A quantitative PCR approach to determine gene copy number

P. Solomon, Simon V. S. Ipcho, James K. Hane, K. Tan, R. Oliver
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引用次数: 51

Abstract

Here, we report on the use of quantitative PCR (qPCR) to determine gene copy number in filamentous fungi. Using the sequenced dothideomycete Stagonospora nodorum, qPCR was used to unequivocally confirm the presence of single, two and three copy regions as predicted by in silico PCR. Further validation of the technique was demonstrated by verifying the copy numbers of introduced gene cassettes in previously characterised transformants of S. nodorum. Apart from increased sensitivity, this technique offers a high-throughput alternative to Southern blots for determining gene copy number, a
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测定基因拷贝数的定量PCR方法
在这里,我们报告了使用定量PCR (qPCR)来确定丝状真菌的基因拷贝数。利用已测序的鹿角孢子菌,qPCR明确证实了单、二、三拷贝区域的存在,与PCR预测的一致。进一步验证该技术是通过验证引入的基因盒的拷贝数在先前表征的诺氏葡萄球菌的转化。除了提高灵敏度外,该技术还提供了一种高通量替代Southern blots测定基因拷贝数的方法
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