Figure 3.
Figure 3. Clonal analysis of secondary transplanted SRCs. (A) Study design for clonal analysis of secondary grafts. 34 indicates CD34+ stem/progenitor cells; M, CD33+ myeloid lineage cells; B, CD19+ B-lymphoid lineage cells; T, CD3+ (spleen) or CD4/CD8 double-positive (thymus) T-lymphoid lineage cells. (B) Relative frequencies of each clone type detected in paired secondary transplanted recipients. Data represent mean ± SD of 3 independent experiments. *P < .01 relative to other type of clones. (C) The proportion of clones detected in CD34+ cells is shown. A total of 43 clones in 3 independent experiments were analyzed. Gray bars represent the clones detected in CD34+ cells. Black bars represent the clones not detected in CD34+ cells. *P < .01 relative to MTB clones found in primary recipients (shown in Figure 1E). (D) The proportion of MTB clones found in CD34+ cells of paired secondary recipients. A total of 27 clones in 3 independent experiments were analyzed. Notation of the left vertical axis: +/+, MTB-MTB clone pairs were detected in CD34+ cells of both secondary recipient pairs; +/–, MTB-MTB clone pairs were detected in the CD34+ cells of 1 of the 2 secondary recipient pairs; and –/–, MTB-MTB clone pairs were not detected in the CD34+ cells of either secondary recipient pairs. (E) Relative clone size of individual clones in each MTB-MTB clone pairs in CD34+ stem cell pool found in paired secondary recipient. The relative clone size of individual clones in 11 MTB-MTB clone pairs detected in CD34+ cells of both secondary recipients was examined by RQ-PCR. The relative clone size of individual clones in each MTB-MTB pair is expressed as the proportion of one clone relative to the other clone. The MTB-MTB clone pairs no. 15-3 and no. 19-7 that was detected in the CD34+ cells of only 1 of the 2 secondary recipient pairs were used as experimental control and demonstrated complete skewing to either one recipient.

Clonal analysis of secondary transplanted SRCs. (A) Study design for clonal analysis of secondary grafts. 34 indicates CD34+ stem/progenitor cells; M, CD33+ myeloid lineage cells; B, CD19+ B-lymphoid lineage cells; T, CD3+ (spleen) or CD4/CD8 double-positive (thymus) T-lymphoid lineage cells. (B) Relative frequencies of each clone type detected in paired secondary transplanted recipients. Data represent mean ± SD of 3 independent experiments. *P < .01 relative to other type of clones. (C) The proportion of clones detected in CD34+ cells is shown. A total of 43 clones in 3 independent experiments were analyzed. Gray bars represent the clones detected in CD34+ cells. Black bars represent the clones not detected in CD34+ cells. *P < .01 relative to MTB clones found in primary recipients (shown in Figure 1E). (D) The proportion of MTB clones found in CD34+ cells of paired secondary recipients. A total of 27 clones in 3 independent experiments were analyzed. Notation of the left vertical axis: +/+, MTB-MTB clone pairs were detected in CD34+ cells of both secondary recipient pairs; +/–, MTB-MTB clone pairs were detected in the CD34+ cells of 1 of the 2 secondary recipient pairs; and –/–, MTB-MTB clone pairs were not detected in the CD34+ cells of either secondary recipient pairs. (E) Relative clone size of individual clones in each MTB-MTB clone pairs in CD34+ stem cell pool found in paired secondary recipient. The relative clone size of individual clones in 11 MTB-MTB clone pairs detected in CD34+ cells of both secondary recipients was examined by RQ-PCR. The relative clone size of individual clones in each MTB-MTB pair is expressed as the proportion of one clone relative to the other clone. The MTB-MTB clone pairs no. 15-3 and no. 19-7 that was detected in the CD34+ cells of only 1 of the 2 secondary recipient pairs were used as experimental control and demonstrated complete skewing to either one recipient.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal