Fig. 3.
Fig. 3. Expression of gp91phox in cultured X-CGD CD34+PBSCs under optimum conditions for ex vivo transduction with lentivector or oncoretrovirus vector. / Shown is the percentage of 17-day cultured CD34+PBSCs expressing gp91phox comparing nontransduced normal CD34+PBSCs (open bar) with X-CGD CD34+PBSCs that had been subjected to 3 daily 7-hour transductions under growth-stimulating conditions (5 cytokines) using either 3rd-generation SIN lentivector–gp91phox (dotted bar) or MFGS–gp91phox (hatched bar). Cultured CD34+PBSCs were labeled with FITC-conjugated anti-gp91phox and analyzed by flow cytometry, and the data were expressed as the percentage of cells that exhibit an expression of gp91phox that is higher than the 95thpercentile of isotype antibody control. By this criterion nontransduced X-CGD CD34+PBSCs do not give rise to any cells that are positive for the expression of gp91phox (not shown). Normal control CD34+PBSCs differentiating in culture first gave rise to differentiated myeloid cells that expressed native gp91phox by approximately day 8 of culture, and this increased to a steady state maximum by approximately day 15, which, in the example shown at day 17 of culture, demonstrated approximately 24% of cells positive for the expression of gp91phox (open bar). Results are representative of 2 experiments.

Expression of gp91phox in cultured X-CGD CD34+PBSCs under optimum conditions for ex vivo transduction with lentivector or oncoretrovirus vector.

Shown is the percentage of 17-day cultured CD34+PBSCs expressing gp91phox comparing nontransduced normal CD34+PBSCs (open bar) with X-CGD CD34+PBSCs that had been subjected to 3 daily 7-hour transductions under growth-stimulating conditions (5 cytokines) using either 3rd-generation SIN lentivector–gp91phox (dotted bar) or MFGS–gp91phox (hatched bar). Cultured CD34+PBSCs were labeled with FITC-conjugated anti-gp91phox and analyzed by flow cytometry, and the data were expressed as the percentage of cells that exhibit an expression of gp91phox that is higher than the 95thpercentile of isotype antibody control. By this criterion nontransduced X-CGD CD34+PBSCs do not give rise to any cells that are positive for the expression of gp91phox (not shown). Normal control CD34+PBSCs differentiating in culture first gave rise to differentiated myeloid cells that expressed native gp91phox by approximately day 8 of culture, and this increased to a steady state maximum by approximately day 15, which, in the example shown at day 17 of culture, demonstrated approximately 24% of cells positive for the expression of gp91phox (open bar). Results are representative of 2 experiments.

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