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首页> 外文期刊>BMC research notes >Quantitative real-time PCR with SYBR Green detection to assess gene duplication in insects: study of gene dosage in Drosophila melanogaster (Diptera) and in Ostrinia nubilalis (Lepidoptera)
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Quantitative real-time PCR with SYBR Green detection to assess gene duplication in insects: study of gene dosage in Drosophila melanogaster (Diptera) and in Ostrinia nubilalis (Lepidoptera)

机译:实时荧光定量PCR和SYBR Green检测可评估昆虫中的基因重复性:研究果蝇(Dipophila melanogaster(Diptera))和成虫Ostrinia nubilalis(鳞翅目)的基因剂量

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Background The accurate determination of the number of copies of a gene in the genome (gene dosage) is essential for a number of genetic analyses. Quantitative real time PCR (qPCR) with TaqMan detection has shown advantages over traditional Southern-blot and FISH techniques, however the high costs of the required labeled probes is an important limitation of this method. qPCR with SYBR Green I detection is a simple and inexpensive alternative, but it has never been applied to the determination of the copy number of low copy number genes in organisms with high allelic variability (as some insects), where a very small margin of error is essential. Findings We have tested the suitability of the qPCR with SYBR Green I detection methodology for the detection of low copy number genes in two insects: the genetically well characterized Drosophila melanogaster (Diptera) and the poor genetically characterized Ostrinia nubilalis (Lepidoptera). The system was applied to determine the copy number of: (1) the O. nubilalis cadherin gene, involved in the mode of action of Bacillus thuringiensis toxins, which showed indirect evidence of duplication, and (2) the D. melanogaster BarH1 and BarH2 genes, located within the Bar region of the X chromosome, to clearly determine whether they both are covered by the tandem duplication in the classical Bar ( B 1 ) mutant. Our results showed that the O. nubilalis cadherin gene is an autosomal single copy gene and that BarH1 , but not BarH2 , is duplicated in the Drosophila B 1 mutant. Conclusions This work shows that qPCR with SYBR Green I detection can be specific and accurate enough to distinguish between one and two gene copies per haploid genome of genes with high allelic variability. The technique is sensitive enough to give reliable results with a minimum amount of sample (DNA from individual thoraxes) and to detect gene duplications in tandem.
机译:背景技术准确确定基因组中基因拷贝数(基因剂量)对于许多遗传分析至关重要。具有TaqMan检测功能的定量实时PCR(qPCR)已显示出优于传统的Southern印迹和FISH技术的优势,但是所需标记探针的高成本是该方法的重要限制。带有SYBR Green I检测的qPCR是一种简单且廉价的替代方法,但从未应用于确定等位基因变异性高的生物体(如某些昆虫)中低拷贝数基因的拷贝数,其中误差很小是必不可少的。研究结果我们已经用SYBR Green I检测方法测试了qPCR在两种昆虫中检测低拷贝数基因的适用性:遗传学上具有良好特征的黑腹果蝇(Diptera)和遗传学上较差的脐橙(鳞翅目)。该系统用于确定以下基因的拷贝数:(1)参与苏云金芽孢杆菌毒素作用方式的脐橙钙粘蛋白基因,它显示出重复的间接证据;(2)黑腹果蝇BarH1和BarH2基因位于X染色体的Bar区域内,以清楚地确定它们是否都被经典Bar(B 1 )突变体中的串联复制所覆盖。我们的结果表明,O。nubilalis cadherin基因是常染色体单拷贝基因,在果蝇B 1 突变体中,BarH1但不是BarH2是重复的。结论这项工作表明,采用SYBR Green I检测的qPCR具有足够的特异性和准确性,可以区分具有高等位基因变异性的每个单倍体基因组一个和两个基因拷贝。该技术足够灵敏,可以用最少的样品(来自单个胸腔的DNA)给出可靠的结果,并可以一前一后地检测基因重复。

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