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Blood, 15 January 2002, Vol. 99, No. 2, pp. 488-498

HEMATOPOIESIS

Differential gene expression profiling of adult murine hematopoietic stem cells

In-Kyung Park, Yaqin He, Fangming Lin, Ole D. Laerum, Qiang Tian, Roger Bumgarner, Christopher A. Klug, Kaijun Li, Christian Kuhr, Michelle J. Doyle, Tao Xie, Michèl Schummer, Yu Sun, Adam Goldsmith, Michael F. Clarke, Irving L. Weissman, Leroy Hood, and Linheng Li

From the University of Michigan, Department of Internal Medicine, Ann Arbor; the Stowers Institute for Medical Research, Kansas City, MO; the University of Washington, Departments of Pediatrics, Microbiology, Surgery, and Molecular Biotechnology, Seattle; the University of Bergen, Department of Pathology, Norway; the University of Alabama at Birmingham, Department of Microbiology; Stanford University, Department of Pathology, Stanford, CA; and the Institute for Systems Biology, Seattle, WA.

Hematopoietic stem cells (HSCs) have self-renewal capacity and multilineage developmental potentials. The molecular mechanisms that control the self-renewal of HSCs are still largely unknown. Here, a systematic approach using bioinformatics and array hybridization techniques to analyze gene expression profiles in HSCs is described. To enrich mRNAs predominantly expressed in uncommitted cell lineages, 54 000 cDNA clones generated from a highly enriched population of HSCs and a mixed population of stem and early multipotent progenitor (MPP) cells were arrayed on nylon membranes (macroarray or high-density array), and subtracted with cDNA probes derived from mature lineage cells including spleen, thymus, and bone marrow. Five thousand cDNA clones with very low hybridization signals were selected for sequencing and further analysis using microarrays on glass slides. Two populations of cells, HSCs and MPP cells, were compared for differential gene expression using microarray analysis. HSCs have the ability to self-renew, while MPP cells have lost the capacity for self-renewal. A large number of genes that were differentially expressed by enriched populations of HSCs and MPP cells were identified. These included transcription factors, signaling molecules, and previously unknown genes.

© 2002 by The American Society of Hematology.
 

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