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首页> 外文期刊>Food Biotechnology >Application of PCR and SYBR green Q Rti-PCR assays for the identification and quantification of chicken meat under different cooking conditions.
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Application of PCR and SYBR green Q Rti-PCR assays for the identification and quantification of chicken meat under different cooking conditions.

机译:PCR和SYBR green Q Rti-PCR分析法在不同烹饪条件下鸡肉的鉴定和定量中的应用。

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Conventional and SYBR Green Q Rti-PCR assays using primers targeting the 12S rRNA of chicken mitochondrial genes were employed for the detection and quantification of chicken used in food stuffs. The assays were recruited to amplify different known concentrations of DNA in the mixtures. Different kinds of processed meats were prepared using various amounts of chicken that were heated at different temperatures in order to detect the chicken in the mixtures. The PCR amplification of DNA revealed that the assay can amplify the species-specific amplicons as little as 0.01 ng of DNA in PCR reactions. Different concentrations of raw chicken were detected based on the threshold cycle. The technique was able to detect from 5% to 90% ratios of the chicken materials in sausages. Analysis of the experimental meat mixtures revealed the usefulness of the assays in detecting and quantifying chicken mitochondrial DNA in the mixtures
机译:使用靶向鸡线粒体基因12S rRNA的引物的常规和SYBR Green Q Rti-PCR分析法用于食品中鸡肉的检测和定量。招募化验以扩增混合物中DNA的不同已知浓度。为了检测混合物中的鸡肉,使用了在不同温度下加热的各种数量的鸡肉制备了不同种类的加工肉。 DNA的PCR扩增显示,该检测法可在PCR反应中扩增出仅0.01 ng DNA的物种特异性扩增子。根据阈值周期检测到不同浓度的生鸡肉。该技术能够检测香肠中5%至90%的鸡肉原料。对实验性肉混合物的分析揭示了该测定法在检测和定量混合物中鸡线粒体DNA方面的有用性

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