西安汉人D1S80位点基因频率调查

利用PCR技术、小型聚丙烯酰胶凝胶电泳及银染法，检测D1S80位点的VNTR扩增片段长度多态性（Amp－FLP）。在175名无关的西安地区汉族人群中发现了22个等位基因，片段大小分布于320～750bp之间，频率分布为0．0057～03314，杂合度为82．3％，个人识别率（DP）为0.9588，非父排除率（EPP）为0．6704。对7个家系23名相关个体分析，证实DIS80位点的遗传符合孟德尔方式。已发现的64种基因型分布符合Hardg－Weinberg定律。     

短串联重复位点ACTBP2(SE33)的扩增片段长度多态性研究

应用变性聚丙烯酸胺凝胶电泳（dn－PAGE）结合银染色技术对短串联重复（STR）位点ACTBP2（SE33）的扩增片段长度多态性（Amp－FLPs）进行了研究。在210名无关中国个体中观察到了25个等位基因，等位基因频率分布在0．007～0．093之间。基因型的分布符合Hardy－Weinberg定律，个体识别能力（DP）值为0．99，杂合度（H）为98．7％。七个家系分析的结果表明，该位点的遗传符合孟德尔遗传法则，未观察到变异。对几种常见的法医物证检材的分析表明，该分型系统对DNA降解放为严重的检村适用性强，而且灵敏度高（0．5ng），适合于法医学实际应用。     

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。     

PCR－RFLP技术鉴定ABO基因型的法医学应用研究

目的建立PCR－RFLP、非变性PAG胶垂直电泳和银染技术进行ABO基因分型的方法体系,并对200名广东汉族人群ABO基因型频率进行了调查。方法用Chelex－100和酚、氯仿抽提法处理样本,PCR扩增后用非变性聚丙烯酰胺凝胶垂直电泳和银染技术检测分型。结果ABO位点特异性扩增片段长度为175bp～210bp,6种基因型频率分布为0.0250～0.4300,杂合度H值为0.5162,个体识别力DP值为0.7111。结论该方法可成功运用于血液、血痕、精斑、毛发、骨组织和混合斑等检材的个体识别及亲权鉴定的检验。     

p33.4位点扩增片段长度多态性及其法医学应用的研究

以聚合酶链反应（PCR）、聚丙烯酰胺凝胶垂直电泳和银染法对中国100名无关个体小卫星区域p33．4位点的扩增片段长度多态性（Amp－FLPs）进行了研究，检出了8个等位基因。通过BIOTRAC系统进行数据处理．各等位基因重复单位的数目分别为7、10到15，其中在13～14之间发现一差值不足一个重复单位长度的罕见等位基因。片段长度分布于603～1115bP之间，基因频率分布于0.5～33．5％间，杂合度为64％，DP值为84．5％。对5个家庭25名相关个体进行分析，符合孟德尔遗传定律；对同一个体不同组织的DNA进行P33.4位点的分型研究表明，该技术适宜于法医物证检验。此外，本研究以Chelex处理不同检材制备DNA模板用于扩增，率先建立了比常规方法更快、更简便、更为实用的检验方法。     

内蒙古中西部地区汉族、蒙古族ApoB基因遗传多态性

目的研究内蒙古中西部地区汉族、蒙古族ApoB基因遗传多态性。方法选取内蒙古中西部地区汉族、蒙古族无关个体,采用聚合酶链反应一限制性片段长度多态性技术,判断样本中是否含有ApoB基因中的稀有等位基因：XbaI（x＋）和＆DRI（E-）,并计算其基因型频率、等位基因频率及相关的群体遗传学参数。结果内蒙古汉族群体中稀有等位基因XbaI（x＋）和＆0RI（E-）频率分别为2％和4．6％,而在蒙古族群体中没有检测出此两种稀有等位基因。结论ApoB基因XbaI和＆0RI位点的等位基因频率分布在不同种族中差异较大,具有种族鉴定的应用可能。     

用PCR-SSP法分析中国辽宁汉族HLA-DRBI基因多态性

应用PCR－SSP方法对辽宁地区159名无关个体进行HLA－DRB1位点基因分型，检出8组等位基因（扩增片段大小为100bp），基因频率范围在0．02201～0．23899。36种可能基因型中检出33种。经x2检验符合Hardy－Weinberg平衡定律。本地区汉族群体的期望杂合度为85％，观察杂合度为83％。个人鉴别机率（DP）为0．94非父排除率（EPP）为66％。本法具有简单、快速、结果可靠的特点，不仅适用于法医学亲子鉴定和个人识别、移植配型，亦可用于相关疾病及人类遗传学研究。     

PCR-RFLP技术鉴定ABO基因型的法医学应用研究

目的 建立 PCR－ RFLP、非变性 PAG胶垂直电泳和银染技术进行 ABO基因分型的方法体系,并对 200名广东汉族人群 ABO基因型频率进行了调查。方法 用 Chelex－ 100和酚、氯仿抽提法处理样本, PCR扩增后用非变性聚丙烯酰胺凝胶垂直电泳和银染技术检测分型。结果 ABO位点特异性扩增片段长度为 175bp～ 210bp, 6种基因型频率分布为 0.025 0～ 0.430 0,杂合度 H值为 0.516 2,个体识别力 DP值为 0.711 1。结论 该方法可成功运用于血液、血痕、精斑、毛发、骨组织和混合斑等检材的个体识别及亲权鉴定的检验。     

用PCR-SSCP法进行亲子鉴定及个体识别

HLA－DR位点是一个具有高度遗传多态性的基因位点。到目前为止已发现其具有68个等位基因，此外还有7个假性基因。从国内外DRll基因频率调查来看，各基因频率的分布比较均衡。因此通过检测HLA－DRB基因位点进行亲子鉴定能获得较高的父权排除率，进行个体识别时能达到较高的个体识别率。以往用RFI，P（限制性片段长度多态性）或SSO（序列特异性寡核着酸）方法进行HI，A－DRB基因的定型所需时间较多，而且不能同时对其假性基因进行分析。根据单链构象多态性（polymerasechainreaction－singlestrandconformatlonPoly－mornhism，PC…     

中国北方汉族人群HLA-DQα基因型及其等位基因频率的分布

应用PCR和等位基因特异性寡该苷酸（ASO）探针杂交技术对中国北方汉族人群的HLA－DQα基因进行分型。在246例无关个体中观察到4种等位基因组成的10种基因型。等位基因频率分布在10．0～31．9％之间。基因型的分布符合Hardy－Weinberg定律。DP值为0．8669。对6个家系49个个体的调查表明，HLA－DQα基因按孟德尔方式遗传。不同人群HLA－DQα的DP值比较，中国人群高于其它人群。     

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.     

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。     

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.     

A New Method for Human ABO Genotyping Using a Universal Reporter Primer System

Abstract: We developed a new method for forensic ABO genotyping based on a universal reporter primer (URP) system. This allows for the simultaneous detection of six single nucleotide polymorphism (SNP) sites in the ABO gene (nucleotide positions 261, 297, 526, 703, 796, and 803). This URP system provides obvious peaks, ranging from 82 to 151 bp in length. ABO genotypes were classified and successfully genotyped by our method, including minor alleles that may cause a discrepancy between the genetic data and serological phenotypes. Full profiles were identified using as little as 0.1 ng (0.05 ng/reaction) of standard K562 and 9947A DNA. Moreover, the success rate of genotyping from a URP system was much higher than that from a conventional primer extension method in degraded DNA. This method enables simple and rapid detection of multiple SNP sites on human ABO genes and is highly specific and sensitive when using limited and degraded DNA.     

Alleles responsible for ABO phenotype-genotype discrepancy and alleles in individuals with a weak expression of A or B antigens

ABO types obtained from evidentiary samples have been used effectively to obtain the initial information leading to the apprehension of culprits in Japanese criminal investigations. A simple ABO genotyping method using multiplex sequence-specific PCR and capillary electrophoresis was developed as a supplement to serological ABO typing. Limitations in predicting a phenotype based on genotype were evaluated using 1134 randomly selected Japanese peripheral blood samples. A concordance rate of 99.82% (1132/1134 samples) was found between genotypes and phenotypes defined as Groups A, B, AB, and O. Sequencing analysis revealed that one discrepant sample contained an O allele having a previously unreported point mutation at the primer binding site in exon 6, and another discrepant sample contained an O allele lacking the guanine deletion at nt 261 (the O301 allele). Therefore, the existence of such alleles must be given some consideration when predicting phenotype based on genotype.     

ABO genotyping by polymerase chain reaction.

ABO blood group system's genotyping by polymerase chain reaction in genomic DNA level is developed. The positions of nucleotide 258 and 700 of cDNA from A transferase were used to distinguish A, B, and O alleles by restriction enzyme digestion. To identify the 258th nucleotide, a 199- or 200-bp DNA fragment was amplified by PCR and digested with Kpn I. For the 700th nucleotide, a 128-bp PCR amplified fragment was designed and digested with Alu I. By examining the DNA fragment digested patterns, ABO genotypes were easily determined. Results obtained using this method on 20 ABO-known peripheral blood samples showed that this new technique could provide accurate ABO genotype. Biologic forensic samples, such as, blood stains, saliva stains, semen stains, hair, bone tissue, and semen contaminated with vaginal secretion were also successfully typed. This rapid, sensitive and reliable method should be applicable not only in forensic identification but also in medical examination.     

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 genotyping by duplex amplification and oligonucleotide arrays assay

Objective

Research on the application feasibility of ABO genotyping for forensic identification by oligonucleotide arrays assay.

Methods

Oligonucleotide microarrays which detect three different SNPs in exon 6 and exon 7 for ABO genotyping were used. After hybridization wash, the arrays were scanned and fluorescence intensities were analyzed using microarray population studies on ABO was carried out in a sample of 115 unrelated Chinese Han individuals oligonucleotide arrays for genotype detection. The method was also applied to cases.

Results

Technique could identify six genotypes of ABO system and the results of GeneChip analyses confirmed by PCR–RFLP. According to the results of population studies, no significant deviations Hardy–Weinberg equilibrium could be found. The observed heterozygosity (H-obs) was 0.591. Expected heterozygosity (H-exp) was 0.616. The polymorphic information content (PIC) was the average exclusion probability in paternity testing for duos (PE (1)) was 0.188. The average exclusion probability in paternity testing for trios (PE(2)) was 0.344. The discrimination power 0.777.

Conclusion

The data and case application demonstrated that ABO typing by oligonucleotide probe arrays was a useful technique for paternity testing and individual identification.     

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.