HLA-DRB1基因分型芯片的法医物证学应用价值研究

目的对HLA-DRB1基因分型芯片在个体识别中的应用价值进行研究。方法根据HLA-DRB1基因座不同等位基因的独特序列设计探针,制成分型芯片。将待测样品DNA用末端标记了CY5的引物进行PCR扩增,产物与芯片进行杂交,根据杂交产生的荧光信号值确定样品在HLA-DRB1位点的基因型。将这一方法应用于561份样本的HLA-DRB1基因分型,根据基因型分布统计分析其法医学应用价值。同时,进行了家系调查和方法灵敏度分析,并应用于部分案例。结果利用微量检材,HLA-DRB1基因芯片可检测DRB1位点等位基因26个,基因型的分布符合Hardy-Weinberg平衡定律,该位点的观察杂合度(Ho)为0.888,期望杂合度(He)为0.902,多态信息含量(PIC)为0.893,平均非父排除率(PE)为0.801。家系调查和案例运用的结果表明,HLA-DRB1位点等位基因由亲代向子代的传递符合孟德尔遗传定律。结论HLA-DRB1为高度多态位点,其基因分型芯片可在亲子鉴定和个体识别中发挥重要作用。     

寡核苷酸芯片技术在HLA-A抗原基因分型中的应用研究

目的建立一种HLA-A位点的基因芯片分型方法,为HLA-A位点的基因分型提供一个较新的思路。方法利用基因芯片技术,根据HLA-A位点不同基因亚型的独特序列设计探针,制成分型芯片;待检测样品经PCR反应标记上荧光之后,与芯片进行杂交,根据杂交产生的荧光信号值分析确定样品HLA-A位点的基因亚型。将这一方法应用于100份标准DNA和200份无关个体的HLA-A位点基因分型并将部分样品进行测序。结果检测结果表明HLA-A基因分型芯片可准确分辨出A位点等位基因20大类,耗时2.5h。结论寡核苷酸芯片技术用于HLA-A基因分型,分辨率高、特异性强、重复性好、操作简便、结果直观,适合于法医学实践和临床应用。     

HLA-DRBl基因分型芯片的法医物证学应用价值研究

目的对HLA-DRBl基因分型芯片在个体识别中的应用价值进行研究。方法根据HLA-DRBl基因座不同等位基因的独特序列设计探针．制成分型芯片。将待测样品DNA用末端标记了CY5的引物进行PCR扩增，产物与芯片进行杂交．根据杂交产生的荧光信号值确定样品在HLA-DRB1位点的基因型。将这一方法应用于561份样本的HLA-DFIBl基因分型，根据基因型分布统计分析其法医学应用价值。同时．进行了家系调查和方法灵敏度分析，并应用于部分案例。结果利用微量检材．HLA-DRB1基因芯片可检测DRB1位点等位基因26个，基因型的分布符合Harely—Weinberg平衡定律．该位点的观察杂合度(Ho)为0．888，期望杂合度(He)为0．902，多态信息含量(PIC)为0．893，平均非父排除率(PE)为0．80l。家系调查和案例运用的结果表明，HLA-DRB1位点等位基因由亲代向子代的传递符合盂德尔遗传定律。结论HLA-DRB1为高度多态位点，其基因分型芯片可在亲子鉴定和个体识别中发挥重要作用。     

运用二重PCR和DNA芯片技术检测ABO基因型

目的以玻片为载体,用寡核苷酸探针杂交技术检测ABO基因型。方法根据ABO基因座外显子6和外显子7的3个SNP点的序列分布特征设计4条寡核苷酸探针,制成分型芯片。将待测样品DNA用末端标记了Cy5的引物进行二重PCR扩增,产物与芯片上的探针进行杂交,根据杂交产生的荧光信号确定样品的ABO基因型。结果利用ABO芯片,可对血斑、毛发等微量检材进行ABO基因型检测。对115名汉族无关个体的调查表明,ABO基因型的分布符合Hardy-Weinberg平衡,等位基因杂合度观察值和期望值分别为0.591、0.616,多态信息含量为0.544,二联体和三联体非父排除率分别为0.188、0.334,个体识别能力为0.777。结论通过DNA芯片检测ABO基因型的技术适用于法医学样本,可满足高通量的检测需求。     

PCR-SBT法检测北京地区人群HLA-DRB1遗传多态性

目的调查北京地区人群HLA-DRB1基因座多态性,并探讨HLA的聚合酶链反应-直接测序分型(PCR-SBT)在法医物证学中的应用价值。方法应用PCR-SBT分型方法对北京地区人群中494名健康无关个体进行HLA-DRB1基因座高分辨分型。结果检出233种HLA-DRB1基因型、102种DRB1等位基因型,基因型的分布符合Hardy-Weinberg平衡定律,该位点的观察杂合度(Ho)为0.9210,期望杂合度(He)为0.9342,多态信息量(PIC)为0.9333,匹配概率(Pm)为0.0104,个体识别率(DP)为0.9896,非父排除率(PPE)为0.7776。结论使用PCR-SBT对HLA进行精确分型在法医学领域具有重要的应用价值。     

HLA DRB基因SSO分型方法的研究

按照第11届国际组织相容性抗原研讨会（IHW）工作会议HLAⅡ类PCR－SSO分型标准和美国国立骨髓供者计划组织（NMDP）对HLADRB基因分型要求,设计合成一对引物,可同时扩增HLA-DRB1＋B3＋B4＋BSDNA片段,长度为256bp,设计合成不同片段大小探针27种,可检出DRB座位上DRB1的39种等位基因,DRB3的3种等位基因,DRB4的1种等位基因和DRB5的3种等位基因。     

31个SNP位点多重PCR扩增和芯片分型技术的建立及其法医学应用

目的对SNP基因分型芯片在个体识别中的应用价值进行研究。方法根据SNP不同等位基因的序列设计探针,制成分型芯片。采用4个复合PCR体系,用末端标记了Cy5的引物进行复合PCR扩增,产物与寡核苷酸探针进行杂交,根据杂交产生的荧光信号值确定样品在各SNP位点的基因型。将这一方法应用于109份样本的分型,根据基因型分布统计分析31个SNP位点的法医学应用价值。同时,进行家系调查和方法灵敏度分析。结果方法的灵敏度为1ng;所检测的31个SNP位点的累积个体识别率为0.9999999999979(偶合率为2.13×10-12),二联体亲子鉴定中累积非父排除率为0.9609,三联体亲子鉴定中累积非父排除率为0.9970。家系调查的结果表明,这些位点等位基因由亲代向子代的传递符合孟德尔遗传定律。结论上述31个SNP位点为中高信息量位点,适用于法医学个体识别,可作为当前STR系统的补充。     

ABO基因分型的等位基因特异性引物消耗法

目的建立一种新的ABO基因型分型的等位基因特异性引物消耗法(CASPA)。方法根据ABO基因碱基序列中的第261、297、803nt3处多态性位点设计6条特异性引物及1条公用引物,采用CASPA法鉴定146名中国汉族无关个体血液斑样品的ABO基因型。结果146名中国汉族无关个体血液斑样品中检出AAb、AB、AO1、BOv、O1Ov、AA、BB、O1O1、BO1等9种基因型,结果明确,其基因频率分布符合Hardy-Weinberg平衡。结论ABO基因型CASPA分型方法为ABO血型的鉴定提供了一个新的检测方法。     

HLA-DQ_α基因的PCR扩增分型技术在88例刑事案件物证检验中应用的回顾

自从PCR（聚合酶链反应）技术问世以来，已有许多基因位点的分型系统开始应用于法医物证的DNA分析[1]，其中应用最为广泛，技术最为成熟的则是HLA－DQ。基因分型系统。此系统应用PCR技术扩增HLA－DQα基因特异片段，结合等位基因特异性寡核着酸（ASO）探针杂交技术检测HLA－DQα位点的四个等位基因，具有特异性好、灵敏度高、结果稳定、准确可靠等优点。本文应用姜先华等人[2]报告的方法，对88例刑事案件的物证进行了HLA－DQα基因的PCR扩增与分型。现报告如下：材料和方法一、检材233份检材来自于全国十九个省市送检的88例刑…     

TaqMan探针技术用于X-SNP位点的分型

目的建立一种基于TaqMan探针技术的快速、准确且经济的实时荧光PCR方法,用于检测X染色体上的单核苷酸多态性(single nucleotide polymorphism,SNP)。方法选择X染色体上的13个SNP位点(X-SNP),针对每个位点分别设计1对PCR引物和TaqMan探针,进行实时荧光PCR扩增,对X-SNP位点进行分型。结果13个位点均符合Hardy-Weinberg平衡;多态信息含量分布为0.3497～0.3750,杂合度为0.4537～0.5021。建立的方法能够用于X-SNP位点的基因分型,检测结果与DNA测序结果完全一致。结论基于TaqMan探针技术的等位基因特异的实时荧光PCR方法灵敏、简单、快速,可实现对X-SNP位点的分型检测;所选择的13个X-SNP位点具有高信息量,在法医遗传学中具有潜在的应用价值。     

A novel method for ABO genotyping using a DNA chip

ABO genotyping is often performed to identify the blood type of decomposed samples, which is difficult to be determined by a serological test. In this study, we developed a simple method for ABO genotyping using a DNA chip. In this method, polymerase chain reaction-amplified and fluorescent-labeled fragments in the ABO gene and primate-specific D17Z1 were hybridized with DNA probes on a chip designed to detect single nucleotide polymorphisms (SNPs) in the ABO gene and part of the D17Z1 sequence. Using blood samples from 42 volunteers and 10 animal species, we investigated whether the chip could be used to detect SNPs in the ABO gene and the D17Z1 sequence. This method was then applied to various forensic samples, and it was confirmed that this method was suitable for the simultaneous analyses of ABO genotyping and species identification. This method fulfills the recent need for the development of rapid and convenient methods for criminal investigations.     

One method of collecting fallen off epithelial cell

In this paper, the comparative analysis of ABO genotyping and serological typing was conducted in 360 unrelated blood samples from northern Chinese Han population using genotyping method and serological typing method, respectively. The results of ABO genotyping were obtained by Goldeneye 16BT STR plus ABO kit. The ABO serological types were determined by the antigen–antibody agglutination test. The ABO types were confirmed by the two methods and no contradiction types were found; two more types were obtained using the ABO genotyping method and the discrimination power was further improved; the information of ABO genotyping and 15 STRs could be obtained at the same time using the Goldeneye 16BT STR plus ABO kit.     

荧光标记的ASP-PCR法对ABO基因分型的研究

目的建立一种方便准确的ABO基因分型检验方法。方法选取ABO基因外显子6和7上的3个位点nt261、nt297和nt803,分别对第6和7外显子进行扩增,并对扩增产物进行测序得出样本的基因型;然后用荧光标记的等位基因特异性引物对已知基因型的样本进行扩增,并用3130遗传分析仪进行电泳分析。结果该方法检出的基因型与测序得出的基因型完全一致。结论等位基因特异性引物法分型结果准确,特异性高,可用于法医学中对犯罪嫌疑人的筛查。     

ABO基因分型与多重STR联合检测在法医学中的应用

目的建立ABO基因型和Goldeneye16A试剂盒联合检测的方法,并评价其在法医学实践中的应用价值。方法将6种ABO基因型(A/A,A/O,B/B,B/O,A/B,O/O)的序列特异性引物(PCR-SSP)检测方法与Goldeneye16A试剂盒相整合进行同步分型。通过对460份男性个体血痕样本、9947A DNA及90份案件样本进行检测,考察方法的一致性、灵敏度及对法庭科学检材的适用性。结果应用本文方法可同时检出6种ABO基因型和15个常染色体STR基因座及性别决定基因座,检测灵敏度为125pg,其中ABO基因检测灵敏度达63pg。460份男性血痕和90份案件检材证实该联合分型方法用于各类检材结果准确、稳定。结论本文ABO基因分型与多重STR联合检测方法,适用于各类含有核细胞的生物检材,在法庭科学DNA鉴定中有较好的应用前景。     

ABO基因分型及其在法医学中的应用

为建立一种ABO血型系统基因分型方法，采用PCR-RFLP技术，成功地将ABO系统区分为AA，AO，AB，OO，BB，BO六种基因型。对240名中国汉族无关个体血样的ABO（基因型频率调查结果表明，6种基因型的频率分布为0．0125～0．3834，符合Hardy－Weinbeng遗传平衡法则（P＞0．1），其DP值为0．8161。家系分析表明，亲代a、b、o基因传递遵守孟德尔遗传规律。对法医学中常见的血痕、混合斑、骨组织及毛发根部等生物样品进行检测，均能准确判定ABO基因型，并可在实际案件鉴定中应用。     

Evaluation of ABO and Lewis genotypes using primer extension preamplification

There are some difficulties with blood typing from ABO variant bloodstains and Lewis negative samples using serologic methods. In these samples, DNA analysis should be employed simultaneously to avoid errors in typing. Primer extension preamplification (PEP) produces copies of template DNA. The minimum quantity to examine nucleotide substitutions of ABO and Lewis genotypes by PCR ranged from 1 to 3 ng DNA. The PCR products with or without PEP treatment showed identical ABO and Lewis genotyping results. Performing both serologic and PCR testing served to crosscheck the ABO and Lewis grouping of such specimens. Errors in ABO and Lewis typing can be avoided as discrepancies are investigated further. The application of the PEP method to limited amounts of DNA samples for ABO and Lewis blood groupings is useful.     

ABO genotyping by mutagenically separated polymerase chain reaction

ABO blood groups were determined by the mutagenically separated polymerase chain reaction (MS-PCR). The products from two sets of PCR reactions using the same program for the nucleotides at positions 261 and 703 from cDNA at the ABO locus were used to distinguish A, B and O alleles. Two forward mutagenic allele-specific primers of different lengths for the ABO polymorphic site were paired with the same reverse primer in each PCR reaction. The 216 bp fragment of the PCR products for the 261th nucleotide was A or B allele-specific and the 195 bp fragment was O allele-specific. The 126 bp fragment of the PCR products for the 703th nucleotide was B allele-specific and the 106 bp fragment was A or O allele-specific. The ABO genotypes were determined by the intersection of the predicted alleles from these two PCR reactions. The PCR products were obtained using 10 ng of DNA in 50 μL of PCR reaction mixture, and electrophoresed in 4% agarose gel. In this study, 265 ABO-phenotype known samples (A: 31, B: 48, AB: 6 and O: 180) in Chinese were used. The results of ABO genotypes were AA: 1, AO: 30, BB: 2, BO: 46, AB: 6 and OO: 180. These results were confirmed by the PCR-RFLP ABO genotyping method. This technique is a simple, rapid, and reliable method for ABO genotyping.     

单管实时PCR快速检验ABO基因型

目的建立快捷特异的ABO基因分型检测方法。方法根据ABO基因结构特点,设计特异性引物和四色双链探针,采用单管实时PCR方法检测ABO基因,结果与传统免疫学方法相对比。结果该方法可检出常见的3个等位基因,区分常见的6种基因型,全部检测过程可在100min内完成。110例中国人的随机个体定型结果与传统免疫学方法一致。结论实时PCR法进行ABO基因分型,简便快捷,灵敏度高,可以有效地为侦查破案服务。     

Multicolor Real-Time PCR Genotyping of ABO System Using Displacing Probes

Abstract:  Rapid and informative ABO genotyping has become increasingly popular in forensic use. We developed a multiplex real-time polymerase chain reaction (PCR) approach to genotype ABO major groups and subgroups. Seven differently fluorophor-labeled displacing probes for O¹(261delG), A(261G), A(796C/803C), B(796A/803C), O² (802G>A), A² (1059delC), and A² (1009A>G) were combined in one or two PCRs to determine either ABO major groups or subgroups. The method correctly detected 13 reference DNA samples. A blind test of 237 samples resulted in complete agreement with their phenotypes, and 110 of these 237 samples as well as with PCR-SSP method. The whole analysis could be finished in less than 100 min at substantially low material cost and the template DNA ranging from 0.16 to 500 ng per reaction could be quantitatively detected. Despite the limited informativeness of ABO genotyping, the developed methods could find application in rapid and inexpensive screening of forensic settings.     

Rapid direct PCR for ABO blood typing

Many different molecular typing methods have been reported to complement routine serological ABO blood typing in forensics. However, these ABO genotyping methods are often time-consuming and call for an initial DNA isolation step that requires the use of expensive kits or reagents. We report here a rapid direct ABO genotyping method that eliminates the need for DNA extraction from fresh blood, hair, and body fluid stains before PCR. Using a fast PCR instrument and an optimized polymerase, the genotyping method-which employs a multiplex allele-specific primer set for the simultaneous detection of three single-nucleotide polymorphism (SNP) sites (nucleotides 261, 526, and 803)-identifies A, B, O01/O02, O03, and cis-AB01 alleles in around 70 min from sample collection to electropherogram. Not only will this ABO genotyping method be efficiently used in forensic practice for rapid screening of samples before full-blown multilocus short tandem repeat profiling, but it will also demonstrate an example of rapid direct genotyping of SNPs that offers the advantages of time- and cost-efficiency, convenience, and reduced contamination during DNA analysis.