Abstract

This proposal will focus on the mechanism of human immunodeficiency virus (HIV) recombination as catalyzed by reverse transcriptase (RT). Recombination during first strand DNA synthesis (synthesis directed by the RNA genome of the retrovirus) is presumed to occur by strand transfer. This process, whereby DNA synthesized on one template (donor) is transferred to another template (acceptor) for additional elongation, occurs twice during the retroviral replication cycle. In addition to these required transfers which occur at the termini of viral templates, other transfers within internal regions of the genome can also occur. An in vitro system designed to examine internal strand transfers will be used to model recombination occurring within internal regions of the donor. Experiments will evaluate the kinetic parameters associated with this process and the influence of RT on specific steps (for example, the dissociation of the nascent DNA from the donor and its association with the acceptor) with the goal of formulating a model for recombination. Strand transfer on specific viral sequences with characteristics that may promote efficient transfer will be examined using a system that can measure the strand transfer efficiency of any region of RNA. The potential effect of base misincorporations on transfer efficiency and the frequency of misincorporation during transfer events will be evaluated. This is particularly relevant given the low fidelity of DNA synthesis by HIV-RT and the fact that misincorporation leads to DNA synthesis pausing which has been proposed to promote transfer. Nucleocapsid protein (NCp) is a nucleic acid binding protein found in the core of the retroviral virion. The properties of this protein suggest that it may influence the DNA synthetic and strand transfer catalysis properties of RT. These possibilities will be evaluated in the above systems. In addition to the studies on recombination, the RNase H cleavage specificity of HIV-RT will be examined, The experiments will use substrates that mimic structures present during replication to determine how the RT recognizes and cleaves such structures and to evaluate the spacial and topological arrangement of the polymerase and RNase H active sites of the RT. Overall, the studies will offer insight into one of the mechanisms by which retroviruses evolve and escape both drug therapy and the host immune response. An understanding of these processes is important for designing drug therapies or other strategies that target unique RT activities.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
First Independent Research Support & Transition (FIRST) Awards (R29)
Project #
5R29GM051140-02
Application #
2189458
Study Section
AIDS and Related Research Study Section 3 (ARRC)
Project Start
1994-05-01
Project End
1999-04-30
Budget Start
1995-05-01
Budget End
1996-04-30
Support Year
2
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
University of Maryland College Park
Department
Microbiology/Immun/Virology
Type
Schools of Earth Sciences/Natur
DUNS #
City
College Park
State
MD
Country
United States
Zip Code
20742

  Publications

Achuthan, Vasudevan; DeStefano, Jeffrey J (2015) Alternative divalent cations (Zn²?, Co²?, and Mn²?) are not mutagenic at conditions optimal for HIV-1 reverse transcriptase activity. BMC Biochem 16:12
Achuthan, Vasudevan; Keith, Brian J; Connolly, Bernard A et al. (2014) Human immunodeficiency virus reverse transcriptase displays dramatically higher fidelity under physiological magnesium conditions in vitro. J Virol 88:8514-27
Lieberman, Ori J; DeStefano, Jeffrey J; Lee, Vincent T (2013) Detection of cyclic diguanylate G-octaplex assembly and interaction with proteins. PLoS One 8:e53689
Nair, Gauri R; Dash, Chandravanu; Le Grice, Stuart F J et al. (2012) Viral reverse transcriptases show selective high affinity binding to DNA-DNA primer-templates that resemble the polypurine tract. PLoS One 7:e41712
Lai, Yi-Tak; DeStefano, Jeffrey J (2012) DNA aptamers to human immunodeficiency virus reverse transcriptase selected by a primer-free SELEX method: characterization and comparison with other aptamers. Nucleic Acid Ther 22:162-76
Fenstermacher, Katherine J; DeStefano, Jeffrey J (2011) Mechanism of HIV reverse transcriptase inhibition by zinc: formation of a highly stable enzyme-(primer-template) complex with profoundly diminished catalytic activity. J Biol Chem 286:40433-42
Lai, Yi-Tak; DeStefano, Jeffrey J (2011) A primer-free method that selects high-affinity single-stranded DNA aptamers using thermostable RNA ligase. Anal Biochem 414:246-53
Olimpo, Jeffrey T; DeStefano, Jeffrey J (2010) Duplex structural differences and not 2'-hydroxyls explain the more stable binding of HIV-reverse transcriptase to RNA-DNA versus DNA-DNA. Nucleic Acids Res 38:4426-35
Gangaramani, Divya R; Eden, Elizabeth L; Shah, Manthan et al. (2010) The twenty-nine amino acid C-terminal cytoplasmic domain of poliovirus 3AB is critical for nucleic acid chaperone activity. RNA Biol 7:820-9
DeStefano, Jeffrey J (2010) Effect of reaction conditions and 3AB on the mutation rate of poliovirus RNA-dependent RNA polymerase in a alpha-complementation assay. Virus Res 147:53-9