RRM
2009 Rustbelt RNA Meeting
RRM
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Poster abstracts
Abstract:
T box antiterminator riboswitch regulation is found primarily in Gram-positive bacteria and is a major regulatory mechanism for genes related to amino acid biosynthesis. The 5’ untranslated region of these genes monitor and respond to the charging ratio of cognate tRNA. The ultimate objective of this project is to develop novel RNA-targeted medicinal agents through examination of the structure and function of the RNA and associated ligands. A more specific aim is to find peptides that are capable of binding to the antiterminator element of the Bacillus subtilis tyrS sequence to modulate the tRNA-antiterminator complex critical for the functioning of the T box riboswitch. The antiterminator contains the highly conserved T box sequence and a seven nucleotide bulge, of which the first four nucleotides base pair with the tRNA in the complex. The model antiterminator, AM1A, contains the same T box sequence and seven nucleotide bulge and is used in binding studies with various peptide sequences. The goal is to find peptides that will bind well with the antiterminator and then place the ligand complex in further testing to identify the effect of the binding on the tRNA-antiterminator interaction. Fluorescence spectroscopy was used to determine two trends: first, the relative binding affinities of a small library of peptides to the AM1A and second, the effect of the relative position of the amino acids within the peptide on the relative binding affinity. Optimization of the assay method will be presented.
Keywords: T box, peptide
