Title of article
Mechanism for De Novo RNA Synthesis and Initiating Nucleotide Specificity by T7 RNA Polymerase
Author/Authors
William P. Kennedy، نويسنده , , Jamila R. Momand، نويسنده , , Y. Whitney Yin، نويسنده ,
Issue Information
روزنامه با شماره پیاپی سال 2007
Pages
13
From page
256
To page
268
Abstract
DNA-directed RNA polymerases are capable of initiating synthesis of RNA without primers, the first catalytic stage of initiation is referred to as de novo RNA synthesis. De novo synthesis is a unique phase in the transcription cycle where the RNA polymerase binds two nucleotides rather than a nascent RNA polymer and a single nucleotide. For bacteriophage T7 RNA polymerase, transcription begins with a marked preference for GTP at the + 1 and + 2 positions. We determined the crystal structures of T7 RNA polymerase complexes captured during the de novo RNA synthesis. The DNA substrates in the structures in the complexes contain a common Φ10 duplex promoter followed by a unique five base single-stranded extension of template DNA whose sequences varied at positions + 1 and + 2, thereby allowing for different pairs of initiating nucleotides GTP, ATP, CTP or UTP to bind. The structures show that the initiating nucleotides bind RNA polymerase in locations distinct from those described previously for elongation complexes. Selection bias in favor of GTP as an initiating nucleotide is accomplished by shape complementarity, extensive protein side-chain and strong base-stacking interactions for the guanine moiety in the enzyme active site. Consequently, an initiating GTP provides the largest stabilization force for the open promoter conformation.
Keywords
de novo RVA synthesis , T7 RNA polymerase , GTP specificity
Journal title
Journal of Molecular Biology
Serial Year
2007
Journal title
Journal of Molecular Biology
Record number
1249503
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