Figure 4
Figure 4. Change in percentage of GFP and GFP transgene insert copy number during prolonged ex vivo culture of transduced human PBSCs. Following transduction of human CD34+ PBSCs with the vectors encoding GFP only, or GFP plus either wt CXCR4 or mutated CXCR4, most cells were transplanted into NOD/SCID mice; for some experiments (n = 4), cells were retained in long-term ex vivo culture. Long-term culture conditions consisted of X-VIVO10 culture medium containing 50 ng/mL hSCF, hTPO, and hFLT3-ligand, and 20 ng/mL hIL3, IL6, G-CSF, and GM-CSF. FACS analysis of GFP expression (lines) or quantitative real-time PCR–based assessment of GFP sequence copy number (bars) was performed at the culture days indicated on the horizontal axis. Percentages of GFP+ cells started out at similar high level and decreased in a parallel fashion for all the groups to about half the value by day 35, consistent with a higher level of transduction of short-term progenitors than transduction of longer-term progenitors (GFP only, ♦; wt CXCR4, •; and mutated CXCR4, ▪). The total GFP copy number per cell for each group is shown to also start out very high and to decrease in parallel more than 3-fold for each of the groups (GFP only, ▪; wt CXCR4, □; and mutated CXCR4, ⊡). The data suggest that as assessed in the long-term culture ex vivo environment, the transduction rates of long-term progenitors are similar in the 3 transduction groups. It is possible that high expression of wt and mutated CXCR4 in short-term progenitors early in culture at the time of transplantation into mice may enhance final long-term engraftment through some “helper” function, even when eventually a much lower percentage of long-term progenitors continues to express transgene.

Change in percentage of GFP and GFP transgene insert copy number during prolonged ex vivo culture of transduced human PBSCs. Following transduction of human CD34+ PBSCs with the vectors encoding GFP only, or GFP plus either wt CXCR4 or mutated CXCR4, most cells were transplanted into NOD/SCID mice; for some experiments (n = 4), cells were retained in long-term ex vivo culture. Long-term culture conditions consisted of X-VIVO10 culture medium containing 50 ng/mL hSCF, hTPO, and hFLT3-ligand, and 20 ng/mL hIL3, IL6, G-CSF, and GM-CSF. FACS analysis of GFP expression (lines) or quantitative real-time PCR–based assessment of GFP sequence copy number (bars) was performed at the culture days indicated on the horizontal axis. Percentages of GFP+ cells started out at similar high level and decreased in a parallel fashion for all the groups to about half the value by day 35, consistent with a higher level of transduction of short-term progenitors than transduction of longer-term progenitors (GFP only, ♦; wt CXCR4, •; and mutated CXCR4, ▪). The total GFP copy number per cell for each group is shown to also start out very high and to decrease in parallel more than 3-fold for each of the groups (GFP only, ▪; wt CXCR4, □; and mutated CXCR4, ⊡). The data suggest that as assessed in the long-term culture ex vivo environment, the transduction rates of long-term progenitors are similar in the 3 transduction groups. It is possible that high expression of wt and mutated CXCR4 in short-term progenitors early in culture at the time of transplantation into mice may enhance final long-term engraftment through some “helper” function, even when eventually a much lower percentage of long-term progenitors continues to express transgene.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal