Abstract

Many important cellular processes are mediated by RNA molecules, and many of the pathways for regulating gene expression involve specific protein - RNA interactions. Virtually all cellular RNAs interact with proteins, and it is not known how proteins recognize specific RNA sites or how they might promote the specific functions of an RNA. The initial goal of the work in this project was to define a few representative, well-behaved systems for which it is feasible, in the long term, to understand 1) how a protein recognizes and modifies the RNA structure, and 2) how the protein - RNA complex accomplishes a specific biological function. Two sets of interactions which illustrate very different aspects of protein RNA recognition, have been defined. In one, ribosomal protein S4 organizes a large and complex region of the 16S rRNA to initiate ribosome assembly; the same protein also binds to its own mRNA as a translational repressor. In the other system, a small, highly conserved rRNA fragment binds the ribosomal protein L11 and a family of peptide antibiotics; both protein and antibiotic binding have specific effects on the GTPase activity of intact ribosomes. The way in which these ligands perturb the RNA structure is thus relevant to ribosome function. By measuring protein or antibiotic affinity for RNAs containing deletions and base changes, the RNA sequences and secondary structures necessary for protein recognition and biological function are being systematically determined. Selection experiments in which about 10(12) RNA sequence variants can be screened for protein recognition are being used to detect additional secondary and tertiary structures. In addition, there is evidence for each of the RNAs under study that the protein perturbs transitions between alternate RNA conformations. The thermodynamics of conformational transitions in these RNAs will be examined, and the effects of protein or antibiotic binding on the transitions determined. 1H and 31P NMR experiments will be carried out on one of the smaller RNAs to detect and locate tertiary structure. The protein binding this RNA, L11, is being overexpressed from a thermophile for NMR studies of its folding. Although these studies will be carried out using fragments of ribosomal or messenger RNA, in each case the physical properties of the fragment RNA - protein complex can be related to the in vivo function of the intact ribosome or messenger. These studies will ultimately be essential for understanding the mechanism of translational repression and the role of proteins in ribosomes, and will also contribute to our general knowledge of strategies used by protein - RNA complexes to carry out specific biological tasks.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM029048-14
Application #
2175370
Study Section
Physical Biochemistry Study Section (PB)
Project Start
1981-04-01
Project End
1996-03-31
Budget Start
1994-04-01
Budget End
1995-03-31
Support Year
14
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
Johns Hopkins University
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
045911138
City
Baltimore
State
MD
Country
United States
Zip Code
21218

  Publications

Bausch, Sarae L; Poliakova, Ekaterina; Draper, David E (2005) Interactions of the N-terminal domain of ribosomal protein L11 with thiostrepton and rRNA. J Biol Chem 280:29956-63
Maeder, Corina; Draper, David E (2005) A small protein unique to bacteria organizes rRNA tertiary structure over an extensive region of the 50 S ribosomal subunit. J Mol Biol 354:436-46
Conn, Graeme L; Gittis, Apostolos G; Lattman, Eaton E et al. (2002) A compact RNA tertiary structure contains a buried backbone-K+ complex. J Mol Biol 318:963-73
Shiman, R; Draper, D E (2000) Stabilization of RNA tertiary structure by monovalent cations. J Mol Biol 302:79-91
GuhaThakurta, D; Draper, D E (1999) Protein-RNA sequence covariation in a ribosomal protein-rRNA complex. Biochemistry 38:3633-40
Conn, G L; Gutell, R R; Draper, D E (1998) A functional ribosomal RNA tertiary structure involves a base triple interaction. Biochemistry 37:11980-8
Rogers, M J; Bukhman, Y V; McCutchan, T F et al. (1997) Interaction of thiostrepton with an RNA fragment derived from the plastid-encoded ribosomal RNA of the malaria parasite. RNA 3:815-20
Sapag, A; Draper, D E (1997) In vitro evolution used to define a protein recognition site within a large RNA domain. Bioorg Med Chem 5:1097-105
Gluick, T C; Gerstner, R B; Draper, D E (1997) Effects of Mg2+, K+, and H+ on an equilibrium between alternative conformations of an RNA pseudoknot. J Mol Biol 270:451-63
Draper, D E (1996) Strategies for RNA folding. Trends Biochem Sci 21:145-9

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