Retinoid-regulated gene expression in normal and leukemic myeloid cells

## Abstract It has previously been shown that there are different molecular forms of macrophage‐ and granulocyte‐inducing (MGI) proteins; one form, MGI‐I, induced the formation of colonies with differentiated cells from normal myeloblasts and another form, MGI‐2, induced normal differentiation in M

## 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 Regulation of gene expression has been analysed in different clones of mouse myeloid leukemic cells treated with the tumor promoter 12‐__O__‐tetradecanoyl‐phorbol‐13‐acetate (TPA), the macrophage‐ and granulocyte‐in‐ducing protein MGI, and combined treatment with TPA and MGI. Two‐dimens

## Abstract A cloned line of myeloid leukemic cells can be induced by the alkylating agent nitrosoguanidine for two macrophage‐ and granulocyte‐inducing (MGI) activities. One activity, MGI‐1, induced the formation of macrophage and granulocyte colonies from normal myeloblasts. Another activity, MGI

## Abstract Regulation of the developmental programs for macrophages and granulocytes has been analysed, using two‐dimensional gel electrophorels of the cytoplasmic protein changes, in a human myeloid leukemic cell line (HL60) that can be induced to differentiate to macrophages by the macrophage an