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An improved method for characterization of the mutation associated to porcine stress syndrome by PCR amplification followed by restriction analysis

机译:一种通过PCR扩增和限制性酶切分析表征猪应激综合征相关突变的改进方法

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摘要

A mutation in the gene coding for the ryanodine receptor 1 (RYR1), also known as halothane (hal) gene or swine stress gene, is associated to the porcine stress syndrome (PSS). Detection of the mutation is normally accomplished by PCR amplification of an 81bp fragment of the hal gene, followed by digestion with the HhaI restriction endonuclease. Wild-type allele (N) is cut in two fragments, whereas the mutant allele (n) is not digested by the restriction enzyme. Electrophoresis of the digested DNA on agarose gel and ethidium bromide staining allows the reading of the result. The correct interpretation is difficult due to the small size of the DNA fragments. In this study we designed a new set of primers for amplification of a 144bp fragment that facilitates the reading of the result. In addition, we optimized the PCR reaction to allow amplification from a single hair bulb, added directly into the PCR mix without previous treatment. This improved method was used to genotype 165 sows and boars used in a breeding program. Forty-nine percent of the animals had the NN genotype, whereas 50% were Nn and only 1% was nn.
机译:编码ryanodine受体1(RYR1)的基因中的突变(也称为氟烷(hal)基因或猪应激基因)与猪应激综合症(PSS)相关。突变的检测通常通过对hal基因的81bp片段进行PCR扩增,然后用HhaI限制性核酸内切酶消化来完成。野生型等位基因(N)被切成两个片段,而突变型等位基因(n)不被限制酶消化。琼脂糖凝胶上消化的DNA电泳和溴化乙锭染色可读取结果。由于DNA片段较小,因此很难正确解释。在这项研究中,我们设计了一套新的引物,用于扩增144bp片段,从而有助于读取结果。此外,我们优化了PCR反应,以允许从单个毛鳞茎中扩增,无需事先处理即可直接添加到PCR混合物中。该改良方法用于对育种程序中使用的165头母猪和公猪进行基因分型。 49%的动物具有NN基因型,而50%的动物为Nn,只有1%的动物为nn。

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