Abstract

The long-term goal of this research is to understand the regulation of eukaryotic RNA synthesis at the molecular level. The general strategy to be employed involves transcription in cell-free systems. It is proposed to extend and improve the existing in vitro approaches in two ways. First, in order to define and characterize the macromolecular complex which is the target of regulatory events, a series of transcription complexes containing DNA template and RNA polymerase II will be prepared. Both newly-initiated and elongating complexes will be studied; in all cases template protection and RNA polymerase configuration and subunit composition will be examined. Studies will also be done to determine the subset of RNA polymerase II subunits involved solely in elongation. Second, in order to more faithfully reproduce in vivo transcription levels and patterns, more physiological templates than the currently-used purified DNAs will be prepared. In this part of the research, we will continue our current studies on reconstituted chromatin templates; we will also prepare chromatin templates from the cell in as close to their native state as possible. Recombinants between genes of interest and bovine papilloma virus will be made and propagated as episomes in mouse cells. Genes in such constructs continue to be properly regulated and may be recovered as minichromosomes. These purified episomes will be used as templates for in vitro RNA synthesis with the intent of demonstrating in vitro transcription levels proportional to the corresponding in vivo levels. Both metal-inducible (metallothione) and developmentally regulaterd (Beta-globin) promoters will be used in the constructs. For those cases in which in vivo transcription patterns can be duplicated, the minichromosomes will be examined for induction-correlated features. These would include: (i) the presence of regulatory proteins bound at the promoter, or at other known regulatory sites (enhancers), and (ii) changes in the configuration of the promoter (absence of nucleosomes, presence of denatured regions, etc.).

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM029487-09
Application #
3277111
Study Section
Molecular Biology Study Section (MBY)
Project Start
1981-07-01
Project End
1992-06-30
Budget Start
1989-07-01
Budget End
1990-06-30
Support Year
9
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
University of Cincinnati
Department
Type
Schools of Medicine
DUNS #
City
Cincinnati
State
OH
Country
United States
Zip Code
45221

  Publications

Luse, Donal S (2013) Promoter clearance by RNA polymerase II. Biochim Biophys Acta 1829:63-8
Luse, Donal S (2012) Rethinking the role of TFIIF in transcript initiation by RNA polymerase II. Transcription 3:156-9
?abart, Pavel; Luse, Donal S (2012) Inactivated RNA polymerase II open complexes can be reactivated with TFIIE. J Biol Chem 287:961-7
Cabart, Pavel; Ujvari, Andrea; Pal, Mahadeb et al. (2011) Transcription factor TFIIF is not required for initiation by RNA polymerase II, but it is essential to stabilize transcription factor TFIIB in early elongation complexes. Proc Natl Acad Sci U S A 108:15786-91
Újvári, Andrea; Pal, Mahadeb; Luse, Donal S (2011) The functions of TFIIF during initiation and transcript elongation are differentially affected by phosphorylation by casein kinase 2. J Biol Chem 286:23160-7
Ujvari, Andrea; Luse, Donal S (2006) RNA emerging from the active site of RNA polymerase II interacts with the Rpb7 subunit. Nat Struct Mol Biol 13:49-54
Pal, Mahadeb; Ponticelli, Alfred S; Luse, Donal S (2005) The role of the transcription bubble and TFIIB in promoter clearance by RNA polymerase II. Mol Cell 19:101-10
Hawryluk, Peter J; Ujvari, Andrea; Luse, Donal S (2004) Characterization of a novel RNA polymerase II arrest site which lacks a weak 3' RNA-DNA hybrid. Nucleic Acids Res 32:1904-16
Ujvari, Andrea; Luse, Donal S (2004) Newly Initiated RNA encounters a factor involved in splicing immediately upon emerging from within RNA polymerase II. J Biol Chem 279:49773-9
Pal, Mahadeb; Luse, Donal S (2003) The initiation-elongation transition: lateral mobility of RNA in RNA polymerase II complexes is greatly reduced at +8/+9 and absent by +23. Proc Natl Acad Sci U S A 100:5700-5

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