Engraftment of primates with G-CSF mobilized peripheral blood CD34+ progenitor cells expanded in G-CSF, SCF and MGDF decreases the duration and severity of neutropenia

We used a primate model of autologous peripheral blood progenitor cell (PBPC) transplantation to study the effect of in vitro expansion on committed progenitor cell engraftment and marrow recovery after transplantation. Four groups of baboons were transplanted with enriched autologous CD34(+) PBPC collected by apheresis after five days of G-CSF administration (100 mu g/kg/day). Groups I and III were transplanted with cryopreserved CD34(+) PBPC and Groups II and IV were transplanted with CD34(+) PBPC that had been cultured for 10 days in Amgen-defined (serum free) medium and stimulated,vith G-CSF, megakaryocyte growth and development factor (MGDF), and stem cell factor each at 100 eta g/ml. Group III and IV animals were administered G-CSF (100 mu g/kg/day) and MGDF (25 mu g/kg/day) after transplant, while animals in Groups I and II were not, For the cultured CD34(+) PBPC from groups II and IV, the total cell numbers expanded 14.4 +/- 8.3 and 4.0 +/- 0.7-fold, respectively, and CFU-GM expanded 7.2 +/- 0.3 and 8.0 +/- 0.4-fold, respectively. All animals engrafted, If no growth factor support was given after transplant (Groups II and I), the recovery of WBC and platelet production after transplant was prolonged if cells had been cultured prior to transplant (Group II). Administration of post-transplant G-CSF and MGDF shortened the period of neutropenia (ANC < 500/mu L) from 13 +/- 4 (Group 1) to 10 +/- 1 (Group III) days for animals transplanted with non-expanded CD34(+) PBPC, For animals transplanted with ex vivo-expanded CD34(+) PBPC, post-transplant administration of G-CSF and MGDF shortened the duration of neutropenia from 14 +/- 2 (Group II) to 3 +/- 4 (Group IV) days. Recovery of platelet production was slower in all animals transplanted with expanded CD34(+) PBPC regardless of post-transplant growth factor administration. Progenitor cells generated in vitro ran contribute to early engraftment and mitigate neutropenia when growth factor support is administered posttransplant. Thrombocytopenia was not decreased despite evidence of expansion of megakaryocytes in cultured CD34(+) populations.