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使用改良的实时定量PCR技术筛查人类β-防御素基因中的拷贝数多态性

Screening of copy number polymorphisms in human beta-defensin genes using modified real-time quantitative PCR.

作者信息

Chen QiXing, Book Malte, Fang XiangMing, Hoeft Andreas, Stuber Frank

机构信息

Department of Anaesthesiology and Intensive Care Medicine, University of Bonn, 53105 Bonn, Germany.

出版信息

J Immunol Methods. 2006 Jan 20;308(1-2):231-40. doi: 10.1016/j.jim.2005.11.001. Epub 2005 Dec 15.

DOI:10.1016/j.jim.2005.11.001
PMID:16380128
Abstract

Defensins are cationic antimicrobial peptides, which play an important role in host immune defense to some infectious diseases as well as immune disease and skin disease. Recent studies identified that the genes coding for human beta-defensin 2 (DEFB4), human beta-defensin 3 (DEFB103) and human beta-defensin 4 (DEFB104) showed variation in copy numbers. This variation may have an impact on gene expression levels. Here, we have demonstrated a real-time PCR-based method to measure beta-defensin gene copy number. Using this relative real-time quantitative PCR, we developed a new rapid and reliable approach, which involves amplification of the target locus (DEFB4 or DEFB103 or DEFB104) and the single-copy reference locus (human serum albumin, ALB) in a single PCR reaction. A calibrator was prepared by recombining one copy of the target gene and one copy of the reference gene into a plasmid. After correcting the PCR amplification efficiency, which differed between the defensin gene and ALB gene, and normalization by the calibrator, the ratio of the copy number of the target gene to that of the reference gene in an unknown sample was determined. This normalized ratio directly related to the gene copy number. The assay was validated using previously genotyped samples, which demonstrated high accuracy and reliability of the method. Furthermore, this method was used to screen the copy number variations of these three beta-defensin genes in healthy blood donors. This method proved to be a reliable and fast tool to genotype gene copy number variations in projects associating genomic variations with gene expression or with population phenotypes in epidemiologic studies.

摘要

防御素是阳离子抗菌肽,在宿主对某些传染病以及免疫疾病和皮肤病的免疫防御中发挥重要作用。最近的研究发现,编码人β-防御素2(DEFB4)、人β-防御素3(DEFB103)和人β-防御素4(DEFB104)的基因在拷贝数上存在变异。这种变异可能会影响基因表达水平。在此,我们展示了一种基于实时PCR的方法来测量β-防御素基因的拷贝数。使用这种相对实时定量PCR,我们开发了一种新的快速可靠的方法,该方法涉及在单个PCR反应中扩增靶基因座(DEFB4或DEFB103或DEFB104)和单拷贝参考基因座(人血清白蛋白,ALB)。通过将一个拷贝的靶基因和一个拷贝的参考基因重组到质粒中来制备校准物。在校正了防御素基因和ALB基因之间不同的PCR扩增效率,并通过校准物进行归一化后,确定未知样品中靶基因拷贝数与参考基因拷贝数的比率。这种归一化比率直接与基因拷贝数相关。使用先前进行基因分型的样品对该测定法进行了验证,结果表明该方法具有很高的准确性和可靠性。此外,该方法还用于筛查健康献血者中这三种β-防御素基因的拷贝数变异。在将基因组变异与基因表达或流行病学研究中的群体表型相关联的项目中,该方法被证明是一种可靠且快速的基因拷贝数变异基因分型工具

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