Stability of Drosophila RNA polymerase II elongation complexes in vitro.

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Mol Cell Biol. 1992 May; 12(5): 2067-2077

Stability of Drosophila RNA polymerase II elongation complexes in vitro.

D D Kephart, N F Marshall and D H Price

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

ABSTRACT

We show that nuclear extract from Drosophila Kc cells supportsefficient elongation by RNA polymerase II initiated from theactin 5C promoter. The addition of 0.3% Sarkosyl, 1 mg of heparinper ml, or 250 mM KCl immediately after initiation has two effects.First, the elongation rate is reduced 80 to 90% as a resultof the inhibition of elongation factors. Second, there is anincrease in the amount of long runoff RNA, suggesting that thereis an early block to elongation that is relieved by the disruptivereagents. Consistent with the first effect, we find that theability of factor 5 (TFIIF) to stimulate the elongation rateis inhibited by the disruptive agents when assayed in a definedsystem containing pure RNA polymerase II and a dC-tailed template.The disruptive agents also inhibit the ability of DmS-II tosuppress transcriptional pausing but only slightly reduce theability of DmS-II to increase the elongation rate twofold. Thepause sites encountered by RNA polymerase II after initiationat a promoter and subsequent treatment with the disruptive reagentsare also recognized by pure polymerase transcribing a dC-tailedtemplate. It has been suggested that 5,6-dichloro-1-beta-D-ribofuranosylbenzimidazoleinhibits RNA polymerase II during elongation, but we find thatthe purine nucleoside analog has no effect on elongation complexescontaining RNA over 500 nucleotides in length or on the actionof factor 5 or DmS-II in the defined system.

Mol Cell Biol. 1992 May; 12(5): 2067-2077

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