Synergism in replication and translation of messenger RNA in a cell-free system

  1. I Y Morozov,
  2. V I Ugarov,
  3. A B Chetverin, and
  4. A S Spirin
  1. Institute of Protein Research, Russian Academy of Sciences, Pushchino, Moscow Region.

Abstract

Combination of the Q beta replicase reaction with the Escherichia coli cell-free translation system markedly enhances replication of a recombinant RQ-DHFR RNA consisting of the dihydrofolate reductase (DHFR) mRNA sequence inserted into RQ135(-1) RNA, an efficient naturally occurring Q beta replicase template. The enhancement is associated with a replication asymmetry previously described for the replication of Q beta phage RNA in vivo; the sense (+)-strands are produced in large excess over the antisense (-)-strands. This, in turn, results in increased synthesis of the functionally active DHFR. These effects are not observed when DHFR mRNAs or RQ135(-1) RNAs are used as templates, if the translation system is not complete, or if it is inhibited by puromycin. The coupled replication-translation of nonviral mRNA recombinants can serve as a useful model for studying the fundamental aspects of virus amplification and can be implemented for large-scale protein synthesis in vitro.

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  1. PNAS October 15, 1993 vol. 90 no. 20 9325-9329
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