Abstract

The primary goal of this project is to determine the molecular structure of a full length HIV-1 integrase, to harness it to elucidate interactions with DNA, and to initiate structure-assisted drug design. The structure will be determined from crystals that derive from a series if mutations introduced in succession with the goal of improving solubility of full length integrase while preserving activity. Initially a low resolution the structure will be determined from current about 0.4 mm sized crystals (space group C2; unit cell dimension a-160A, b=245A, c=302A, and beta=94 degrees. Further mutations will be used to introduce unique labeling sites, for heavy metal isomorphous replacement and anomalous dispersion procedures. Molecular replacement will use the catalytic domains of HIV-1 integrase, ASV integrase, and Mu transposes.
The aim i s to reveal the relative positions of the N-terminal zinc-finger domain, the catalytic domain, and DNA binding C-terminal domain in the apoenzyme complex. Another aim is to improve resolution of diffraction. The ensuring strategy builds on the now routine crystal growth deriving from the intensive mutagenesis, expression, purification, characterization and crystallization efforts in the Pis laboratory. The first crystals provide the key assay, by means of x-ray diffraction, needed for improvement in resolution of diffraction. Screens of future conditions, and further diffraction, needed for improvement in resolution of diffraction. Screens of further conditions, and further mutagenesis will be used. Functional assessment of variants will be carried out in collaboration. Attempts will be made to cocrystalize our soluble integrase construct with already known inhibitors, and inhibitors under development. Cocrystallization of integrase with oligonucleotides will be attempted using a Y-shaped duplex previously constructed to mimic a reaction intermediate, and linear constructs. Further nucleic acid constructs will be designed in collaboration. The size and length of double stranded oligonucleotide constructs will be varied to obtain crystals of a complex suitable for structure determination.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Program Projects (P01)
Project #
5P01GM056531-05
Application #
6496329
Study Section
Project Start
2001-09-01
Project End
2002-08-31
Budget Start
1998-10-01
Budget End
1999-09-30
Support Year
5
Fiscal Year
2001
Total Cost
$159,403
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Type
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Ohol, Yamini M; Goetz, David H; Chan, Kaman et al. (2010) Mycobacterium tuberculosis MycP1 protease plays a dual role in regulation of ESX-1 secretion and virulence. Cell Host Microbe 7:210-20
Lang, P Therese; Brozell, Scott R; Mukherjee, Sudipto et al. (2009) DOCK 6: combining techniques to model RNA-small molecule complexes. RNA 15:1219-30
Lim, Mark D; Craik, Charles S (2009) Using specificity to strategically target proteases. Bioorg Med Chem 17:1094-100
Daugherty, Matthew D; D'Orso, Ivan; Frankel, Alan D (2008) A solution to limited genomic capacity: using adaptable binding surfaces to assemble the functional HIV Rev oligomer on RNA. Mol Cell 31:824-34
Graves, Alan P; Shivakumar, Devleena M; Boyce, Sarah E et al. (2008) Rescoring docking hit lists for model cavity sites: predictions and experimental testing. J Mol Biol 377:914-34
Raorane, Digvijay A; Lim, Mark D; Chen, Fanqing Frank et al. (2008) Quantitative and label-free technique for measuring protease activity and inhibition using a microfluidic cantilever array. Nano Lett 8:2968-74
He, Xin; Alian, Akram; Ortiz de Montellano, Paul R (2007) Inhibition of the Mycobacterium tuberculosis enoyl acyl carrier protein reductase InhA by arylamides. Bioorg Med Chem 15:6649-58
Lazic, Ana; Goetz, David H; Nomura, Anson M et al. (2007) Substrate modulation of enzyme activity in the herpesvirus protease family. J Mol Biol 373:913-23
Mills, Nicholas L; Shelat, Anang A; Guy, R Kiplin (2007) Assay Optimization and Screening of RNA-Protein Interactions by AlphaScreen. J Biomol Screen 12:946-55
Huang, Niu; Jacobson, Matthew P (2007) Physics-based methods for studying protein-ligand interactions. Curr Opin Drug Discov Devel 10:325-31

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