTT)2. The nomenclature is based on the number of repeated units of the variable (CCTT)n-stretch only. In 13% of the samples intermediate alleles, namely 14.3A, 14.3B and 15.3 were detected. In these alleles the variable repeat block is interrupted by a CTT motif (14.3A: (CCTT)3CTT(CCTT)11; 14.3B and 15.3: (CCTT)7CTT(CCTT)7/8). A comparison with GenBank entries revealed the existence of a length variant due to a deletion of one cytosine in the 5' flanking region of the first repeat block. We designed an alternative forward primer to circumvent possible ambiguities in the allele designation. A total of 54 different genotypes were identified in 135 men corresponding to a discrimination capacity (DC) of 40% and a gene diversity (GD) of 0.97. These values are much higher than those of other Y-chromosomal short tandem repeats (Y-STRs). DYS464 has the same haplotype diversity (HD) as the combination of the five Y-STR loci with the lowest gene diversities of the Y-STR core set. On the other hand, a combination of the three most diverse loci (DYS464, DYS385 and DYS390) has the same capacity to distinguish between paternal lineages than the complete minimal haplotype (minHT) consisting of eight Y-STR loci. In our population sample the addition of DYS464 to the minHT increases the number of different haplotypes from 110 to 122. The mutation-rate estimate based on the 70 meioses analyzed amounts to 2.86 x 10(-2) (95% confidence interval 3.5 x 10(-3) to 9.95 x 10(-2)). This value is approximately 10 times higher than the average mutation-rate estimate for Y-STRs.     

Two loci ‘exclusion’ of true paternity is due to genetic disorder in a child

We describe a paternity case with three genetic incompatibilities between a three-year-old boy and his putative father.STR analysis of 2 out of 25 markers revealed the absence of paternal alleles and presence of two maternal alleles at D2S441 and D2S1338 loci in the child. The rest 23 STR markers served to confirm paternity. In addition, we analyzed Y-STRs and determined the same haplotype in the child and his putative father.With massive parallel sequencing on HID Ion GeneStudio S5 System using Precision ID GlobalFiler NGS STR Panel v2 (Applied Biosystems) we confirmed the presence of two alleles of maternal origin at D2S441, D2S1338 loci and identified two maternal alleles at additional locus D2S1776 located on chromosome 2 in the child.Finally, we confirm paternity. Three loci ‘exclusion’ was due to maternal uniparental disomy of chromosome 2 in the child.     

荧光复合扩增4个Y染色体STR的单倍型及其法医学应用

目的建立一套Y染色体STR的双色荧光复合扩增系统,调查4个Y-STR基因座单倍型分布情况及其在混合斑物证检验中的法医学应用前景。方法荧光标记引物复合扩增Y-GATA-A10、DYS531、DYS557和DYS448四个Y染色体特异性STR基因座,并用ABⅠ310遗传分析仪对扩增产物进行检测、分型。结果在成都汉族120名无关男性个体中,四个基因座分别检出5、5、8、7个等位基因,共检出78种单倍型,单倍型基因多样性为0.9881。对3例本教研室不能用常规常染色体STR对男性成份作出同一认定的混合斑检材,该系统成功的作出了与嫌疑人血液Y-STR基因型一致的鉴定结论。结论建立的Y-STR荧光标记复合扩增系统具有很高的识别能力,对建立Y染色体STR数据库,研究群体遗传学和进行法医学混合斑物证鉴定有重要意义。     

Evaluation of haplotype discrimination capacity of 35 Y-chromosomal short tandem repeat loci

The haplotype discrimination capacity of the 9 Y-chromosomal short tandem repeat (Y-STR) loci comprising the so called minimal haplotype together with additional 26 recently described single-copy Y-STRs was evaluated within 391 males from Germany, The Netherlands, and Turkey. The aim of this study was to identify the minimum number of Y-STRs needed in addition to the recommended 9 minimal haplotype loci or the 11 SWGDAM loci for individualizing male lineages. Highest gene diversities were shown for DYS385 loci, DYS449, DYS481, DYS570, DYS447, DYS576, DYS389-II, and DYS390 (D=0.7518-0.8746). The five Y-STRs DYS447, DYS449, DYS481, DYS570, and DYS576 comprised the smallest set of loci in addition to the previously recommended standard Y-STRs leading to the individualization of all males from each single population group. Complete resolution of the pooled population was achieved by the additional genotyping of two further loci, DYS446 or DYS505 and DYF406S1 or DYS522.     

Forensic value of 14 novel STRs on the human Y chromosome

We identified and characterized 14 novel short-tandem-repeats (STRs) on the Y chromosome and typed them in two samples, a globally diverse panel of 73 cell lines, and 148 individuals from a European-American population. These Y-STRs include eight tetranucleotide repeats (DYS449, DYS453, DYS454, DYS455, DYS456, DYS458, DYS459, and DYS464), five pentanucleotide repeats (DYS446, DYS447, DYS450, DYS452, and DYS463), and one hexanucleotide repeat (DYS448). Sequence data were obtained to designate a repeat number nomenclature. The gene diversities of an additional 22 Y-STRs, including the most commonly used in forensic databases, were directly compared in the cell line DNAs. Six of the 10 most polymorphic markers include the newly identified Y-STRs. Furthermore, these novel Y-STRs greatly improved the resolution of paternal lineages, above the level obtained with commonly used Y-STRs, in the European-American population.     

Evaluation of rapidly mutating Y-STRs in Pakistani population

Y-chromosomal Short Tandem Repeats have been widely used in forensic investigations, identification of males for criminal justice purpose and population genetics. Commercially available Y-STRs kits allow the identification of male pedigrees and has a limited application in forensic genetics because of its limitation in differentiating closely related male individuals. Recent research with the Rapidly Mutating Y-STRs (RM Y-STRs) have revealed that these loci deliver significantly higher discrimination capacity and haplotype diversity in worldwide populations when compared with the conventional Y-STRs. Although a number of RM Y-STRs have found their way in most updated commercial kits, there are still some loci that are not yet used in such kits. The aim of this study is to develop RM Y-STR haplotypes frequency database for the Pakistani population, in order to appraise the resolution power of these loci. A total of 212 unrelated males from the Pakistani population were typed with 13 RM Y-STRs which comprise DYF399S1, DYF387S1, DYS570, DYS576, DYS518, DYS526a + b, DYS626, DYS627, DYF403S1a + b, DYF404S1, DYS449, DYS547 and DYS612. 211 unique haplotypes were identified, out of which 1 haplotype was shared between two individuals, accounting for 0.9952 discrimination capacity (DC). Haplotype diversity was found to be 0.999925. Gene diversity (GD) values of all the loci were higher than 0.5, where the highest GD values were observed at DYF399S1, DYF403S1a and DYF404S1; with values of 0.99419, 0.98252 and 0.93061 respectively. Results of our study revealed that these 13 RM Y-STRs produced significantly stronger discriminatory power in Pakistani populations.     

Mutations at Y-STR loci: implications for paternity testing and forensic analysis

Knowledge about mutation rates and the mutational process of Y-chromosomal short-tandem-repeat (STR) or microsatellite loci used in paternity testing and forensic analysis is crucial for the correct interpretation of resulting genetic profiles. Therefore, we recently analysed a total of 4999 male germline transmissions from father/son pairs of confirmed paternity (probability > or = 99.9%) at 15 Y-STR loci which are commonly applied to forensics. We identified 14 mutations. Locus specific mutation rate estimates varied between 0 and 8.58 x 10(-3), and the overall average mutation rate estimate was 2.80 x 10(-3) (95% CIL 1.72 x 10(-3)-4.27 x 10(-3)). In two confirmed father/son pairs mutation at two Y-STRs were observed. The probability of two mutations occurring within the same single germline transmission was estimated to be statistically not unexpected. Additional alleles caused by insertion polymorphisms have been found at a number of Y-STRs and a frequency of 0.12% was estimated for DYS19. The observed mutational features for Y-STRs have important consequences for forensic applications such as the definition of criteria for exclusions in paternity testing and the interpretation of genetic profiles in stain analysis. In order to further enrich our knowledge of Y-STR mutations we suggest the establishment of a Y-STR mutation database and ask the forensic community for data contribution.     

Forensic value of 14 novel STRs on the human Y chromosome

We identified and characterized 14 novel short-tandem-repeats (STRs) on the Y chromosome and typed them in two samples, a globally diverse panel of 73 cell lines, and 148 individuals from a European–American population. These Y-STRs include eight tetranucleotide repeats (DYS449, DYS453, DYS454, DYS455, DYS456, DYS458, DYS459, and DYS464), five pentanucleotide repeats (DYS446, DYS447, DYS450, DYS452, and DYS463), and one hexanucleotide repeat (DYS448). Sequence data were obtained to designate a repeat number nomenclature. The gene diversities of an additional 22 Y-STRs, including the most commonly used in forensic databases, were directly compared in the cell line DNAs. Six of the 10 most polymorphic markers include the newly identified Y-STRs. Furthermore, these novel Y-STRs greatly improved the resolution of paternal lineages, above the level obtained with commonly used Y-STRs, in the European–American population.     

PowerPlex^TM16体系OL等位基因序列分析及命名探讨

目的观察中国汉族人群PowerPlexTM16体系STR基因座分型标准物外等位基因(OL等位基因)的序列组成,探讨其类型及命名。方法应用PowerPlexTM16体系和ABI377或3100遗传分析仪,对10071名中国汉族无关个体的血样DNA进行15个STR基因座的分型,筛选出OL等位基因样本;对该样本进行单基因座扩增、聚丙稀酰胺凝胶电泳、银染显色,获取等位基因条带并再次扩增和测序。结果在11个基因座检见OL等位基因,共32个,频率0.05‰￣4.02‰,各基因座OL等位基因数目1￣9个不等。按其组成分为四类:(1)重复单位完整重复,但重复次数在ladder范围外;(2)不完整重复;(3)侧翼序列个别碱基的插入或缺失;(4)较大片断的缺失。结论OL等位基因类型不一,既有重复次数的变化,也有侧翼序列或核心序列的变化,现有命名原则尚不能反映其组成类型。