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©The Author(s) 2021.
World J Stem Cells. Sep 26, 2021; 13(9): 1197-1214
Published online Sep 26, 2021. doi: 10.4252/wjsc.v13.i9.1197
Published online Sep 26, 2021. doi: 10.4252/wjsc.v13.i9.1197
Table 3 Comparison of different protocols used during cryopreservation of induced pluripotent stem cells
| Source of cell | Storage periode and temperature | Cryopreservation | Viability | Parameters | Results | Ref. |
| 1.5 x 106-2 x 106 hiPSC line UMN PCBC16iPS | Controlled rate; -196 °C | NEAA, sucrose, glycerol, isoleucine and albumin in a P188 in HBSS vs 7.5% DMSO; Aggregates vs single cells | Viability, adherence and intracellular ice formation | P188 was found here to not only inhibit ice formation significantly but also soften the solid-liquid interface of ice and increase the distance between adjacent ice crystals; The cryoprotective effects of the DMSO- free CPA cocktail could be capitalized only with the optimized composition. Deviation from the optimum may result in less desirable outcomes | [96,97] | |
| H9 hESC and hiPSC | 3-6 d,controlled rate; -80 °C | 10% DMSO, 10% EG, 10% PG, 10% glycerol, clumps vs single cells; ROCK inhibitor after thawing | EG-DMSO> PG>>glycerol | Toxicity of CPAs, expression of NANOG by hiPSCs | Freezing single cell iPSCs in the presence of a ROCK inhibitor and EG and programmable freezing drastically improved the yield of iPSCs in comparison to standard freezing in clumps without ROCK inhibitor | [98] |
| 1-2x106 hiPSC | -196 °C | A: 10% DMSO/90% FBS; B: 10% DMSO/90% KSR; C: 10% DMSO/ESC medium + 20%KSR + ROCK inhibitor; Single cells | A: 90%; B: 70%; C: 70% | Viability, karyotype, expression of pluripotency markers TRA-1-60, TRA-1-81, Oct4, SSEA-3, and SSEA-4, embryoid body formation, neuronal differentiation, colony formation | Addition of ROCK inhibitor to pre- and post-thaw culture media increased survival rate, hiPSCs retained typical morphology, stable karyotype, expression of pluripotency markers and the potential to differentiate into derivatives of all three germ layers after long-term culture | [103,105,108] |
| hiPSC | -196 °C | 10% DMSO in KO DMEM, 20% KSR, 1% NEAA, 1% L-glutamine, 0.2% b-mercaptoethanol, 1% antibiotic/ antimycotic and 8 ng/mL bFGF; ROCK inhibitor after thawing; Single cells | Colony number and size | ROCK inhibitor Y-27632 significantly improves the recovery of cryopreserved human iPS cells and their growth upon subculture | [104] | |
| hiPSC line 253G4 and 201B2 | 7 d, Vitrification in; -196 °C | VS2E vitrification solution (40% EG, 10% PEG in Euro-Collins medium), DAP213 vitrification solution (1.2% DMSO, 22% PG, 5.9% acetamide); Single cells | VS2E>DAP213 | Proliferation, expression of pluripotency markers Oct3/4, SSEA4, ALP, pluripotency in teratoma assay | Higher recovery rate of hiPSCs with DMSO and serum-free VS2E vitrification medium, cells after vitrification expressed Oct-3/4 and SSEA-4 and alkaline phosphatase and retained their pluripotency | [114] |
- Citation: Erol OD, Pervin B, Seker ME, Aerts-Kaya F. Effects of storage media, supplements and cryopreservation methods on quality of stem cells. World J Stem Cells 2021; 13(9): 1197-1214
- URL: https://www.wjgnet.com/1948-0210/full/v13/i9/1197.htm
- DOI: https://dx.doi.org/10.4252/wjsc.v13.i9.1197