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首页> 外文期刊>Veterinary Immunology and Immunopathology >Specific TaqMan probed real-time quantitative RT-PCR methods and their application to differentiate the transcripts of duplicated BF or BLB genes in chicken MHC
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Specific TaqMan probed real-time quantitative RT-PCR methods and their application to differentiate the transcripts of duplicated BF or BLB genes in chicken MHC

机译:TaqMan探针实时定量RT-PCR方法及其在区分鸡MHC中重复的BF或BLB基因转录本中的应用

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摘要

BF and BLB genes of chicken major histocompatibility complex (MHC) are responsible for classical antigen processing and presentation; therefore they play a central role in determining the genetic resistance or susceptibility of different MHC-B haplotypes to some infectious diseases. In this study, we developed specific TaqMan probed real-time quantitative reverse transcription PCR (TaqMan qRT-PCR) methods based on the diagnostic nucleotide polymorphisms present in duplicated BE or BLB genes in B2 and B19 haplotypes. The results showed very similar amplification efficiency but no cross-reaction between the duplicated BF or BLB genes of the same haplotype. Spleen mRNA samples of B2 and B19 chickens were used to validate these TaqMan qRT-PCR methods. We observed that BF2 or BLB2 gene was dominantly transcribed in all B2 and B19 chickens. Our findings verified the impact of diversified promoter sequences on the function of duplicated BE or BLB genes. Hence the principles adopted to establish these specific TaqMan qRT-PCR methods in this study can be applied to differentiate the transcripts of duplicated BE or BLB genes of other MHC-B haplotypes in chicken. (C) 2012 Elsevier B.V. All rights reserved.
机译:鸡主要组织相容性复合体(MHC)的BF和BLB基因负责经典抗原的加工和呈递。因此,它们在确定不同MHC-B单倍型对某些传染病的遗传抗性或易感性中起着核心作用。在这项研究中,我们基于B2和B19单倍型中重复的BE或BLB基因中存在的诊断核苷酸多态性,开发了特定的TaqMan探针实时定量逆转录PCR(TaqMan qRT-PCR)方法。结果显示,扩增效率非常相似,但是相同单倍型的重复BF或BLB基因之间没有交叉反应。使用B2和B19鸡的脾脏mRNA样本来验证这些TaqMan qRT-PCR方法。我们观察到,BF2或BLB2基因在所有B2和B19鸡中均被显性转录。我们的发现证实了多样化的启动子序列对重复的BE或BLB基因功能的影响。因此,本研究中建立这些特定TaqMan qRT-PCR方法所采用的原理可用于区分鸡中其他MHC-B单倍型的重复BE或BLB基因的转录本。 (C)2012 Elsevier B.V.保留所有权利。

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