Control of normal differentiation of myeloid leukemic cells. VIII. Induction of differentiation to mature granulocytes in mass culture

## Abstract An enriched population of early myeloid cells has been obtained from normal mouse bone marrow by injection of mice with sodium caseinate and the removal of cells with C3 (EAC) rosettes by Ficoll‐Hypaque density centrifugation. This enriched population had no EAC or Fc (EA) rosettes and

## Abstract Sera from different strains of mice injected with endotoxin induced clones (D^+^) from a cultured line of myeloid leukemic cells to undergo normal differentiation to mature granulocytes and macrophages. Other clones (D^−^) derived from the same cell line were not inducible by these sera

## Abstract Normal hematopoietic cells require the presence of a protein (MGI) in the appropriate conditioned medium (CM) for cell viability and growth and for differentiation to mature macrophages and granulocytes. Clones of myeloid leukemic cells have been established in culture (D^+^ clones) whi

## Abstract A line of mouse myeloid leukemic cells in culture contained two types of clones. One type can be induced by the differentiation‐inducing protein MGI to undergo normal differentiation to mature macrophages and granulocytes (D^+^ clones), whereas the other type could not be induced to dif

1) 'Cells were cultured in the absence or presence of trypsin (40 pMj. NBT reduction was determined on day 4 and macrophages on days 10 and 14. AB, KS, and GM were patients were acute myeloid leukemia from whoin leukemia cells were isolated and cultured. ' < 5 % of the cells. :'>80% of the cells.

## Abstract It is shown that the competence of differentiation‐defective clones of mouse myeloid leukemic cells (MGI^−^D^−^ clones) to be induced for some differentiation‐associated properties can be modulated. For certain inducers this was effected by changing the type of serum and for another ind