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Using the method outlined in this study, 25 to 37 million bone marrow cells can be successfully isolated from a litter size of five C57BL/6 mouse pups. This method has been validated with litter sizes ranging from 5 to 7 pups. The minimum age for isolation in our experiments has been 7 days old. Depending on the litter size and the number of cells required for the experiment being less than a million, researchers could attempt this protocol for mice younger than 7 days old. In the presence of L929-cell supernatant as a source of M-CSF, bone marrow cells were differentiated into macrophages in 5 days (Figure 2). Formation of spindle-shaped cells was observed on the second day of differentiation (Figure 2B), nearly half of the cells showed a spindle shape on day three (Figure 2C), and most of the cells adhered and formed elongated spindle shapes on day five of differentiation (Figure 2D). The yield of bone marrow-derived macrophages (BMDMs) with this method was 2.5-5 million cells from 5 pups of 7 days of age.
To characterize the differentiated BMDMs phenotypically, cells from 5-day cultures were immunolabeled for CD11b, CD206, and F4/80. Forward/side scatter and single-marker gating schemes can be seen in Supplementary Figure 1. The results from the flow cytometry analysis demonstrated that 76.4% of the BMDMs are positive for both CD11b and F4/80 (Figure 3A). The F480-CD11b+ population is consistent with the approximate number of cells positive for CD206 (Figure 3B). The latter is generally considered a marker consistent with M2-like macrophages, and while the abundance of CD206 labeling can range as much as two-fold more, a higher proportion of F4/80 labeling is consistent with the ability of M-CSF to promote differentiation to an M1-like phenotype16,17(Figure 3).
We further evaluated the capability of the differentiated neonatal BMDMs to phagocytose bacteria and traffic them to acidified compartments as a functional measure. The bacteria labeled with a pH-sensitive dye should only fluoresce green when phagocytosed and trafficked to acidified compartments. Abundant green fluorescent bacteria phagocytosed inside the BMDMs were detected following infection (Figure 4A). The green fluorescence further localizes with red fluorescence indicative of acidified lysosomes (Figure 4B,C). The phagocytosis and appearance of green pH-sensitive dye-positive neonatal BMDMs were also observed throughout the 4 h infection (Figure 4D and Supplemental video). The functional activity displayed here is consistent with M1-like inflammatory macrophage activity.

Figure 1: Isolation of 7-day-old C57BL/6J mouse pups bone marrow. (A) Hind limb bones of 7-day-old pups in a 100 mm dish. (B) Hind limb of a 7-day-old pup after removing the skin and subcutaneous tissue; black dotted lines indicate the place to cut for the bone marrow extraction. (C) The neonatal hind limb processed bones with marrow prior to crushing. (D) The neonatal hind limb processed bones after crushing using a syringe plunger in a strainer. (E) The mean number ± standard error of bone marrow (BM) and bone marrow-derived macrophage cells obtained from three independent experiments. Please click here to view a larger version of this figure.

Figure 2: Differentiation of BMDMs from 7-day-old neonatal bone marrow cells. Bone marrow cells on day 1 (A), day 2 (B), day 3 (C), and day 5 of differentiation (D). Red arrows on panel B indicate spindle-shaped adhered cells on day 2 of differentiation. Scale bars: 200 µm. Please click here to view a larger version of this figure.

Figure 3: Detection of murine macrophage markers using flow cytometric analysis. Differentiated neonatal bone marrow-derived macrophages showing the expression of F4/80 and CD11b (A) or CD206 and CD11b (B) surface antigens. Please click here to view a larger version of this figure.

Figure 4: Phagocytosis of pH-sensitive dye-labeled E. coli by neonatal BMDMs. (A) Bone marrow-derived macrophages showing phagocytosed pH-sensitive dye-labeled (green) E. coli after 4 h of infection. (B) BMDMs labeled with stain for acidified lysosomes (red). (C) Merged image of panels (A) and (B). Scale bars: 20 µm. (D) An overlay of green fluorescent bacteria on macrophages shown in phase contrast. Magnification in (D) is the same as that in (A). Please click here to view a larger version of this figure.
Supplementary video. A 4 h video of live cell imaging of green florescent bacteria by neonatal BMDMs as in Figure 4 panel A. Please click here to download this Video.
Supplementary Figure 1: Flow cytometry analysis of BMDMs. (A) BMDMs were first gated on FSC and SSC to remove debris and doublets. Single staining of F4/80 (B), CD11b (C), and CD206 (D) is shown. Please click here to download this File.