Table 2.
Summary of studies describing isolate methods and in vitro culture conditions for mouse BM-MSCs.
| Isolate method | Operation | Oxygen concentration | Initial medium replacement interval | Reference |
|---|---|---|---|---|
| Differential adhesion of the bone marrow | BM was flushed out from the bone cavity of femurs and tibias | Not mentioned | 72 h | [25, 56] |
| BM was flushed out from the bone cavity of femurs and tibias | Not mentioned | 48 h | [8, 31, 57] | |
| BM was flushed out from the bone cavity of femurs and tibias | Not mentioned | 24 h | [7, 30] | |
| BM was flushed out from the bone cavity of femurs and tibias | Not mentioned | 3 h | [32] | |
| Frequent medium change and treatment of the primary cultures with trypsin were used to purify the BM-MSCs | Not mentioned | 72 h | [19] | |
| Adapted centrifuge tubes were used to collect the bone marrow | Not mentioned | 24 h | [23] | |
| Frequent medium change and the diminishing trypsinization time were used to purify the BM-MSCs | Not mentioned | 8 h | [21] | |
| Density gradient centrifugation | BM was flushed out from the tibia and femur into lymphocyte separation medium | Not mentioned | 72 h | [58] |
| BM was loaded on 2 ml lymphodex and centrifuged at 350 ×g for 15 min | Not mentioned | 168 h | [20] | |
| Immunomagnetic bead cell sorting | Anti-CD11b-, CD34-, and CD45-conjugated dynabeads were used for immunodepletion | Not mentioned | 24 h or 48 h | [16] |
| The magnetic beads conjugated to anti-CD11b, anti-CD34, and anti-CD45 antibodies were used for immunodepletion | Not mentioned | 48 h | [17] | |
| Fluorescence-activated cell sorting | Cells isolated from BM were labeled with monoclonal antibodies and sorted with FACSAria II | 21%, 5%, or 2% | 72 h or 96 h | [22] |