Lieschke GJ, Grail D, Hodgson G, Metcalf D, Stanley E, Cheers C, Fowler KJ, Basu S, Zhan YF, Dunn AR:
Mice lacking granulocyte colony-stimulating factor have chronic neutropenia, granulocyte and macrophage progenitor cell deficiency, and impaired neutrophil mobilization.
Blood 1994 Sep 15;84(6):1737-46
ABSTRACT
Mice lacking granulocyte colony-stimulating factor (G-CSF) were
generated by targeted disruption of the G-CSF gene in embryonal stem
cells. G-CSF-deficient mice (genotype G-CSF-/-) are viable, fertile,
and superficially healthy, but have a chronic neutropenia.
Peripheral blood neutrophil levels were 20% to 30% of wild-type mice
(genotype G-CSF+/+) and mice heterozygous for the null mutation had
intermediate neutrophil levels, suggesting a gene-dosage effect. In
the marrow of G-CSF-/- mice, granulopoietic precursor cells were
reduced by 50% and there were reduced levels of granulocyte,
macrophage, and blast progenitor cells. Despite G-CSF deficiency,
mature neutrophils were still present in the blood and marrow,
indicating that other factors can support neutrophil production in
vivo. G-CSF-/- mice had reduced numbers of neutrophils available for
rapid mobilization into the circulation by a single dose of G-CSF.
G-CSF administration reversed the granulopoietic defect of G-CSF-/-
mice. One day of G-CSF administration to G-CSF-/- mice elevated
circulating neutrophil levels to normal, and after 4 days of G-CSF
administration, G-CSF+/+ and G-CSF-/- marrows were morphologically
indistinguishable. G-CSF-/- mice had a markedly impaired ability to
control infection with Listeria monocytogenes, with diminished
neutrophil and delayed monocyte increases in the blood and reduced
infection-driven granulopoiesis. Collectively, these observations
indicate that G-CSF is indispensible for maintaining the normal
quantitative balance of neutrophil production during "steady-state"
granulopoiesis in vivo and also implicate G-CSF in "emergency"
granulopoiesis during infections.
