Differentiation of erythroid progenitors in organ cultures of mouse embryonal liver

To study the reasons for the failure of erythroid differentiation in a long-term organ culture of mouse embryonal liver, the development of erythroid colony-forming progenitors was examined. The "early" (BFUei) and "late" (CFUei) erythropoietin-independent erythroid progenitors were present in washes from organ cultures for at least 56 days and in the "rests" of the cultures for 46 days. The mean concentration and the correlation of the "early" and "late" progenitors were similar to those in the bone marrow and initial embryonal liver. The data suggest that the stopping of erythroid differentiation in organ culture of embryonal liver occurs after CFUei formation, interfering with their maturation to morphologically recognizable erythroid cells.     

Electron-microscopic and electron-autoradiographic characteristics of embryonal lung cells in organ cultures]

Cells of the mouse embryonal lung at early stages of organotypical cultivation were studied by electron microscopy and autoradiography. The electron autoradiography technique allowed the fate of poorly differentiated cells to be elucidated.     

Colony-forming capacity of porcine liver epithelial cells in culture

Previously, we reported the presence of certain nonparenchymal epithelial cells (NPECs) in adult porcine livers that demonstrate differentiation patterns including an emergence of duct-like structures (DLSs) in the colonies. In the present study, we examined the effect of supplements to the NAIR-1 medium (Dulbecco modified Eagle medium [DMEM]-F12 containing 5% fetal bovine serum [FBS] and 11 supplements) used in these cultures on formation of DLSs-emerged colonies (type I colonies). No type I colonies were observed in the cultures of the nonparenchymal cell fraction when Roswell Park Memorial Institute-1640 medium or DMEM-F12 (1:1) supplemented with 5% FBS was used as the culture medium. NAIR-1 medium without each component did not produce any significant results. No type I colonies were formed when epidermal growth factor, and hydrocortisone and insulin mixture (A) or nicotinamide and l-ascorbic acid phosphate magnesium salt (Asc2P) mixture (B) was added to the DMEM-F12 medium supplemented with 5% FBS. However, when a combination of A and B was added, colonies were formed at a significant level. Together, the number of type I colonies was increased in the combination of A and B containing a higher concentration of Asc2P. We conclude that NPECs need a mixture of Asc2P and other components as supplements for type 1 colony formation.     

Effect of colony-stimulating activity on hematopoiesis in the organ culture of mouse embryonal liver

The effect of the colony-stimulating activity (CSA) on hemopoiesis in a long-term culture (4.5 week) of mouse embryonal liver was studied. After addition of the spleen cell-conditioned medium containing CSA to the organ culture, there was a decrease in the number of CFUs and in the granulocyte and macrophage precursors. However, the production of granulocytes and macrophages in the test cultures either did not fall or increased with primary differentiation of neutrophils. Addition of the medium with CSA shifted the equilibrium in the culture towards more intense production of differentiated cells at a lower level of the maintenance of precursors.     

Sensitivity of embryonal lungs of mice, rats and humans to exposure to nitrosomethylurea in organ cultures

With the direct action of nitrosomethylurea (NMU) in a concentration of 0.05 mg/ml on the organic cultures of the embryonic lung of mice of the A line, Wistar rats and man they developed a different degree of degenerative changes and hyperplastic epithelial proliferates. A toxic effect prevailed in the cultures at the initial experimental periods. The most sensitive to the toxic action of NMU was the lung tissue of rat embryos, and the least--of mice. The incidence of hyperplastic proliferates was, on the contrary, the greatest in the cultures of mouse lungs, and the least--of rat lungs. The sensitivity of the embryonic lungs of the man and rodents to the toxic action of NMU in repeated administration into the nutrient medium diminished during the cultivation. There was an increase of survival of the experimental cultures in comparison with the intact control.     

In vitro production of hemopoietic stem cells: washings from organ cultures of embryonic liver]

Hemopoietic cells including CFUs could be washed off from the organ culture of fetal liver periodically for 4 weeks. Under the cultivation conditions employed this treatment did not reduce the CFUs content of the culture essentially; thus, the washings off could be used to elevate the CFUs yield per culture.     

Medium conditioned by feeder cells inhibits the differentiation of embryonal carcinoma cultures

Non-dividing STO mouse fibroblasts have been used for some time as feeder cells for maintaining certain embryonal carcinoma cells in an undifferentiated state. We report here that medium conditioned by these feeders can inhibit embryonal carcinoma (ec) cell differentiation induced either by removal from feeders, or, in the case of cells not normally requiring a feeder layer, by retinoic acid treatment.     

Expression of c-myb in embryonal carcinoma cells and embryonal stem cells

Mouse c-myb has been implicated in the regulation of differentiation and proliferation of haematopoietic cells. Analysis of the chromatin structure of the promoter region of c-myb in embryonal carcinoma (EC) cells and embryonal stem (ES) cells reveals a DNAse I-hypersensitive site coincident with a site found in c-myb-expressing haematopoietic cells, but absent in murine fibroblasts (which do not express c-myb). EC and ES cells were found to express c-myb mRNA, albeit at a level lower than found in haematopoietic cells. Differentiation of ES cells into embryoid bodies resulted in an elevated level of c-myb expression.     

Proliferation of hemopoietic stem cells in culture of embryonal liver of mice

The vinblastine technique was used to demonstrate that the proliferative capacity of colony-forming cells in organ culture of embryonal liver of mice between the first and seventeenth day of cultivation is adequately high. The relative content of CFU increases in culture with a maximum between one and two weeks.     

Colony-forming hematopoietic cells in the mouse embryonic lung

The colony-forming activity of embryo lung cells CBA mice was determined according to the Till and McCulloch technique (1961). After intravenous injection to jung cells (1 x 10(6)) from 14-day embryos the total number of colonies on the area of 1 mm2 of spleen sections from irradiated recipient mice averaged 2.31 +/- 0.39 whereas after transplantation of lung cells from 15-day embryos it averaged 2.34 +/- 0.53. The percent of macrocolonies equalled 52.5% in the former case and only 2.5% in the latter case. Macrocolonies contained cells of the myeloid, erythroid and megakaryocyte lines. Microcolonies predominantly consisted of granulocytes at various stages of differentiation. Thus, polypotent stem hematopoietic cells migrate into the fetal lung in vivo. The colony-forming ability of the lung polypotent stem cells decreases as the period of embryogenesis increases.     

Myotube-like structures in cultures of rat liver cells

Branching and budding myotube-like structures developed in primary cultures of rat liver cells and in the JH1 cell line derived from them. Elongated uninuclear cells aligned in chains and fused into multinuclear tubes of varying length and thickness. The tubes contained thick and thin filaments running in all directions. The filaments were occasionally linked with M lines and formed incomplete hexagonal patterns resembling those of skeletal muscle myofilaments, but a regular arrangement of the filaments and organelles was lacking. Cross-striation and contractions were never observed. Both uninuclear cells and multinuclear tubes contained numerous lysosomes, myelin figures and lamellated bodies as well as electronlucent or content-filled vacuoles and cisternae of variable size, sometimes reminding the sarcoplasmic reticulum in early stages of its development. Endocytotic caveolae and vesicles were present in all elements. These features together with interdigitated cell processes and specialized cell contacts suggested a possible relationship of the cells to the reticuloendothelial system.