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首页> 外文期刊>Tissue antigens. >Identification of DRB alleles in rhesus monkeys using polymerase chain reaction-sequence-specific primers (PCR-SSP) amplification.
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Identification of DRB alleles in rhesus monkeys using polymerase chain reaction-sequence-specific primers (PCR-SSP) amplification.

机译:使用聚合酶链反应序列特异性引物(PCR-SSP)扩增鉴定恒河猴中的DRB等位基因。

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Major histocompatibility complex (MHC) class In molecules play a vital role in the regulation of T-cell functions in the mammalian immune system. Two key features characterize the polymorphism of MHC haplotypes in humans and non-human primates: the existence of a large number of alleles, and the high degree of genetic diversity between those alleles. Rhesus monkeys and Chimpanzees have been extensively used as relevant models for human diseases and transplantation We have investigated DRB genes in 19 macaques, members of 3 families, using polymerase chain reaction with sequence-specific primers (PCR-SSP) and denaturing gradient gel electrophoresis (DGGE). After amplification PCR products were purified and subjected direct sequencing. Seven animals (Madison #1) were typed by DDGE also. We report that the DRB haplotypes defined by PCR-SSP exhibit a high degree of concordance with the data obtained by DGGE and direct sequening. Our data show prominent variability in the number of DRB1 alleles ranging from 1-4 per genotype within these families. This analysis demonstrated that most of the amplicons were identical to Mamu-DRB alleles that our PCR primers were to amplify. However, 98-99% similarity was noticed in the case of Mamu-DRB1*0303, Mamu-DRB6*0103 and Mamu-DRB*W201 alleles. The observed mismatches were located in non-polymorphic regions. Thus, family studies in rhesus macaques performed by molecular methods confirmed the multiplicity of Mamu-DRB1 alleles per haplotype and the existence of allelic associations published earlier. In addition, we propose 3 more DRB allele associations (haplotypes): Mamu-DRB1*04-DRB5*03; Mamu-DRB1*04-*DRB*W5; Mamu-DRB1*04*W2. The proposed medium-resolution PCR-SSP technique appears to be a highly reproducible and discriminatory typing method for detecting polymorphisms of DRB genes in rhesus monkeys.
机译:主要的组织相容性复合体(MHC)类分子在哺乳动物免疫系统中T细胞功能的调节中起着至关重要的作用。人类和非人类灵长类动物中MHC单倍型的多态性具有两个关键特征:存在大量等位基因,以及这些等位基因之间的高度遗传多样性。恒河猴和黑猩猩已被广泛用作人类疾病和移植的相关模型。我们已通过序列特异性引物(PCR-SSP)的聚合酶链反应和变性梯度凝胶电泳对3个科的19只猕猴的DRB基因进行了研究( DGGE)。扩增后,纯化PCR产物并进行直接测序。 DDGE也输入了7只动物(Madison#1)。我们报告说,PCR-SSP定义的DRB单倍型与DGGE和直接测序获得的数据高度一致。我们的数据显示这些家族中DRB1等位基因的数量在每个基因型中介于1-4之间。该分析表明,大多数扩增子与我们的PCR引物将扩增的Mamu-DRB等位基因相同。但是,在Mamu-DRB1 * 0303,Mamu-DRB6 * 0103和Mamu-DRB * W201等位基因中,发现98-99%的相似性。观察到的错配位于非多态区域。因此,通过分子方法在恒河猴中进行的家族研究证实了每个单倍型的Mamu-DRB1等位基因的多样性以及早先发表的等位基因关联的存在。此外,我们提出了3个其他DRB等位基因关联(单体型):Mamu-DRB1 * 04-DRB5 * 03; Mamu-DRB1 * 04- * DRB * W5; Mamu-DRB1 * 04 * W2。拟议的中等分辨率PCR-SSP技术似乎是一种高度可重复且具有区别性的打字方法,用于检测恒河猴DRB基因的多态性。

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