Control of formation of two distinct classes of RNA polymerase II elongation complexes.

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Mol Cell Biol. 1992 May; 12(5): 2078-2090

Control of formation of two distinct classes of RNA polymerase II elongation complexes.

N F Marshall and D H Price

Department of Biochemistry, University of Iowa, Iowa City 52242.

ABSTRACT

We have examined elongation by RNA polymerase II initiated ata promoter and have identified two classes of elongation complexes.Following initiation at a promoter, all polymerase moleculesenter an abortive mode of elongation. Abortive elongation ischaracterized by the rapid generation of short transcripts dueto pausing of the polymerase followed by termination of transcription.Termination of the early elongation complexes can be suppressedby the addition of 250 mM KCl or 1 mg of heparin per ml soonafter initiation. Elongation complexes of the second class carryout productive elongation in which long transcripts can be synthesized.Productive elongation complexes are derived from early pausedelongation complexes by the action of a factor which we callP-TEF (positive transcription elongation factor). P-TEF is inhibitedby 5,6-dichloro-1-beta-D-ribofuranosylbenzimidazole at concentrationswhich have no effect on the initiation of transcription. Byusing templates immobilized on paramagnetic particles, we showthat isolated preinitiation complexes lack P-TEF and give riseto transcription complexes which can carry out only abortiveelongation. The ability to carry out productive elongation canbe restored to isolated transcription complexes by the additionof P-TEF after initiation. A model is presented which describesthe role of elongation factors in the formation and maintenanceof elongation complexes. The model is consistent with the availablein vivo data concerning control of elongation and is used topredict the outcome of other potential in vitro and in vivoexperiments.

Mol Cell Biol. 1992 May; 12(5): 2078-2090

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