Structural Basis for the Transition from Initiation to Elongation Transcription in T7 RNA Polymerase

Artigo Acesso aberto Revisado por pares

Structural Basis for the Transition from Initiation to Elongation Transcription in T7 RNA Polymerase

2002; American Association for the Advancement of Science; Volume: 298; Issue: 5597 Linguagem: Inglês

10.1126/science.1077464

ISSN

1095-9203

Autores

Y. Whitney Yin, Thomas A. Steitz,

Tópico(s)

RNA and protein synthesis mechanisms

Resumo

To make messenger RNA transcripts, bacteriophage T7 RNA polymerase (T7 RNAP) undergoes a transition from an initiation phase, which only makes short RNA fragments, to a stable elongation phase. We have determined at 2.1 angstrom resolution the crystal structure of a T7 RNAP elongation complex with 30 base pairs of duplex DNA containing a “transcription bubble” interacting with a 17-nucleotide RNA transcript. The transition from an initiation to an elongation complex is accompanied by a major refolding of the amino-terminal 300 residues. This results in loss of the promoter binding site, facilitating promoter clearance, and creates a tunnel that surrounds the RNA transcript after it peels off a seven–base pair heteroduplex. Formation of the exit tunnel explains the enhanced processivity of the elongation complex. Downstream duplex DNA binds to the fingers domain, and its orientation relative to upstream DNA in the initiation complex implies an unwinding that could facilitate formation of the open promoter complex.

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Structural Basis for the Transition from Initiation to Elongation Transcription in T7 RNA Polymerase