Figure 1
Figure 1. Retroviral transduction after baCD3/CD28 activation and culture with γ-chain cytokines results in central memory TK+ lymphocytes. (A) PBMCs were stimulated with either baCD3/CD28+ IL-7/IL-15 (■), baCD3/CD28+ IL-7 (), baCD3/CD28+ IL-2 (), aCD3+ IL-2 (□), or baCD3/CD28 only (▦). At 48 and 72 hours after stimulation, cells were transduced with the cell-free supernatant carrying the retroviral vector SCFMM-3 Mut2. Transduction efficiency was measured by flow cytometry at day 7. Averages plus or minus SD of 9 independent experiments from different donors are shown. **P < .01 versus all other samples. (B) TK+ lymphocytes were cultured until day 21. Cytokines were added every 3 to 4 days. Immune-selected cells were counted with trypan blue exclusion at days 7, 9, 15, and 21. To evaluate and compare TK+ lymphocyte expansion, while avoiding biases related to variable transduction efficiency, cell expansion was calculated according to the following formula: (no. of cells at day X/no. of cells at day 7). baCD3/CD28+ IL-7/IL-15 (◆), baCD3/CD28+ IL-7 (), baCD3/CD28+ IL-2 (), aCD3+ IL-2 (□), or baCD3/CD28 only (black square with dotted line). Median of 3 independent experiments from different donors is shown. *P < .05; **P < .01 versus baCD3/CD28+ IL-7/IL-15. (C) CD4/CD8 ratio was measured on transduced lymphocytes by flow cytometry at day 10. Averages plus or minus SD of 9 independent experiments from 9 independent donors are shown. **P < .01 versus all other samples. (D) Expression of CD45RA and CD62L was assessed on TK+ lymphocytes at day 10 by flow cytometry. Relative distribution plus or minus SD of TNA (CD45RA+CD62L+, ▥), TCM (CD45RA−CD62L+, ▨), TEM (CD45RA−CD62L−, ▩), and TE (CD45RA+CD62L− ▩) lymphocytes on CD3 TK+ lymphocytes are shown. N = 6 or more per group from 10 independent experiments with 10 independent donors. **P < .01, versus all other samples. (E) Expression of CD27 and CD28 was assessed on TK+ lymphocytes at day 10 by flow cytometry. Relative distribution plus or minus SD of CD27+CD28+ (▨), CD27+CD28− (▩), CD27−CD28+ (▥), and CD27−CD28− (▩) cells in CD3 TK+ lymphocytes are indicated. N = 5 or more per group from 9 independent experiments with 9 independent donors. *P < .05; **P < .01, versus aCD3+ IL-2. (F) At day 10, TK+ lymphocytes were stimulated by PMA/ionomycin and analyzed by flow cytometry for IFNγ and IL-2 production. Averages plus or minus SD of IFNγ−IL-2+ (▨), IFNγ+IL-2+ (▩), and IFNγ+IL-2− (▩) cells in CD3 TK+ lymphocytes are indicated. N = 5 per group from 5 independent experiments with 5 independent donors. *P < .05; **P < .01 versus aCD3+ IL-2.

Retroviral transduction after baCD3/CD28 activation and culture with γ-chain cytokines results in central memory TK+ lymphocytes. (A) PBMCs were stimulated with either baCD3/CD28+ IL-7/IL-15 (■), baCD3/CD28+ IL-7 (), baCD3/CD28+ IL-2 (), aCD3+ IL-2 (□), or baCD3/CD28 only (▦). At 48 and 72 hours after stimulation, cells were transduced with the cell-free supernatant carrying the retroviral vector SCFMM-3 Mut2. Transduction efficiency was measured by flow cytometry at day 7. Averages plus or minus SD of 9 independent experiments from different donors are shown. **P < .01 versus all other samples. (B) TK+ lymphocytes were cultured until day 21. Cytokines were added every 3 to 4 days. Immune-selected cells were counted with trypan blue exclusion at days 7, 9, 15, and 21. To evaluate and compare TK+ lymphocyte expansion, while avoiding biases related to variable transduction efficiency, cell expansion was calculated according to the following formula: (no. of cells at day X/no. of cells at day 7). baCD3/CD28+ IL-7/IL-15 (◆), baCD3/CD28+ IL-7 (), baCD3/CD28+ IL-2 (), aCD3+ IL-2 (□), or baCD3/CD28 only (black square with dotted line). Median of 3 independent experiments from different donors is shown. *P < .05; **P < .01 versus baCD3/CD28+ IL-7/IL-15. (C) CD4/CD8 ratio was measured on transduced lymphocytes by flow cytometry at day 10. Averages plus or minus SD of 9 independent experiments from 9 independent donors are shown. **P < .01 versus all other samples. (D) Expression of CD45RA and CD62L was assessed on TK+ lymphocytes at day 10 by flow cytometry. Relative distribution plus or minus SD of TNA (CD45RA+CD62L+, ▥), TCM (CD45RACD62L+, ▨), TEM (CD45RACD62L, ▩), and TE (CD45RA+CD62L ▩) lymphocytes on CD3 TK+ lymphocytes are shown. N = 6 or more per group from 10 independent experiments with 10 independent donors. **P < .01, versus all other samples. (E) Expression of CD27 and CD28 was assessed on TK+ lymphocytes at day 10 by flow cytometry. Relative distribution plus or minus SD of CD27+CD28+ (▨), CD27+CD28 (▩), CD27CD28+ (▥), and CD27CD28 (▩) cells in CD3 TK+ lymphocytes are indicated. N = 5 or more per group from 9 independent experiments with 9 independent donors. *P < .05; **P < .01, versus aCD3+ IL-2. (F) At day 10, TK+ lymphocytes were stimulated by PMA/ionomycin and analyzed by flow cytometry for IFNγ and IL-2 production. Averages plus or minus SD of IFNγIL-2+ (▨), IFNγ+IL-2+ (▩), and IFNγ+IL-2 (▩) cells in CD3 TK+ lymphocytes are indicated. N = 5 per group from 5 independent experiments with 5 independent donors. *P < .05; **P < .01 versus aCD3+ IL-2.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal