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A Novel Method for the Preparation of Template DNA for PCR from Beer to Detect Materials and to Develop DNA Markers to Evaluate the Quality of Beer

机译:从啤酒中制备用于PCR的模板DNA的新方法,以检测材料并开发DNA标记物以评估啤酒的质量

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We developed a method for the preparation of template DNAs for polymerase chain reaction (PCR) from beer. We improved the method by (i) lyophilizing and pulverizing the beer to concentrate DNAs, (ii) decomposition of polysaccharides and proteins so as not to inhibit DNA extraction by the use of heat-resistant amylase and proteinase K, (iii) separation of template DNA by purification using 70% EtOH extraction and isopropyl alcohol precipitation, and (iv) the use of magnetic beads to purify DNA. We developed suitable 7 STS (sequence-tagged site) primers related to beer quality for PCR, and it proved possible to identify 16 dominant malting barley cultivars and 22 kinds of beers. To digitize the results of PCR, discriminative DNA bands were binarized as 0 (disappeared) or 1 (appeared) and subjected to multiple regression analysis. Estimation formulae for the quality of beer were developed using the above-mentioned independent variables based on the results of PCR against dependent variables related to the qualities of beer, including foam stability, bitterness, sourness and astringency. These equations showed multiple regression coefficients of 0.93, 0.82, 0.87, and 0.87 for calibration.
机译:我们开发了一种从啤酒中制备用于聚合酶链反应(PCR)的模板DNA的方法。我们通过以下方法改进了方法:(i)冻干并粉碎啤酒以浓缩DNA,(ii)分解多糖和蛋白质,以免通过使用耐热淀粉酶和蛋白酶K抑制DNA提取,(iii)分离模板通过使用70%乙醇萃取和异丙醇沉淀的方法纯化DNA,以及(iv)使用磁珠纯化DNA。我们开发了7种与啤酒质量相关的STS(序列标记位点)引物用于PCR,证明有可能鉴定出16个主要的制麦大麦品种和22种啤酒。为了数字化PCR结果,将区分性DNA条带二值化为0(消失)或1(出现),并进行多元回归分析。基于PCR的结果,针对与啤酒质量相关的因变量(包括泡沫稳定性,苦味,酸味和涩味),使用上述自变量开发了啤酒质量的估算公式。这些方程式显示了0.93、0.82、0.87和0.87的多重回归系数以进行校准。

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