Literature DB >> 3546320

Interactions of a proteolytically nicked RNA polymerase of bacteriophage T7 with its promoter.

R A Ikeda, C C Richardson.   

Abstract

The association of nicked RNA polymerase of bacteriophage T7 (Ikeda, R. A., and Richardson, C. C. (1987) J. Biol. Chem. 262, 3790-3799) with the T7 phi 10 promoter has been examined by DNA cleavage protection. The phi 10 promoter consists of a 23-base pair consensus sequence that extends from -17 to +6 with respect to the site of the initiation of transcription (+1). Nicked T7 RNA polymerase alone protects 20 bases from -21 to -2 (+/- 1) base at each border. Initiation and synthesis of the trinucleotide r(GGG) expands and shifts the sequence protected by nicked T7 RNA polymerase. Twenty-five bases are protected from -17 to +8 (+/- 1). The polymerization of three additional ribonucleotides, synthesis of the hexamer r(GGGAGA), further expands the protected sequence. Twenty-seven bases are protected from -17-+10 (+/- 1). Finally, the synthesis of a pentadecaribonucleotide transcript, r(GGGAGACCACGG), leads to the formation of a transcription complex that protects 22 bases from -2-+20 (+/- 1). In comparison to the sequences protected by T7 RNA polymerase the sequences protected by the nicked enzyme are shortened at the 5' end and are translocated downstream much earlier during the initiation of transcription. It appears that a portion of the DNA contacts made at the amino terminus of T7 RNA polymerase are disrupted in the small fragment of nicked T7 RNA polymerase. The changes that are observed in the sequences protected by nicked T7 RNA polymerase are reflected in the physical characteristics of the DNA X enzyme complexes. The number of ion pairs formed by the r(GGG)-initiated complex of the nicked enzyme is reduced, and the association constant for the formation of the r(GGG)-initiated complex is decreased as compared to the intact T7 RNA polymerase.

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Year:  1987        PMID: 3546320

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  12 in total

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Authors:  B S Chan; D A Court; P J Vierula; H Bertrand
Journal:  Curr Genet       Date:  1991-08       Impact factor: 3.886

3.  A Highly Productive, One-Pot Cell-Free Protein Synthesis Platform Based on Genomically Recoded Escherichia coli.

Authors:  Benjamin J Des Soye; Vincent R Gerbasi; Paul M Thomas; Neil L Kelleher; Michael C Jewett
Journal:  Cell Chem Biol       Date:  2019-11-06       Impact factor: 8.116

4.  New insights into the mechanism of initial transcription: the T7 RNA polymerase mutant P266L transitions to elongation at longer RNA lengths than wild type.

Authors:  Luis E Ramírez-Tapia; Craig T Martin
Journal:  J Biol Chem       Date:  2012-08-24       Impact factor: 5.157

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Authors:  Thomas A Steitz
Journal:  EMBO J       Date:  2006-08-09       Impact factor: 11.598

6.  Library of synthetic transcriptional AND gates built with split T7 RNA polymerase mutants.

Authors:  David L Shis; Matthew R Bennett
Journal:  Proc Natl Acad Sci U S A       Date:  2013-03-11       Impact factor: 11.205

7.  ompT encodes the Escherichia coli outer membrane protease that cleaves T7 RNA polymerase during purification.

Authors:  J Grodberg; J J Dunn
Journal:  J Bacteriol       Date:  1988-03       Impact factor: 3.490

8.  Abortive initiation by bacteriophage T3 and T7 RNA polymerases under conditions of limiting substrate.

Authors:  M L Ling; S S Risman; J F Klement; N McGraw; W T McAllister
Journal:  Nucleic Acids Res       Date:  1989-02-25       Impact factor: 16.971

Review 9.  The structural changes of T7 RNA polymerase from transcription initiation to elongation.

Authors:  Thomas A Steitz
Journal:  Curr Opin Struct Biol       Date:  2009-10-05       Impact factor: 6.809

10.  A mutant T7 RNA polymerase as a DNA polymerase.

Authors:  R Sousa; R Padilla
Journal:  EMBO J       Date:  1995-09-15       Impact factor: 11.598

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