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Excess antisense RNA from infectious recombinant SV40 fails to inhibit expression of a transfected, interferon-inducible gene

机译:来自感染性重组sV40的过量反义RNa不能抑制转染的干扰素诱导型基因的表达

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摘要

SV40-based infectious virus constructs were used to produce a high copy number of full-length antisense RNA in essentially every cell in a population. Chloramphenicol acetyltransferase (CAT) cDNA was placed in either the sense or antisense orientation relative to the SV40 early promoter in helper-free recombinant virus. RNA synthesized at high levels from the antisense virus was without effect on the expression of a stably-transfected CAT mini-gene controlled by an interferon-inducible promoter in monkey CV1 and large T antigen-expressing tsCOS cells. In double infection experiments the antisense RNA was similarly without effect on expression from CAT cDNA placed in the sense orientation in a second virus vector. No activation of the ppp(A2'p)nA(n greater than or equal to 2) system was observed after interferon treatment in either type of experiment. There was no evidence, therefore, for the formation of double-stranded (ds)RNA. It can be concluded that a large excess of a full-length antisense RNA is not necessarily sufficient to cause inhibition of gene expression even when interferon treatment is used to enhance any effect of dsRNA.
机译:基于SV40的感染性病毒构建体用于在种群中的每个细胞中产生高拷贝数的全长反义RNA。在无辅助重组病毒中,相对于SV40早期启动子,氯霉素乙酰转移酶(CAT)cDNA处于有义或反义方向。从反义病毒高水平合成的RNA对在猴CV1和表达T大的tsCOS细胞中受干扰素诱导的启动子控制的稳定转染的CAT基因的表达没有影响。在双重感染实验中,反义RNA类似地对以第二种病毒载体的有义方向放置的CAT cDNA的表达没有影响。在任一类型的实验中,干扰素治疗后均未观察到ppp(A2'p)nA(n大于或等于2)系统的活化。因此,没有证据表明双链(ds)RNA的形成。可以得出结论,即使使用干扰素治疗来增强dsRNA的任何作用,全长反义RNA的大量过量也不一定足以引起基因表达的抑制。

著录项

  • 作者

    Kerr, S M; Stark, G R; Kerr, I M;

  • 作者单位
  • 年度 1988
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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