Abstract

The catabolite gene activator protein (CAP) of E. coli is a member of a class of sequence-specific DNA binding proteins that utilize a highly conserved alpha-helix-turn-alpha-helix structural motif to mediate interaction with DNA. This class of sequence-specifc DNA binding proteins has at least 75 members, including the homeo box proteins, which are involved in the regulation of eukaryotic development. Our research project regarding DNA-sequence recognition by CAP is directed at three long-range objectives: (i) identification of the individual amino acid-DNA contacts involved in DNA-sequence recognition by CAP, (ii) investigation of the chemistry and thermodynamics of specificity, and (iii) elucidation of rules--a """"""""coded""""""""--relating the amino acid sequence of the helix-turn-helix motif of a DNA binding protein to the nucleotide sequence of the specific DNA site. The experiments in this proposal have as specific aims the investigation of two examples of DNA-sequence recognition mediated through protein-base pair contacts, and the investigation of two examples of DNA-sequence recognition mediated through protein-phosphate contacts. DNA-sequence recognition mediated through protein-specific DNA binding protein. The approach to be employed emphasizes the use of single amino acid substitutions to identify and quantify important amino acid- DNA interactions. Single amino acid substitutions will be introduced into CAP using site-directed mutagenesis. The DNA- sequence recognition properties of the substituted CAP variants then will be investigated in in vitro binding assays using as ligands the consensus DNA site and a battery of non-consensus and chemically modified DNA sites; free energies of binding and free energies of specificity will be determine from the equilibrium binding data. The experimentally measured effects of the amino acid substitutions on the binding and specificity free energies will be interpreted in two fashions: (i) qualitatively, using computer-assisted molecule graphics and the known three- dimensional structures of CAP and B-DNA; and (ii) quantitatively, using molecular energy calculations. The results to be obtained will be relevant to understanding protein-nucleic acid interaction and its role in the regulation of gene expression. In addition, the results to be obtained will be relevant to understanding other examples of protein-ligand interaction, including: enzyme-substrate, receptor-hormone, and receptor-drug interactions.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM041376-02
Application #
3299546
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1988-12-01
Project End
1992-11-30
Budget Start
1989-12-01
Budget End
1990-11-30
Support Year
2
Fiscal Year
1990
Total Cost
Indirect Cost

  Institution

Name
Rutgers University
Department
Type
Organized Research Units
DUNS #
038633251
City
New Brunswick
State
NJ
Country
United States
Zip Code
08901

  Publications

Gabizon, Ronen; Lee, Antony; Vahedian-Movahed, Hanif et al. (2018) Pause sequences facilitate entry into long-lived paused states by reducing RNA polymerase transcription rates. Nat Commun 9:2930
Vvedenskaya, Irina O; Bird, Jeremy G; Zhang, Yuanchao et al. (2018) CapZyme-Seq Comprehensively Defines Promoter-Sequence Determinants for RNA 5' Capping with NAD. Mol Cell 70:553-564.e9
Lin, Wei; Das, Kalyan; Degen, David et al. (2018) Structural Basis of Transcription Inhibition by Fidaxomicin (Lipiarmycin A3). Mol Cell 70:60-71.e15
Sosio, Margherita; Gaspari, Eleonora; Iorio, Marianna et al. (2018) Analysis of the Pseudouridimycin Biosynthetic Pathway Provides Insights into the Formation of C-nucleoside Antibiotics. Cell Chem Biol 25:540-549.e4
Maffioli, Sonia I; Sosio, Margherita; Ebright, Richard H et al. (2018) Discovery, properties, and biosynthesis of pseudouridimycin, an antibacterial nucleoside-analog inhibitor of bacterial RNA polymerase. J Ind Microbiol Biotechnol :
Walker, Scott S; Degen, David; Nickbarg, Elliott et al. (2017) Affinity Selection-Mass Spectrometry Identifies a Novel Antibacterial RNA Polymerase Inhibitor. ACS Chem Biol 12:1346-1352
Maffioli, Sonia I; Zhang, Yu; Degen, David et al. (2017) Antibacterial Nucleoside-Analog Inhibitor of Bacterial RNA Polymerase. Cell 169:1240-1248.e23
Lin, Wei; Mandal, Soma; Degen, David et al. (2017) Structural Basis of Mycobacterium tuberculosis Transcription and Transcription Inhibition. Mol Cell 66:169-179.e8
Yu, Libing; Winkelman, Jared T; Pukhrambam, Chirangini et al. (2017) The mechanism of variability in transcription start site selection. Elife 6:
Bird, Jeremy G; Nickels, Bryce E; Ebright, Richard H (2017) RNA Capping by Transcription Initiation with Non-canonical Initiating Nucleotides (NCINs): Determination of Relative Efficiencies of Transcription Initiation with NCINs and NTPs. Bio Protoc 7:

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