Abstract

GRANT=6967773;P01HL Gene therapy of sickle cell disease requires gene transfer vectors that confer table, regulated, lineage-specific expression of the gamma-globin gene at relatively high levels without the risk of cellular transformation or tumorigenesis. Our proposal to achieve this is based on two recent findings: I) adenovirus (Ad) vectors containing the Ad serotype 35 fibers (Ad5/35) particularly subsets with potential stem cell capacity and ii) incorporation of AAV ITRs into Ad vectors devoid of all viral genes (Ad.AAV) mediates efficient random vector integration and allows for stable gene transfer into human hematopoietic stem cells. To achieve adequate globin expression, we will produce helper-dependent Ad5/35 containing the 26 kb beta-globin LCR (5?HS1 to 5?HS5, beta-globin promoter, 3 HS1); whereby the LCR cassette is flanked by AAV ITRs (Ad,AAV-LCR).
In Specific Aim 1, vector production will be optimized with a recently constructed Ad.AAV-LCR vector expressing the GFP gene under the control of the beta-promoter/LCR. To minimize the risk of tumorigenesis, we will further modify Ad.AAV-LCR vectors to allow for selection against vector integration into active genes and to increase the frequency of site-specific integration by transient co-expression of AAV Rep78.
In Specific Aim 2, we will study the persistence of GFP expression and the integration pattern of our vectors in clones of transduced erythroleukemic cells.
In Specific Aim 3, expression studies and monitoring of integration sites will be performed with colonies of transduced CD34+ cells grown in semisolid cultures, followed by studies in NOD-SCID mice. In an attempt to assess vector-induced tumorigenesis, we will compare the expression profiles of the pool of transduced long-term culture initiating cells and NOD-SCID mice. In an attempt to assess vector-induced tumorigenesis, we will compare the expression profiles of the pool of transduced long-term culture initiating cells and NOD-SCID repopulating cells with that of mock-infected cells using DNA arrays. Finally, if we confirm safety and efficacy with our new vector, in Specific Aim 4, we will construct gamma-globin expressing Ad.AAV-LCR vectors and perform transduction studies in CD34+ cells derived from healthy donors and patients with sickle cell disease. Gamma-globin expression will be analyzed in progenitor assays.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Program Projects (P01)
Project #
5P01HL053750-13
Application #
7275414
Study Section
Heart, Lung, and Blood Initial Review Group (HLBP)
Project Start
Project End
Budget Start
2006-09-01
Budget End
2007-08-31
Support Year
13
Fiscal Year
2006
Total Cost
$277,184
Indirect Cost

  Institution

Name
University of Washington
Department
Type
DUNS #
605799469
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Constantinou, Varnavas C; Bouinta, Asimina; Karponi, Garyfalia et al. (2017) Poor stem cell harvest may not always be related to poor mobilization: lessons gained from a mobilization study in patients with ?-thalassemia major. Transfusion 57:1031-1039
Gori, Jennifer L; Butler, Jason M; Kunar, Balvir et al. (2017) Endothelial Cells Promote Expansion of Long-Term Engrafting Marrow Hematopoietic Stem and Progenitor Cells in Primates. Stem Cells Transl Med 6:864-876
Psatha, Nikoletta; Karponi, Garyfalia; Yannaki, Evangelia (2016) Optimizing autologous cell grafts to improve stem cell gene therapy. Exp Hematol 44:528-39
Li, Li B; Ma, Chao; Awong, Geneve et al. (2016) Silent IL2RG Gene Editing in Human Pluripotent Stem Cells. Mol Ther 24:582-91
Liu, Mingdong; Maurano, Matthew T; Wang, Hao et al. (2015) Genomic discovery of potent chromatin insulators for human gene therapy. Nat Biotechnol 33:198-203
Polak, Paz; Karli?, Rosa; Koren, Amnon et al. (2015) Cell-of-origin chromatin organization shapes the mutational landscape of cancer. Nature 518:360-364
Karponi, Garyfalia; Psatha, Nikoletta; Lederer, Carsten Werner et al. (2015) Plerixafor+G-CSF-mobilized CD34+ cells represent an optimal graft source for thalassemia gene therapy. Blood 126:616-9
Vierstra, Jeff; Reik, Andreas; Chang, Kai-Hsin et al. (2015) Functional footprinting of regulatory DNA. Nat Methods 12:927-30
Qi, Heyuan; Liu, Mingdong; Emery, David W et al. (2015) Functional validation of a constitutive autonomous silencer element. PLoS One 10:e0124588
Watts, Korashon L; Beard, Brian C; Wood, Brent L et al. (2014) No evidence of clonal dominance after transplant of HOXB4-expanded cord blood cells in a nonhuman primate model. Exp Hematol 42:497-504

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