Detection of in vitro macrophage colony-forming cells (M-CFC) in mouse bone marrow, spleen, and peripheral blood

## Abstract In vitro moocyte‐macrophage colony‐forming cells (CFC) have been detected in the thymus (30/10^6^ cells) and in the cervical (22/10^6^) and mesenteric (20/10^6^) lymph nodes (LN) of the mouse. Thymus and LN derived CFC differed from bone marrow derived CFU‐c in several characteristic pa

An adaptation of a previously reported flow cytometric technique is described. This technique was applied to study the DNA distribution of mouse granulocyte-macrophage colony forming cells (GM-CFc) grown in a methyl cellulose culture system. This method involved the collection of cell clusters and c

## Abstract The technique of buoyant density separation in gradients of Bovine Serum Albumin has been used to separate hemopoietic cell populations in mouse bone marrow that form __in vivo__ spleen colonies and __in vitro__ colonies of granulocytes and macrophages in an agar culture system. The den

## Abstract Three assays for bone marrow progenitor cells have been used to determine the effect of single doses of two cytotoxic agents, cyclophosphamide and vinblastine. The assays employed were the agar colony forming and spleen colony forming assays and the crythroid repopulating ability. In n

## Abstract C~57~BL bone marrow cells were separated on the basis of their sedimentation velocity at unit gravity and cell fractions cultured in agar using three types of colony stimulating factor (CSF). Colony‐forming cells separated as a single peak (s = 4.4 mm/hr) in cultures stimulated by mouse

The production of granulocyte-macrophage colony-stimulating activity (CSA) by isolated murine femur shafts, non-dispersed bone marrow and spleens was assessed following administration of Vinblastine (VLB). These organs were removed from 2 h to 10 days post-VLB and allowed to condition endotoxin-free