Figure 3.
Figure 3. In vitro colony assays. Sorted CD34+CD1a– and CD34+CD1a+ thymocytes and CD34+ UCB cells were plated in semisolid cultures containing appropriate cytokines to generate myeloid (CFU-GM) or erythroid (BFU-E) colonies. (A) Typical myeloid (left) and erythroid (right) colonies generated from CD34+CD1a– thymocytes. (B) Overview of BFU-E dishes in which 105 CD34+CD1a– or CD34+CD1a+ thymocytes or 103 CD34+ UCB cells were plated. No colonies were detected in dishes with CD34+CD1a+ thymocytes. (C) RQ-PCR analysis of immature TCRD gene rearrangements (Dδ2-Dδ3) in original CD34+CD1a– thymocytes, myeloid and erythroid colonies generated from CD34+CD1a– thymocytes, myeloid colonies generated from CD34+ UCB cells, and CD34+ cells from children's BM sorted into either CD13/33– (mostly B-cell progenitors) and CD13/33+ (myeloid progenitors) fractions. Percentages of rearranged alleles in each sample are shown.

In vitro colony assays. Sorted CD34+CD1a and CD34+CD1a+ thymocytes and CD34+ UCB cells were plated in semisolid cultures containing appropriate cytokines to generate myeloid (CFU-GM) or erythroid (BFU-E) colonies. (A) Typical myeloid (left) and erythroid (right) colonies generated from CD34+CD1a thymocytes. (B) Overview of BFU-E dishes in which 105 CD34+CD1a or CD34+CD1a+ thymocytes or 103 CD34+ UCB cells were plated. No colonies were detected in dishes with CD34+CD1a+ thymocytes. (C) RQ-PCR analysis of immature TCRD gene rearrangements (Dδ2-Dδ3) in original CD34+CD1a thymocytes, myeloid and erythroid colonies generated from CD34+CD1a thymocytes, myeloid colonies generated from CD34+ UCB cells, and CD34+ cells from children's BM sorted into either CD13/33 (mostly B-cell progenitors) and CD13/33+ (myeloid progenitors) fractions. Percentages of rearranged alleles in each sample are shown.

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