Experimental Hematology
Volume 36, Issue 7 , Pages 823-831, July 2008

Tightly regulated gene expression in human hematopoietic stem cells after transduction with helper-dependent Ad5/35 vectors

  • Hongje Wang

      Affiliations

    • Division of Medical Genetics, Department of Medicine, University of Washington, Seattle, Wash., USA
  • ,
  • Hua Cao

      Affiliations

    • Division of Medical Genetics, Department of Medicine, University of Washington, Seattle, Wash., USA
  • ,
  • Martin Wohlfahrt

      Affiliations

    • Fred Hutchinson Cancer Research Center, Seattle, Wash., USA
  • ,
  • Hans-Peter Kiem

      Affiliations

    • Fred Hutchinson Cancer Research Center, Seattle, Wash., USA
  • ,
  • André Lieber

      Affiliations

    • Division of Medical Genetics, Department of Medicine, University of Washington, Seattle, Wash., USA
    • Department of Pathology, University of Washington, Seattle, Wash., USA
    • Corresponding Author InformationOffprint requests to: André Lieber, M.D., Ph.D., Division of Medical Genetics, University of Washington, Box 357720, Seattle, WA 98195

Received 26 September 2007; received in revised form 7 December 2007; accepted 18 January 2008. published online 07 April 2008.

Objective

Inducible and transient expression of transcription factors, growth factors, or mitogenic factors can be used to influence proliferation or differentiation of hematopoietic progenitor/stem cells (HSC). Furthermore, transient expression of proteins with site-specific endonuclease activity, potentially, can support targeted integration of exogenous transgenes into specific sites in the genome, a task that is currently a focus in development of gene therapy vectors.

Materials and Methods

We constructed a set of helper-dependent adenovirus (Ad) vectors with serotype 35 fiber knob domains (HD-Ad5/35), which can efficiently transduce human CD34+ cells, particularly subsets with potential stem cell capacity. These vectors contain Tet-inducible expression systems that were shielded by insulators and transcription stop signals to minimize unspecific interference by transcriptional elements present in viral and stuffer DNA. We compared two vectors, containing a fusion between the Krüppel-associated box (KRAB) domain and the tetracycline repressor (HD-Ad5/35.Tet-1) or an autoregulated rtTA (HD-Ad5/35.Tet-2) for regulated transgene expression in Mo7e cells, a model for HSC, and primary human CD34+ cells.

Results

HD-Ad5/35.Tet-1 conferred lower background expression than HD-Ad5/35.Tet-2, although levels of induced gene expression were higher for HD-Ad5/35.Tet-2. In CD34+ cells, while HD-Ad5/35.Tet-1 allowed for activated gene expression in all transduced cells, induced gene expression from HD-Ad5/35.Tet-2 was restricted to a small subset of CD34+ cells. Importantly, clonogeneic assays and repopulation studies in nonobese diabetic/severe combined immunodeficient mice showed that both HD-Ad5/35.Tet-1 and -2 vectors mediated induced gene expression in primitive hematopoietic cells. These studies also confirmed that transduction of CD34+ cells with HD-Ad5/35 vectors is not associated with cytotoxicity, a problem observed with first-generation Ad5/35 vectors.

Conclusions

Both HD-Ad5/35 vector expression systems confer tightly regulated, transient transgene expression in human HSC.

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PII: S0301-472X(08)00050-7

doi:10.1016/j.exphem.2008.01.014

Experimental Hematology
Volume 36, Issue 7 , Pages 823-831, July 2008