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Separation of the Messenger RNAs of Newcastle Disease Virus by Gel Electrophoresis

机译:凝胶电泳分离新城疫病毒信使RNA

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摘要

We have separated the 18-22S putative messenger RNA of Newcastle disease virus into seven species ranging in molecular weight from 0.55 to 1.53 × 106 using sodium dodecyl sulfate-acrylamide-gel electrophoresis at relatively high concentrations of acrylamide and for a relatively long time. Studies of the number and molecular weights of the proteins and the 18-22S RNAs of the virus suggests that these RNAs are in the right molecular weight range to code for the known proteins of Newcastle disease virus. In preliminary studies using this separation technique, we have demonstrated that: (a) there is no difference between the 18-22S RNA made during a normal infection and when genome replication is blocked; and (b) there is a strain-specific difference between the RNAs of Newcastle disease virus-AV and Newcastle disease virus-HP.
机译:我们已经使用十二烷基硫酸钠-丙烯酰胺-凝胶电泳在相对较高的丙烯酰胺浓度下和相对较长的时间,将新城疫病毒的18-22S信使RNA分为7种,分子量从0.55至1.53×106。对蛋白质和病毒的18-22S RNA的数量和分子量的研究表明,这些RNA在正确的分子量范围内,可编码新城疫病毒的已知蛋白质。在使用这种分离技术的初步研究中,我们证明:(a)在正常感染过程中和基因组复制受阻时,18-22S RNA之间没有差异; (b)新城疫病毒-AV和新城疫病毒-HP的RNA之间存在菌株特异性差异。

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