Abstract

Hematopoietic stem cells (HSC) possess the ability to self-renew, differentiate, and produce massive numbers of blood cells of all lineages. If the molecular mechanisms governing the decision to expand vs. commit to differentiation could be fully understood, the knowledge could be applied to expand stem cells ex-vivo and to do successful gene therapy using retroviral vectors. Currently, all culture procedures lead to a progressive loss of pluripotent stem cells, so engineered HSC populations cannot yet be returned to an ablated donor with the confidence that they will sustain long-term multilineage blood cell production. The proposed studies will define culture conditions that can be used to expand primitive progenitors without differentiation. The long-term xenograft system with clonal marking is crucial in these studies because it allows identification of individual stem cells that have cycled during the culture period (identified by their ability to accept a retroviral vector), and have retained the ability to produce both lymphoid and myeloid progeny. They have used this system to show that human stem cells lose the capacity to sustain long-term engraftment if cultured for 72 hours without binding to fibronectin (FN). They hypothesize that engagement of the integrins 24^D1 to FN maintains the primitive phenotype of HSC by sustained activation and nuclear localization of MAPK proteins, resulting in phosphorylation of GATA-2, induction of c-ets-1 and maintenance of expression of c-myb. In suspension, MAPK will remain in the cytoplasm, c-ets-1 will not be induced, and c-myb levels will drop, causing a loss of expression of CD34, flt3 and c-kit. They will verify their hypotheses at the molecular level while determining the best conditions to induce HSC expansion. They predict that culture on FN with stimulatory cytokines, neutralization of TGF^D1, and reduction in levels of the cyclin-dependent kinase inhibitors (CDKI) p27kip1 and p15INK4 will cause division of HSC without induction of pathways of differentiation. They will measure the molecular and cellular effects of these conditions on progenitors (CD34+, colony-forming cells, and B cell precursors) and long-lived HSC (CD34+38-, extended long-term culture initiation cells (e-LTCIC), (e-LTCIC), and immune deficient mouse repopulating cells). Expansion of stem cells will be measured as an increase in the number of transduced e-LTCIC bearing the same clonal integration site, assessed by single colony inverse PCR, and increased number of T cells and myeloid progeny bearing the same proviral integration site following long-term engraftment in bnx mice, indicating that cones of both lineages arose from the same stem cell. The results of the proposed studies will define in vitro culture conditions which induce stem cell division without forcing lineage commitment during retroviral-mediated transduction or ex-vivo stem cell expansion, and will give insight into the molecular changes that precede lineage commitment.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK053041-03
Application #
6177710
Study Section
Hematology Subcommittee 2 (HEM)
Program Officer
Badman, David G
Project Start
1998-06-01
Project End
2002-05-31
Budget Start
2000-06-01
Budget End
2001-05-31
Support Year
3
Fiscal Year
2000
Total Cost
$182,791
Indirect Cost

  Institution

Name
Children's Hospital of Los Angeles
Department
Type
DUNS #
094878337
City
Los Angeles
State
CA
Country
United States
Zip Code
90027

  Publications

Feng, Jun-Feng; Liu, Jing; Zhang, Lei et al. (2017) Electrical Guidance of Human Stem Cells in the Rat Brain. Stem Cell Reports 9:177-189
Kambal, Amal; Mitchell, Gaela; Cary, Whitney et al. (2011) Generation of HIV-1 resistant and functional macrophages from hematopoietic stem cell-derived induced pluripotent stem cells. Mol Ther 19:584-93
Gruenloh, William; Kambal, Amal; Sondergaard, Claus et al. (2011) Characterization and in vivo testing of mesenchymal stem cells derived from human embryonic stem cells. Tissue Eng Part A 17:1517-25
Fierro, Fernando A; Kalomoiris, Stefanos; Sondergaard, Claus S et al. (2011) Effects on proliferation and differentiation of multipotent bone marrow stromal cells engineered to express growth factors for combined cell and gene therapy. Stem Cells 29:1727-37
Rosova, Ivana; Link, Daniel; Nolta, Jan A (2010) shRNA-mediated decreases in c-Met levels affect the differentiation potential of human mesenchymal stem cells and reduce their capacity for tissue repair. Tissue Eng Part A 16:2627-39
Sondergaard, Claus S; Hess, David A; Maxwell, Dustin J et al. (2010) Human cord blood progenitors with high aldehyde dehydrogenase activity improve vascular density in a model of acute myocardial infarction. J Transl Med 8:24
Meyerrose, Todd; Olson, Scott; Pontow, Suzanne et al. (2010) Mesenchymal stem cells for the sustained in vivo delivery of bioactive factors. Adv Drug Deliv Rev 62:1167-74
Anderson, Joseph S; Walker, Jon; Nolta, Jan A et al. (2009) Specific transduction of HIV-susceptible cells for CCR5 knockdown and resistance to HIV infection: a novel method for targeted gene therapy and intracellular immunization. J Acquir Immune Defic Syndr 52:152-61
Anderson, Joseph S; Javien, John; Nolta, Jan A et al. (2009) Preintegration HIV-1 inhibition by a combination lentiviral vector containing a chimeric TRIM5 alpha protein, a CCR5 shRNA, and a TAR decoy. Mol Ther 17:2103-14
Zhou, Ping; Wirthlin, Louisa; McGee, Jeannine et al. (2009) Contribution of human hematopoietic stem cells to liver repair. Semin Immunopathol 31:411-9

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