![Fig. 5. The TRIP vector efficiently transduces NOD/SCID mice long-term reconstituting human cells. / (A) Phenotype of cells harvested from the BM of NOD/SCID mice grafted 15 weeks earlier with 7 × 104CD34+ CB cells transduced with the TRIP vector. At that time, human CD34+ cells were isolated by immunomagnetic selection. CD34+CD38− primitive cells were further sorted on a FACS Vantage. (B) Phenotype of cells differentiated from 104 CD34+CD38− cells, purified from reconstituted mice, following bulk culture in lymphomyeloid conditions. rhEPO was added to the bulk culture to allow terminal erythroid differentiation (glycophorin A [GPA+] cells). (C) The experiment was performed as described in panel B, except that the cells were cultured at 1 cell per well in the absence of rhEPO. Progeny of 39 of 120 cultures proliferated sufficiently to be phenotyped by FACS and were assessed 2 to 3 weeks later using flow cytometry, as illustrated in Figure 4B. Eight of 39 (20%) clones produced CD19+ B, CD56+ NK, and CD11b+ myeloid cells defining multipotential progenitors. Shown in panel C is a representative analysis of the progeny of an input multipotent progenitor.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/96/13/10.1182_blood.v96.13.4103/5/h82400496005.jpeg?Expires=1723201962&Signature=tX-szlNSoTmaKv32bm9OyxJDefH5yYauKznb9xN18h6Ky-sPzX59Y2zenwOGGqzt3~~XHQSEOxo2s71~sIIToWUpJhseZ-SOPzSegeYPHhXKoFmfJZEfWVtmaVOlQ6p39iv-hD~KQK6IYKFCLrTyOGvb02lSJM6ZHTPMYpg6SfITEoFyQ3dSz4t-PjHTy3BOdjQ03~LCsvUlThmaISWARG9WKpzDapC~4UkTS-3YhlNCVKtQzcOu2KLD8Wyr4zTolTzk30DmSOJ1-Stw9DrfoXkbAUCcODLNXHHEvnGgHzco8QUonnSSImLvIAf9dbZ1OeEJGeYHESLYpyvmWE674w__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
The TRIP vector efficiently transduces NOD/SCID mice long-term reconstituting human cells.
(A) Phenotype of cells harvested from the BM of NOD/SCID mice grafted 15 weeks earlier with 7 × 104CD34+ CB cells transduced with the TRIP vector. At that time, human CD34+ cells were isolated by immunomagnetic selection. CD34+CD38− primitive cells were further sorted on a FACS Vantage. (B) Phenotype of cells differentiated from 104 CD34+CD38− cells, purified from reconstituted mice, following bulk culture in lymphomyeloid conditions. rhEPO was added to the bulk culture to allow terminal erythroid differentiation (glycophorin A [GPA+] cells). (C) The experiment was performed as described in panel B, except that the cells were cultured at 1 cell per well in the absence of rhEPO. Progeny of 39 of 120 cultures proliferated sufficiently to be phenotyped by FACS and were assessed 2 to 3 weeks later using flow cytometry, as illustrated in Figure 4B. Eight of 39 (20%) clones produced CD19+ B, CD56+ NK, and CD11b+ myeloid cells defining multipotential progenitors. Shown in panel C is a representative analysis of the progeny of an input multipotent progenitor.
