Theoretical approaches to determination of optimal cryopreservation regimens for cell spheroids of different cultivation terms

doi:10.26565/2075-3810-2021-46-01

A. I. Moisieiev Institute for Problems of Cryobiology and Cryomedicine of the NAS of Ukraine 23, Pereyaslavska str., Kharkiv, Ukraine, 61016 https://orcid.org/0000-0003-4585-1194
I. F. Kovalenko Institute for Problems of Cryobiology and Cryomedicine of the NAS of Ukraine 23, Pereyaslavska str., Kharkiv, Ukraine, 61016 https://orcid.org/0000-0002-7063-6712
G. A. Bozhok Institute for Problems of Cryobiology and Cryomedicine of the NAS of Ukraine 23, Pereyaslavska str., Kharkiv, Ukraine, 61016 https://orcid.org/0000-0002-4188-9286
O. I. Gordiyenko Institute for Problems of Cryobiology and Cryomedicine of the NAS of Ukraine 23, Pereyaslavska str., Kharkiv, Ukraine, 61016 https://orcid.org/0000-0002-4459-4213

DOI: https://doi.org/10.26565/2075-3810-2021-46-01

Keywords: spheroids, cryopreservation, L929 line fibroblasts, filtration coefficients, permeability coefficients for DMSO, activation energy, cooling rate

Abstract

Background: Three-dimensional culture systems are unique platforms for studying complex biological processes in vitro. Cell-cell and cell-extracellular matrix interactions form a communication network of biochemical and mechanical signals, bring spheroids (SP) closer to native tissues and significantly distinguish them from monolayer cultures. It is important for cell technologies to develop methods for cryopreservation of 3D cultures, that allows creating the stocks of valuable cell samples, save time and materials, and prevent the loss of cultures due to technical failures, contamination, phenotype drift and aging.

Objectives: Development of approaches to cellular spheroids cryopreservation. Determination of the permeability parameters of L929 cells spheroids at different cultivation periods for the theoretical assessment of optimal freezing regimens.

Materials and methods: We have used L929 cells, which form SPs of different diameters and can be maintained for a long time in 3D conditions. To determine the integral filtration Lp and permeability for DMSO kp coefficients for SP at different periods of cultivation, the volumetric method was used. The study of the changes in the spheroids volume in time was carried out with a confocal microscope LSM 510 META. The numerical values of the integral SF permeability coefficients were determined by approximating the experimental data on the change in the relative volume of the SP versus the exposure time in the test solution with theoretical curves calculated on the basis of a physical and mathematical model for passive mass transfer between the spheroid and the environment, provided that they coincide as much as possible. Prediction of the osmotic behavior of spheroids under cooling conditions was carried out based on the differential equation describing the kinetics of changes in the relative cell volume during extracellular crystallization of a cryoprotective solution, substituting determined values of integral permeability coefficients Lp and kp and activation energies E_AL and E_Ak into the model equations. The kinetics of changes in the extracellular solution concentration during freezing was set analytically by approximating the phase melting diagram of the DMSO solution.

Results: The filtration and permeability for DMSO molecules coefficients in SP were determined and their significant decrease with a cultivation duration was shown. The activation energy values for the penetration of water and DMSO molecules into the SP were calculated and their dependence on the cultivation time was determined. Proceeding from the determined parameters of permeability, the dynamic of changes in the volume of SPs for different periods of cultivation at different rates of cooling was calculated.

Conclusions: The optimal cooling modes of SP from L929 cells were in theory determined: for 7 days of cultivation — 1,5-2 °C/min with cooling to -80°C and subsequent immersion in nitrogen; for 14 and 21 days of cultivation — 0.5 °C/min to -40°C and subsequent immersion in nitrogen.

Downloads

Download data is not yet available.

References

Woappia Y, Altomareb D, Creek K, Pirisi L. Self-assembling 3D spheroid cultures of human neonatal keratinocytes have enhanced regenerative properties. Stem Cell Research. 2020;49:102048. https://doi.org/10.1016/j.scr.2020.102048

Petrenko Y, Syková E, Kubinová Š. The therapeutic potential of three-dimensional multipotent mesenchymal stromal cell spheroids. Stem Cell Research&Therapy.2017;8:94. https://doi.org/10.1186/s13287-017-0558-6

Edmondson R, Broglie J, Adcock A, Yang L. Three-dimensional cell culture systems and their applications in drug discovery and cell-based biosensors. Assay Drug Dev Technol. 2014;12(4):207–218. https://doi.org/10.1089/adt.2014.573

Xu Y, Shi T, Xu A, Zhang L. 3D spheroid culture enhances survival and therapeutic capacities of MSCs injected into ischemic kidney. J Cell Mol Med. 2016;20(7):1203-1213. https://doi.org/10.1111/jcmm.12651

Seno K, Munakata Y, Sano M, et al. Aggregation of human trophoblast cells into three-dimensional culture system enhances anti-inflammatory characteristics through cytoskeleton regulation. Int J Mol Sci.2018;19:2322. https://doi.org/10.3390/ijms19082322

Baptista, LS, Kronemberger GS, Cortes I, et al. Adult stem cells spheroids to optimize cell colonization in scaffolds for cartilage and bone tissue engineering. Int J Mol Sci. 2018;19:1285. https://doi.org/10.3390/ijms19051285

Dong H, Li X, Chen K, Li N, Kagami H. Cryopreserved spontaneous spheroids from compact bone-derived mesenchymal stromal cells for bone tissue engineering. Tissue Eng Part C Methods. 2021;27(4):253–263. https://doi.org/10.1089/ten.TEC.2021.0001

Jensen C, Teng Y. Is it time to start transitioning from 2D to 3D cell culture?.Front Mol Biosci. 2020;7:33. https://doi.org/10.3389/fmolb.2020.00033

Griffith LG, Swartz MA. Capturing complex 3D tissue physiology in vitro. Nat Rev Mol Cell Biol. 2006;7(3):211-224. https://doi.org/10.1038/nrm1858

Lin RZ, Chang HY. Recent advances in three-dimensional multicellular spheroid culture for biomedical research. Biotechnol J. 2008;3(9-10):1172–1184. https://doi.org/10.1002/biot.200700228

Pampaloni F, Reynaud E, Stelzer E. The third dimension bridges the gap between cell culture and live tissue. Nat Rev Mol Cell Biol. 2007; 8 (10): 839–845. https://doi.org/10.1038/nrm2236

Ryu N, Lee S, Park H. Spheroid culture system methods and applications for mesenchymal stem cells. Cells. 2019;8(12):1620. https://doi.org/10.3390/cells8121620

Gordiyenko OI, Kovalenko SYe, Kovalenko IF, Ogurtsova VV, Todrin AF. Theoretical estimation of the optimum cooling rate of a cell suspension at linear freezing modes based on a two factor theory of cryodamage. CryoLetters. 2018;39(6):380–385.

Lee JH, Jung DH, Lee DH, Park JK, Lee SK. Effect of spheroid aggregation on susceptibility of primary pig hepatocytes to cryopreservation. Transplant Proc. 2012;44(4):1015–7. https://doi.org/10.1016/j.transproceed.2012.03.009

Ehrhart F, Schulz JC, Katsen-Globa A, Shirley SG, Reuter D, Bach F, at al. A comparative study of freezing single cells and spheroids: towards a new model system for optimizing freezing protocols for cryobanking of human tumours. Cryobiology. 2009;58(2):119–27. https://doi.org/10.1016/j.cryobiol.2008.11.005

Purcell WM, Atterwill CK, Xu J. Cryopreservation of organotypic brain spheroid cultures. Altern Lab Anim. 2003 Dec; 31(6): 563–73. https://doi.org/10.1177/026119290303100605

Sundlisaeter E, Wang J, Sakariassen P, Marie M, Mathisen J, Karlsen B, at al. Primary glioma spheroids maintain tumourogenicity and essential phenotypic traits after cryopreservation. Neuropathol Appl Neurobiol.2006;32(4):419–27. https://doi.org/10.1111/j.1365-2990.2006.00744.x

Gordiyenko YeO, Gordiyenko OI, Maruschenko VV, Sakun OV. [Improved model for the passive mass transfer through the cell plasma membrane]. Biophysical bulletin. 2008;21(2);75–80. (in Ukrainian).

Tarusin DN, Kireyev VA, Kovalenko SYe, Kovalenko IF, Rozanov LF, Petrenko AYu. Selection of protocols to cryopreserve mesenchymal stromal cells in suspension and alginate microspheres by studying their osmotic responses in 1M DMSO. Problems of cryobiology and cryomedicine. 2016;26 (2):133–144. https://doi.org/10.15407/cryo26.02

Amereh M, Edwards R, Akbari M, Nadler B. In-silico modeling of tumor spheroid formation and growth. Micromachines (Basel). 2021;12(7):749. https://doi.org/10.3390/mi12070749

Netti L. Baxter Y. Boucher R. Skalak R. Jain M. Fluid тransport in living tissues: application to solid tumors. Aiche Journal. 1997;43:818–834.

Demuynck R, Efimova I, Lin A, Declercq H, Krysko D. A 3D cell death assay to quantitatively determine ferroptosis in spheroids. Cells. 2020 Mar 13; 9(3):703. https://doi.org/10.3390/cells9030703

Ogurtsova VV, Kovalenko SYe,.Kovalenko IF, Gordiyenko OI. Determination of osmotically inactive volume of murine enterocytes, Probl Cryobiol Cryomed. 2016;26(1):93-97. https://doi.org/10.15407/cryo26.01.093

Gordiyenko YeO, Pushkar NS. [Physical basis for low temperature preservation of cell suspensions]. Кyiv: Naukova dumka; 1994. 140 p. (In Russian).

Todrin OF. Popivnenko LI, Kovalenko SYE. Thermophysical properties of cryoprotectants. I. Temperature and Heat of Melting. Problems of Cryobiology. 2009;19(2):163–176

Gordienko OI, Kovalenko IF, Kovalenko SYe, Kuleshova LG, Todrin OF. Theoretical estimation of optimal linear cooling rate for PK-15 cell suspension. Probl Cryobiol Cryomed. 2021;31(3):214–222. https://doi.org/10.15407/cryo31.03

Shevchenko NA, Strybul TF, Rozanov LF. Effect of multiatom alcohols, amides and DMSO on grape and potato meristems integrity. Problems of Cryobiology. 2004;3:79–85

Achilli T-M, Meyer J, Morgan JR. Advances in the formation, use and understanding of multi-cellular spheroids. Expert Opin Biol Ther. 2012;12(10):1347–60. https://doi.org/10.1517/14712598.2012.707181

Mazur P. Theoretical and experimental effects of cooling and warming velocity on the survival of frozen and thawed cells. Cryobiology. 1966;2:181–92

Chang T, Zhao G. Ice Inhibition for Cryopreservation: Materials, Strategies, and Challenges. Adv Sci (Weinh). 2021;8(6):2002425. https://doi.org/10.1002/advs.202002425

Yu G, Yap Y, Pollock K, Hubel A. Characterizing Intracellular Ice Formation of Lymphoblasts Using Low-Temperature Raman Spectroscopy. Biophys J. 2017;112(12):2653–63. https://doi.org/10.1016/j.bpj.2017.05.009

Mazur P. The role of intracellular freezing in the death of cells at supraoptimal rates. Cryobiology. 1977;14(2):251–72

Pegg DE. Principles of cryopreservation. Methods Mol Biol. 2015;1257:3–19. https://doi.org/10.1007/978-1-4939-2193-5_1

Wesley-Smith J, Walters C, Pammenter NW, Berjiak P. Why is intracellular ice lethal? A microscopical study showing evidence of programmed cell death in cryo-exposed embryonic axes of recalcitrant seeds of Acer saccharinum. Ann Bot. 2015;115(6):991–1000. https://doi.org/10.1093/aob/mcv009

Li R, Yu G., Azarin SM, Hubel A. Freezing Responses in DMSO-Based Cryopreservation of Human iPS Cells: Aggregates Versus Single Cells. Tissue Eng Part C Methods. 2018;24(5):289–99. https://doi.org/10.1089/ten.TEC.2017.0531

Kosheleva NV, Efremov YM, Shavkuta BS. Cell spheroid fusion: beyond liquid drops model. Sci. Rep.2020; 10:12614. https://doi.org/10.1038/s41598-020-69540-8