Fig. 5.
Fig. 5. Maintenance of NGFR transgene expression in CAFC progeny. (A) Sorted NGFR-expressing, CD34+Lin− cells transduced with either the LINGFR (LIN, NGFR+) or MINGFR (MIN, GFR+) vectors, or the sorted CD34+Lin− cells lacking NGFR expression at day 2 posttransduction with LINGFR (LIN, NGFR−) or MINGFR (MIN, NGFR−) vectors (see Fig 3) were plated on SyS-1 stromal cell monolayers. Two-fold serial dilution of 100 CD34+Lin− input cells were seeded per well and examined for cobblestone area (CA) formation weekly up to 6 weeks. The number of wells lacking any CA at week 5 were plotted as a function of numbers of sorted cells, respectively. The frequencies of CAFC were estimated based on Poisson distribution and the results are indicated. (B) NGFR transgene expression in B cells formed at week 6 of CAFC assays. CD19+ B cells (in addition to CD14+and CD15+ myeloid cells) were generated from sorted CD34+Lin−NGFR+ cells in the presence of SyS-1 stromal cells as shown by the presence of the CD19 marker. Among CD19+ B cells, approximately 14% and 50% of the progeny cells derived from LINGFR-transduced (LINGFR+) and MINGFR-transduced (MINGFR+) CD34+Lin−NGFR+ cells, respectively, expressed the NGFR transgene at the end of CAFC assays.

Maintenance of NGFR transgene expression in CAFC progeny. (A) Sorted NGFR-expressing, CD34+Lin cells transduced with either the LINGFR (LIN, NGFR+) or MINGFR (MIN, GFR+) vectors, or the sorted CD34+Lin cells lacking NGFR expression at day 2 posttransduction with LINGFR (LIN, NGFR) or MINGFR (MIN, NGFR) vectors (see Fig 3) were plated on SyS-1 stromal cell monolayers. Two-fold serial dilution of 100 CD34+Lin input cells were seeded per well and examined for cobblestone area (CA) formation weekly up to 6 weeks. The number of wells lacking any CA at week 5 were plotted as a function of numbers of sorted cells, respectively. The frequencies of CAFC were estimated based on Poisson distribution and the results are indicated. (B) NGFR transgene expression in B cells formed at week 6 of CAFC assays. CD19+ B cells (in addition to CD14+and CD15+ myeloid cells) were generated from sorted CD34+LinNGFR+ cells in the presence of SyS-1 stromal cells as shown by the presence of the CD19 marker. Among CD19+ B cells, approximately 14% and 50% of the progeny cells derived from LINGFR-transduced (LINGFR+) and MINGFR-transduced (MINGFR+) CD34+LinNGFR+ cells, respectively, expressed the NGFR transgene at the end of CAFC assays.

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