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Factors influencing the accuracy of measurements with real-time PCR: The example of the determination of processed animal proteins.

机译:影响实时PCR测量准确性的因素:确定加工动物蛋白的示例。

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Quantification of traces of processed animal proteins (PAPs) in feedingstuffs is an important requirement to enforce upcoming European legislation on the use of these materials in animal nutrition. One of the techniques proposed in this context is real-time polymerase chain reaction (real-time PCR) allowing for the determination of PAPs at various taxonomic levels. A challenge in this field is the fact that real-time PCR measures DNA copy numbers, whereas legislation expresses tolerance limits in terms of mass fractions of PAPs in feedingstuffs. Here, we evaluated the impact of different sterilisation temperatures performed under real world rendering conditions showing that at high temperatures the DNA copy number was significantly reduced. This effect complicates the determination of the PAPs mass fraction in feedingstuffs by means of real-time PCR. In addition we showed that measuring at trace levels could lead to a high variation of the measured DNA copy number, characterised by a positively skewed distribution. Various implications of these findings are discussed. All rights reserved, Elsevier.
机译:饲料中痕量加工动物蛋白(PAP)的定量是执行即将实施的有关在动物营养中使用这些材料的欧洲法规的一项重要要求。在这种情况下提出的技术之一是实时聚合酶链反应(实时PCR),可用于确定各种分类学水平上的PAP。该领域的一个挑战是实时PCR测量DNA拷贝数的事实,而立法以饲料中PAP的质量分数来表示耐受极限。在这里,我们评估了在现实世界渲染条件下执行的不同灭菌温度的影响,结果表明在高温下,DNA的拷贝数显着减少。这种效果使通过实时PCR测定饲料中PAPs质量分数变得复杂。此外,我们表明以痕量水平进行测量可能会导致所测量的DNA拷贝数发生较大变化,其特征是正偏分布。讨论了这些发现的各种含义。保留所有权利,Elsevier。

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