Abstract

Current approaches to transfer genes in vivo employ either recombinant viral vectors or non-viral delivery systems. We are engaged in studying the molecular biology of the human parvovirus adeno-associated virus (AAV) with the intent to using this virus as a platform for developing a novel, safe, and efficient delivery system for human gene therapy. Our research pioneered the use of? recombinant AAV (rAAV) as a gene delivery system for central nervous system, and muscle cells demonstrating vector expression for over 1.5 years without immune consequences or vector toxicity. While promising, these studies uncovered rate limiting steps involved in AAV vector transduction; namely receptor mediated entry, and conversion of singled-stranded viral genomes to double-stranded expressing templates (i.e. second-strand synthesis). In addition to this rate-limiting step, the finite packaging capacity of this virus (4.5kb) has restricted the use of this vector to small genes or cDNAs. To advance the prospects of efficient AAV gene delivery, vectors sufficient to carry larger genes must be developed. In addition, virions that specifically and efficiently target defined cell types will be required for clinical application. The focus of this grant will be to address these issues. Three approaches will be analyzed in this proposal to overcome AAV?s problem of viral entry, inefficient second-strand synthesis, and packaging constraints. We have generated exciting new mouse data supporting differential infectivity in type I vs. type II muscle using traditional AAV type II vectors, as well as increased transduction when using other AAV serotype specific vectors. These results emphasize the importance of receptor mediated AAV entry. Mapping and characterization of other AAV serotype capsid domains required for entry will be explored to facilitate more infectious vectors. AAV type II as well as serotype specific vectors 1-5 will be tested in the Chapel Hill canine model for efficient FIX gene delivery in an effort to extend current mouse studies in a large animal model. We have now developed a method for generating AAV vectors carrying duplex viral genomes. These reagents will be characterized for efficient transgene expression after vector delivery in an effort to study rate-limiting steps involved in second-strand synthesis and vector gene expression in vivo. Finally, efforts to engineer vectors that carry twice the packaging capacity of wild type AAV will be explored by using split gene vectors that rely on hetero-dimer concatemers after vector infection. The long term objective is to develop novel delivery systems that exploit the advantages of AAV viral infectivity without the disadvantages of inefficient viral entry, rate limiting steps involved in second-strand synthesis, or packaging constraints.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Program Projects (P01)
Project #
1P01HL066973-01A1
Application #
6533325
Study Section
Heart, Lung, and Blood Program Project Review Committee (HLBP)
Project Start
2001-09-30
Project End
2006-07-31
Budget Start
Budget End
Support Year
1
Fiscal Year
2001
Total Cost
Indirect Cost

  Institution

Name
University of North Carolina Chapel Hill
Department
Type
DUNS #
078861598
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599

  Publications

Monahan, Paul E; Sun, Junjiang; Gui, Tong et al. (2015) Employing a gain-of-function factor IX variant R338L to advance the efficacy and safety of hemophilia B human gene therapy: preclinical evaluation supporting an ongoing adeno-associated virus clinical trial. Hum Gene Ther 26:69-81
Monahan, P E (2015) Gene therapy in an era of emerging treatment options for hemophilia B. J Thromb Haemost 13 Suppl 1:S151-60
Piacentino 3rd, Valentino; Milano, Carmelo A; Bolanos, Michael et al. (2012) X-linked inhibitor of apoptosis protein-mediated attenuation of apoptosis, using a novel cardiac-enhanced adeno-associated viral vector. Hum Gene Ther 23:635-46
Kantor, Boris; Bayer, Matthew; Ma, Hong et al. (2011) Notable reduction in illegitimate integration mediated by a PPT-deleted, nonintegrating lentiviral vector. Mol Ther 19:547-56
Cockrell, Adam S; van Praag, Henriette; Santistevan, Nicholas et al. (2011) The HIV-1 Rev/RRE system is required for HIV-1 5' UTR cis elements to augment encapsidation of heterologous RNA into HIV-1 viral particles. Retrovirology 8:51
Monahan, Paul E; Lothrop, Clinton D; Sun, Junjiang et al. (2010) Proteasome inhibitors enhance gene delivery by AAV virus vectors expressing large genomes in hemophilia mouse and dog models: a strategy for broad clinical application. Mol Ther 18:1907-16
Li, C; Hirsch, M; Carter, P et al. (2009) A small regulatory element from chromosome 19 enhances liver-specific gene expression. Gene Ther 16:43-51
Gui, T; Reheman, A; Ni, H et al. (2009) Abnormal hemostasis in a knock-in mouse carrying a variant of factor IX with impaired binding to collagen type IV. J Thromb Haemost 7:1843-51
Li, Chengwen; Goudy, Kevin; Hirsch, Matt et al. (2009) Cellular immune response to cryptic epitopes during therapeutic gene transfer. Proc Natl Acad Sci U S A 106:10770-4
Kantor, Boris; Ma, Hong; Webster-Cyriaque, Jennifer et al. (2009) Epigenetic activation of unintegrated HIV-1 genomes by gut-associated short chain fatty acids and its implications for HIV infection. Proc Natl Acad Sci U S A 106:18786-91

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