In Vitro Culture and Differentiation of Primary Monocytes into Macrophages
In Vitro Culture and Differentiation of Primary Monocytes into Macrophages
내레이션 대본
Monocytes are immune cells that differentiate into macrophages and antigen-presenting dendritic cells to protect against infection.
To culture monocytes and induce their differentiation in vitro, begin by taking a suspension of primary human monocytes in a suitable culture medium. Add the cell suspension into the wells of a culture plate. Incubate at physiological conditions to allow the cells to adhere.
Add differentiation-inducing cytokines — granulocyte-macrophage colony-stimulating factor, or GM-CSF, to one well and macrophage colony-stimulating factor, or M-CSF, to another. Incubate for an appropriate duration.
GM-CSF binds to its heterodimeric receptor on the cells and induces the differentiation of the monocytes. GM-CSF binding results in the activation of intracellular signaling pathways, leading to the expression of genes for priming into an M1 macrophage-like phenotype.
The M1-like cells — rounded cells with a large cytoplasmic volume — are pro-inflammatory and assist in the defense against infection.
In the other well, the M-CSF binds to its homodimeric receptor on the monocytes and induces the differentiation of the cells. M-CSF binding results in the activation of intracellular signaling pathways different from GM-CSF, leading to the expression of genes for priming into an M2 macrophage-like phenotype.
The M2-like cells — with an elongated shape — are anti-inflammatory and exhibit tissue remodeling and repair functions.
The differentiated macrophage cells are ready for further downstream assays.