浙江汉族人群HLA-DPA1和-DPB1基因多态性分析

目的 检测浙江地区汉族人群HLA-DPA1和HLA-DPB1等位基因及单倍型频率.方法 应用PCR-直接测序分型法对100名健康、无血缘关系的浙江汉族人外周血标本进行HLA-DPA1和HLADPB1等位基因分析.结果 在100份标本中检出8个HLA-DPA1等位基因和19个HLA-DPB1等位基因.HLA-DPA1等位基因频率较高的依次为DPA1*020202(47.0%)、DPA1*010301(38.5%)和DPA1*020101(10.5%).HLA-DPB1等位基因中,频率较高的依次为DPB1*0501(39.5%)、DPB1*020102(13.5%)和DPB1*040101(13.0%).连锁分析发现共有44个HLA-DPA1-DPB1单倍型,单倍型频率最高为DPA1*020202-DPB1*0501(29.5%).结论 浙江地区汉族人群HLA-DPA1和DPB1基因座等位基因具有丰富的多态性,2个基因座呈现连锁不平衡.     

浙江汉族人群HLA-DPA1和-DPB1基因多态性分析

目的 检测浙江地区汉族人群HLA-DPA1和HLA-DPB1等位基因及单倍型频率.方法 应用PCR-直接测序分型法对100名健康、无血缘关系的浙江汉族人外周血标本进行HLA-DPA1和HLADPB1等位基因分析.结果 在100份标本中检出8个HLA-DPA1等位基因和19个HLA-DPB1等位基因.HLA-DPA1等位基因频率较高的依次为DPA1*020202(47.0%)、DPA1*010301(38.5%)和DPA1*020101(10.5%).HLA-DPB1等位基因中,频率较高的依次为DPB1*0501(39.5%)、DPB1*020102(13.5%)和DPB1*040101(13.0%).连锁分析发现共有44个HLA-DPA1-DPB1单倍型,单倍型频率最高为DPA1*020202-DPB1*0501(29.5%).结论 浙江地区汉族人群HLA-DPA1和DPB1基因座等位基因具有丰富的多态性,2个基因座呈现连锁不平衡.     

浙江汉族人群HLA-DPA1和-DPB1基因多态性分析

目的 检测浙江地区汉族人群HLA-DPA1和HLA-DPB1等位基因及单倍型频率.方法 应用PCR-直接测序分型法对100名健康、无血缘关系的浙江汉族人外周血标本进行HLA-DPA1和HLADPB1等位基因分析.结果 在100份标本中检出8个HLA-DPA1等位基因和19个HLA-DPB1等位基因.HLA-DPA1等位基因频率较高的依次为DPA1*020202(47.0%)、DPA1*010301(38.5%)和DPA1*020101(10.5%).HLA-DPB1等位基因中,频率较高的依次为DPB1*0501(39.5%)、DPB1*020102(13.5%)和DPB1*040101(13.0%).连锁分析发现共有44个HLA-DPA1-DPB1单倍型,单倍型频率最高为DPA1*020202-DPB1*0501(29.5%).结论 浙江地区汉族人群HLA-DPA1和DPB1基因座等位基因具有丰富的多态性,2个基因座呈现连锁不平衡.     

山西汉族人群HLA-A、-B、-DRB1基因多态性研究

目的 调查山西汉族人群HLA-A、-B、DRB1基因多态性，获得完整准确的遗传学数据。方法 应用聚合酶链反应，序列特异性引物方法对7440名健康、无血缘关系的山西汉族个体进行HLA—A、-B、-DRB1基因型检测，并与不同人群等位基因进行比较。结果 检出A等位基因18个，B等位基因40个，DRB1等位基因13个，其中A＊02、A＊24、A＊11、A＊01、A＊03、B＊13、B＊51、B＊15、B＊40、B＊35、DRB1＊15、DR＊09、DR＊1：2、DR＊04、DR＊07等位基因频率分布较高。结论 山西汉族人群HLA—A，-B，-DRB1基因具有中国北方汉族人群共有的遗传特征，但也有其自身的分布特点。     

北京地区人群HLA-A、B、DRB1的聚合酶链反应-直接测序分型研究

目的调查北京人群人类白细胞抗原（human leukocyte antigen，HLA）-A、B、DRB1的基因多态性，获得完整准确的遗传学数据。方法应用聚合酶链反应-直接测序分型（polymerase chain reaction sequence-based typing，PCR-SBT）法对北京地区人群中618名健康无关个体进行HLA-A、B、DRB1基因座高分辨分型。结果检出HLA-A、B、DRB1的基因型数和等位基因数分别为199和84、366和143、286和122，这3个基因座分布均符合Hardy-Weinberg平衡定律（P〉0．05）。结论从基因水平分析了北京地区HLA-A、B、DRB1基因座的群体分布特征，提供了一套比较完整准确的HLA-A、B、DRB1等位基因频率、基因型频率，为器官移植的供体选择、法医学个体认定、HLA与疾病相关性及人类学等研究提供了重要的参考数据。     

福建汉族人群卸LA-DRB1等位基因多态性研究

目的调查福建汉族人群HLA-DRB1等位基因的多态性。方法应用寡核苷酸基因芯片分型技术对福建地区620名汉族人群进行HLA-DRB1位点的基因分型。结果在HLA-DRB1位点共检出了14种等位基因，基因频率较高的依次为DRB1＊09、12、15、04、08。结论福建汉族HLA-DRB1等位基因多态性与南方汉族人群相近，但也有其独特的特点。     

福建汉族人群HLA-DRB1等位基因多态性研究

目的调查福建汉族人群HLA-DRB1等位基因的多态性。方法应用寡核苷酸基因芯片分型技术对福建地区620名汉族人群进行HLA-DRB1位点的基因分型。结果在HLA-DRB1位点共检出了14种等位基因,基因频率较高的依次为DRB1*09、12、15、04、08。结论福建汉族HLA-DRB1等位基因多态性与南方汉族人群相近,但也有其独特的特点。     

昆明彝族人群HLA-DRB1、DQB1基因多态性

目的　调查昆明彝族 HL A- DRB1、DQB1基因的多态性。方法　应用聚合酶链反应 -序列特异性引物基因分型技术 ,对昆明地区 70名彝族健康儿童进行了 HL A- DRB1、DQB1位点的基因分型。结果在 HL A- DRB1位点共检出了 12种等位基因 ,其中等位基因频率大于 10 %的依次为 HL A- DRB1* 12 (33.5 7% )、DRB1* 0 90 1(11.4 3% )、DRB1* 0 4 (11.4 3% ) ,等位基因频率大于 5 %而小于 10 %的依次为 DRB1* 0 1(8.5 7% )、DRB1* 11(7.86 % )、DRB1* 14 (7.14 % )、DRB1* 15 (7.14 % )、DRB1* 0 8(5 % ) ,等位基因频率小于 5 %依次为 HL A- DRB1* 0 3(2 .86 % )、DRB1* 13(2 .14 % )、DRB1* 0 7(1.4 3% )、DRB1* 16 (1.4 3% )。在 HL A- DQB1位点共检出了 7种等位基因 ,其中等位基因频率大于 10 %的依次为 HL A- DQB1*0 30 1(45 % )、DQB1* 0 5 (2 2 .14 % )、DQB1* 0 30 3(12 .14 % ) ,等位基因频率大于 5 %而小于 10 %的依次为DQB1* 0 4 (6 .4 3% )、DQB1* 0 6 (6 .4 3% ) ,等位基因频率小于 5 %的依次为 DQB1* 0 2 0 1(4.2 9% )、DQB1* 0 30 2 (3.5 7% )。结论　昆明彝族 HL A基因多态性分布不同于北方汉族人群 ,也不同于南方汉族人群 ,有其独特性。     

内蒙古地区鄂温克族人群HLA-DRB1基因多态性

目的对内蒙古鄂温克族人群人类白细胞抗原（human leukocyte antigen，HLA）Ⅱ类基因DRB1位点进行基因型检测。方法采用DNA序列分析的分型技术（sequencing based typing，SBT），对84名鄂温克族个体进行分析。结果DRB1等位基因中，共检出25种等位基因，内蒙古鄂温克族以DRB1＊03011（14．88％）的频率最高，其次为DRB1＊09012（13．69％）、＊07011（8．92％）、＊04011（9．52％）、12011（8．33％）。结论鄂温克族人群中HLA—DRB1分布特征有其独特性，为本民族的人类学及疾病相关性研究提供了重要的参考依据。     

辽宁汉族人群HLA-DRB1基因多态性分布

目的调查HLA-DRB1基因位点遗传多态性在辽宁汉族人群中的分布。方法应用聚合酶链反应．序列特异性引物方法和反向聚合酶链反应．序列特异性寡核苷酸探针杂交的方法对13265名辽宁汉族人进行中低分辨率HLA-DRB1基因分型。结果共检出HLA-DRB1位点的13种等位基因，其中以HLA-DRB1＊15频率最高（17．49％），其次为HLA-DRB1＊09、＊12和HLA-DRB1＊07，基因频率分别为13．40％、11．87％和11．8l％。HLA-DRB1＊03（18）和HLA-DRB1＊14（8）等位基因未检出。对观察值和期望值进行X^2检验，符合Hardy-Weinberg平衡（X^2=73．34，af=78，P〉0．5）。该人群与南北方汉族人群、日本人、白人和黑人分别进行X^2值检验差异有统计学意义，X^2值分别为112．053、8．514、692．141、70．558和121．755。结论辽宁汉族人群HLA-DRB1基因分布有自身特点。     

Association of HLA-DQ with idiopathic dilated cardiomyopathy in a northern Chinese Han population

Autoimmune mechanisms are likely involved in the pathogenesis of idiopathic dilated cardiomyopathy (IDC)and components of MHC may serve as markers for the propensity to develop immune-mediated myocardialdamage.This study was conducted to investigate the possible association between HLA-DQA1,-DQB1 allelesand IDC in Han population from northern China by using PCR-based sequence-specific primer (PCR-SSP)technique for HLA genotyping.Among 68 unrelated IDC patients,4 probands of IDC pedigrees and 100healthy controls,we found that the alleles of HLA-DQA1*0501 and HLA-DQB1*0303 conferred susceptibilityto IDC while HLA-DQA1*0201 and HLA-DQB1*0502,*0504 alleles were in negative association with IDC.Theserine at position 57 (SER~(57)) in the exon of HLA-DQB1*0502 and *0504 was confirmed in our experiment as amarker for resistance to IDC.The results suggest that HLA-DQ polymorphism may be involved in thepathogenesis of IDC.Cellular & Molecular Immunology.2004;1 (4):311-314.     

中国汉族人群DC-SIGN和DC-SIGNR基因遗传多态性

目的了解中国汉族人群DC-SIGN和DC-SIGNR基因颈区重复序列的遗传多态性分布，获得相应位点的汉族人群的遗传学数据。方法应用PCR技术、琼脂糖凝胶电泳结合测序对DC-SIGN和DC-SIGNR基因的颈区重复序列分型，计算DC-SIGNR的多态信息含量。结果DC-SIGN多态性低，颈区绝大多数为等位基因7重复，该等位基因频率为0．9808，但亦检出少量的等位基因4、5、6、8等变异，而美国白人只含有等位基因6、8变异；DC-SIGNR存在高度多态性，多态信息含量为0．5312，存在4、5、6．7、8、9等位基因，检出16种基因型。6／5、7／4、7／5、7／6、7／7、9／5、9．／7、9／9基因型和5、6、7、9等位基因频率在中国汉族人群和美国白人中的分布构成差异有统计学意义（P〈0．01），与美国白人比较，中国汉族人群似乎存在更多的插入突变。结论中国汉人的DC-SIGN和DC-SIGNR基因型分布和基因频率与美国白人相比其差异有统计学意义，并有其独特的群体遗传学特征。     

青海土族、撒拉族HLA-DQA1和-DQB1基因多态性探讨

目的 :检测青海土族和撒拉族健康个体HLA DQA1和 DQB1等位基因频率 ,了解和分析这两个民族的HLA DQA1和 DQB1基因多态性。方法 :用PCR SSO方法检测 132名土族和 80名撒拉族健康个体的HLA DQA1和 DQB1的基因多态性 ,并将所得结果与国内其他民族的同类资料进行比较。结果 :土族和撒拉族在HLA DQA1和 DQB1高频率等位基因分布上有共同点 ,也有一定的独特性。这两种民族HLA DQA1 0 10 2和 0 5 0 1以及DQB1 0 2 0 1、 0 30 1、 0 4 0 2和 0 6 0 2基因分布频率上具有显著性差异。结论 :土族和撒拉族与北方诸民族的等位基因频率接近 ,而与其他南方诸民族的差异相对较大。     

HLA-DQA1, -DQB1 Polymorphism and Genetic Susceptibility to Idiopathic Dilated Cardiomyopathy in Hans of Northern China

Autoimmune mechanisms are likely to participate in the pathogenesis of at least a subgroup of idiopathic dilated cardiomyopathy (IDC), and components of the major histocompatibility complex (MHC) may serve as markers for the propensity to develop immune‐mediated myocardial damage. Human leukocyte antigen (HLA) class II genes, especially HLA‐DQ genes, which are highly polymorphic, play an important role in the activation of immune responses and thus control the predisposition to, or protection from, IDC. This study was conducted to investigate the association of HLA‐DQA1, ‐DQB1 allele polymorphisms with an autoantibody against the myocardial mitochondria ADP/ATP carrier, and to explore susceptibility to idiopathic dilated cardiomyopathy (IDC) among the Han ethnic group in northern China and the immunological mechanisms and hereditary susceptibility to IDC. Polymerase chain reaction sequence‐specific primer (PCR‐SSP) techniques were used to analyze polymorphisms of the second exon of HLA‐DQA1 and ‐DQB1 alleles among 68 unrelated IDC patients, 4 probands of IDC pedigrees, and 100 healthy controls, all of Han nationality and having lived in northern China for a long time. Following echocardiography examination the IDC subjects were stratified according to ejection fraction (EF) values. Those with EF values higher than 50% were placed in subgroup 1, subgroup 2 included the patients with an EF value of 15–35%, and subgroup 3 consisted of those whose EF values were less than 15%. An autoantibody against the myocardial mitochondria ADP/ATP carrier was examined using immunoblot analysis. The frequencies of HLA‐DQA1*0501 and HLA‐DQB1*0303 were 0.3889 and 0.1806 in the IDC group, significantly higher than those of the healthy controls (0.0900 and 0.0364 respectively, both P < 0.05). The OR was 5.20 (95% CI: 3.60–8.50) and 4.85 (95% CI: 2.56–9.39) respectively. Further analysis of the three subgroups showed a higher frequency of HLA‐DQA1*0501 among patients whose EF was less than 15% than those whose EF values were ≥15%. Conversely, the frequencies of HLA‐DQA1*0201 and ‐DQB1*0502, *0504 were significantly lower in the IDC group (0.0139, 0.0139 and 0.0417 respectively) than in the control group (0.2000, 0.0727 and 0.1091 respectively) (P < 0.05). The frequency of the HLA‐DQA1*0501 allele was significantly higher in IDC patients whose autoantibody is positive in contrast with those whose autoantibody is negative (18.57% vs. 5.86%, P < 0.05); the relative risk (RR) was 4.32. The other frequencies of HLA‐DQA1 and ‐DQB1 alleles showed no significant difference in the antibody positive and negative groups of IDC patients. The alleles of HLA‐DQA1*0501 and HLA‐DQB1*0303 were closely associated with poor EF values in the IDC group, and may be involved in susceptibility to the disease. The DQA1*0201 and DQB1*0502, *0504 alleles may confer protection to IDC among individuals of northern Chinese Han nationality. The SER⁵⁷ residue in the second exon of DQB1*0502 and *0504 may confer resistance to IDC, and defects or substitution of this amino acid residue at position 57 of the DQβ chain may be associated with IDC susceptibility. HLA‐DQ allele polymorphisms may serve as genetic markers for IDC and be involved in the regulation of the immune specific response to auto or exterior anti‐myocardium antibodies.     

Association of HLA-DQA1 (rs9272219) with susceptibility to rheumatoid arthritis in a Han Chinese population

HLA-DQA1 (rs9272219) has been previously reported that it is a susceptibility locus in rheumatoid arthritis (RA) of UK Caucasian population and North American; however, it has not reported in RA of Chinese population. Our study was to identify whether or not this relationship is reside between rs9272219 and RA in a Han Chinese population. 207 patients with RA and 199 control subjects were recruited. The single nucleotide polymorphism (SNP) of rs9272219 was tested in alleles and genotype frequencies and the data was analyzed by doing the statistic analysis of odds ratio (OR) and 95% confidence interval (CI) from multivariate unconditional logistic regression analyses after pairwise linkage disequilibrium (LD) was estimated. Finally, the Alleles and genotype frequencies distribution of rs9272219 locus among RA patients and control subjects were in accordance with Hardy-Weinberg equilibrium. We found significant association between rs9272219 and RA of Chinese population (OR 0.494, 95% confidence interval [95% CI] 0.354-0.688, P = 0 and OR 2.541, 95% CI 1.695-3.808, P = 0, respectively). In this study, we found that the SNP of rs9272219 in HLA-DQA1 is a potential susceptibility locus in RA of Han Chinese population; the results suggest that HLA-DQA1 may be related to the development of RA.     

江浙沪地区HLA-DQB1基因对重症肌无力的遗传易感性研究

探讨中国汉人ＭＧ易感性与ＨＬＡ－ＤＱＢ１基因多态性的相关。方法：运用ＰＣＲ－ＲＦＬＰ法进行ＨＬＡ－ＤＱＢ１基因分型。结果：ＭＧ病例组与对照组比较都有ＤＱＢ＊０３０３频率的明显增高,ＤＱＢ＊０６０１和ＤＱＢ１＊０．６０２频率的明显降低,差异都有显著性。结论：ＤＱＢ１＊０３０３参与中国汉人ＭＧ的易感性,而ＤＱＢ１＊０６０１和ＤＱＢ１＊０６０２是保护基因。     

HLA-DQB1基因多态性与中国汉族人群系统性红斑狼疮的相关性

目的 探讨HLA-DQB1基因单核苷酸多态性(single nucleotide polymorphisms,SNP)与汉族人群系统性红斑狼疮(systemic lupus erthematosus,SLE)遗传易感性的相关性.方法 通过聚合酶链式反应-连接酶检测反应(polymerase chain reaction-ligase detection reaction,PCR-LDR)技术对908例SLE患者和961例健康对照rs3129716(HLA-DQB1)位点进行基因分型,同时结合临床表现分型,分析该位点与疾病及临床表型的相关性.分型结果用PLINK1.07软件进行统计分析.结果 rs3129716(HLA-DQB1)位点等位基因频率和基因型频率在SLE疾病组和对照组的分布差异无统计学意义(P＞0.05).三种遗传模型下的分析显示,两组间差异无统计学意义(P＞0.05).将SLE患者按血清学指标及临床表现分型,未发现相关性.结论 rs3129716(HLA-DQB1)与中国汉族人群SLE患者遗传易感性不相关.     

HLA-DQA1 polymorphism in autochthonous Basques from Navarre (Spain): genetic position within European and Mediterranean scopes

In this work, a sample of 112 individuals from an autochthonous Basque population (Northern Navarre, Spain) were typed at the DNA level for the HLA-DQA1 locus, with the aim of characterizing its polymorphism and analyzing the genetic relationships of Basque Navarrese with other Caucasian populations. Northern Navarre is a neighboring area with Guipúzcoa, a province located in the core of the Basque territory having the highest proportion of Basque-speakers. In Navarrese population, the most frequent alleles were DQA1*01 (0.375) and DQA1*02 (0.259). Frequency clines for both DQA1*0103 allele and DQA1*04* allele cluster (including DQA1*0401, DQA1*0501 and DQA1*0601) among the European and Mediterranean populations considered are reported for the first time. Furthermore, a spatial structuring previously described for DQA1*02 allele is corroborated. The information provided by the highly polymorphic HLA-DQA1 locus was stressed by using genetic distances and non-metrical multidimensional scaling (MDS). The analysis of genetic relationships among populations showed a high genetic affinity between the Basque subpopulations of Northern Navarre and Guipúzcoa, which in turn tended to plot separately from the remaining European and Mediterranean populations. In the same way, the Basques showed no clear relationship to North African populations, as postulated in several previous HLA studies. The observed genetic heterogeneity seems to be conditioned by the high frequencies of the DQA1*02 allele in Basques from Guipúzcoa and North Navarre. These two subpopulations seem to show low levels of admixture with other non-Basque neighboring populations, probably because of their deeply rooted ethnicity and the existence of a linguistic barrier to random mating.     

华南、华北人群HLA-DQB1等位基因多态性

目的从基因水平调查了中国华南、华北地区人群HLA-DQB1等位基因频率，并研究比较两地区人群HLA-DQB1多态性分布。方法采用深圳益生堂生物企业有限公司研制开发的“HLA-DQB1低分辨率分型基因芯片检测试剂盒”，应用聚合酶链反应．序列特异性引物＋序列特异性寡核苷酸探针芯片检测技术，对700名南方地区的中国人和320名北方地区的中国人进行基因分型。结果鉴定了10个HLA-DQB1等位基因，获得了一组准确、科学的统计数据。结论得到了中国华南、华北地区人群HLA-DQB1等位基因频率差异的数据，证明中国人群HLA-DQB1＊02，05，0601，0602，0603的分布南北差异有统计学意义（P〈0．05），为疾病相关性研究、人文科学研究提供了可靠的遗传学数据。