The effect of Me 2 SO overexposure during cryopreservation on HOS TE85 and hMSC viability, growth and quality

Morris, Timothy; Picken, Andrew; Sharp, Duncan M.C.; Slater, Nigel K.H.; Hewitt, Christopher J.; Coopman, Karen

doi:10.1016/j.cryobiol.2016.09.004

Cited by 15 publications

(11 citation statements)

References 35 publications

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“… Assumption that data from sperm and embryos translated to somatic cells. Slow thawing – confounding of post thaw DMSO toxicity and slow thawing 36 , 37 . …”

Section: Discussionmentioning

confidence: 99%

The Impact of Varying Cooling and Thawing Rates on the Quality of Cryopreserved Human Peripheral Blood T Cells

Baboo

Kilbride

Delahaye

et al. 2019

Sci Rep

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For the clinical delivery of immunotherapies it is anticipated that cells will be cryopreserved and shipped to the patient where they will be thawed and administered. An established view in cellular cryopreservation is that following freezing, cells must be warmed rapidly (≤5 minutes) in order to maintain high viability. In this study we examine the interaction between the rate of cooling and rate of warming on the viability, and function of T cells formulated in a conventional DMSO based cryoprotectant and processed in conventional cryovials. The data obtained show that provided the cooling rate is −1 °C min −1 or slower, there is effectively no impact of warming rate on viable cell number within the range of warming rates examined (1.6 °C min −1 to 113 °C min −1 ). It is only following a rapid rate of cooling (−10 °C min −1 ) that a reduction in viable cell number is observed following slow rates of warming (1.6 °C min −1 and 6.2 °C min −1 ), but not rapid rates of warming (113 °C min −1 and 45 °C min −1 ). Cryomicroscopy studies revealed that this loss of viability is correlated with changes in the ice crystal structure during warming. At high cooling rates (−10 °C min −1 ) the ice structure appeared highly amorphous, and when subsequently thawed at slow rates (6.2 °C min −1 and below) ice recrystallization was observed during thaw suggesting mechanical disruption of the frozen cells. This data provides a fascinating insight into the crystal structure dependent behaviour during phase change of frozen cell therapies and its effect on live cell suspensions. Furthermore, it provides an operating envelope for the cryopreservation of T cells as an emerging industry defines formulation volumes and cryocontainers for immunotherapy products.

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“… Assumption that data from sperm and embryos translated to somatic cells. Slow thawing – confounding of post thaw DMSO toxicity and slow thawing 36 , 37 . …”

Section: Discussionmentioning

confidence: 99%

The Impact of Varying Cooling and Thawing Rates on the Quality of Cryopreserved Human Peripheral Blood T Cells

Baboo

Kilbride

Delahaye

et al. 2019

Sci Rep

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“…Currently, the existing cryopreservation methods for MSCs can be classified into two main categories, slow freezing and vitrification (rapid freezing) [ 10 ]. But both methods have some notable limitations [ 11 ], and there is an increasing amount of evidence showing the adverse effects of conventional cryopreservation methods for MSCs, such as the cytotoxicity of the standard cryoprotectant dimethyl sulfoxide (DMSO), cell apoptosis, cellular structure damages, and oxidative stress [ 12 – 14 ]. Recently, many approaches have been proposed for a more efficient application of cryopreserved MSCs, among which addition of selected agents in cryopreservation solution has shown good application prospects [ 15 , 16 ].…”

Section: Introductionmentioning

confidence: 99%

Icariin Improves the Viability and Function of Cryopreserved Human Nucleus Pulposus-Derived Mesenchymal Stem Cells

Chen

Deng

et al. 2018

Oxidative Medicine and Cellular Longevity

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Nucleus pulposus-derived mesenchymal stem cells (NPMSCs) have shown a good prospect in the regeneration of intervertebral disc (IVD) tissues. However, fresh NPMSCs are not always readily available for basic research and clinical applications. Therefore, there is a need for an effective long-term cryopreservation method for NPMSCs. The aim of this study was to determine whether adding icariin (ICA) to the conventional cryoprotectant containing dimethyl sulfoxide (DMSO) had a better cryoprotective effect for NPMSCs. The results showed that the freezing solution containing ICA along with DMSO significantly increased the postthawed cell viability, decreased the apoptosis rate, improved cell adherence, and maintained the mitochondrial functions, as compared to the freezing solution containing DMSO alone. And the inhibition of oxidative stress and upregulation of heat shock proteins (HSPs) in the presence of ICA also confirmed the beneficial effect of ICA. Furthermore, ICA had no cytotoxicity and did not alter the characteristics of postthawed NPMSCs. In conclusion, these results suggested that the addition of ICA to the conventional freezing medium could improve the viability and function of the cryopreserved human NPMSCs and provided an optimal formulated freezing solution for human NPMSC cryopreservation.

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“…Recent studies with HepG2 cells suggested slow thawing up to -10°C, and then rapid thawing from -10°C to 4°C is beneficial due to the reduction of microfluctuations [39]. Finally, rapid thawing may not be beneficial due to the potential for increased toxicity of DMSO, especially if temperatures approach 37°C before wash-out [40]. An ideal thawing protocol for some cell types may consist of slow thawing to 4°C, followed by immediate dilution of cells in cold medium to reduce the toxic effects of DMSO prior to centrifugation.…”

Section: Discussionmentioning

confidence: 99%

Cryopreservation of midbrain dopaminergic neural cells differentiated from human embryonic stem cells

Drummond

Dolt

Canham

et al. 2020

Preprint

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Recent advancements in protocols to differentiate human pluripotent stem cells into midbrain dopaminergic (mDA) neurons has improved the ability to model Parkinson's disease (PD) in a dish, and has provided a scalable source of donor cells for emerging PD cell replacement therapy (CRT). However, to facilitate reproducibility, collaboration, and clinical trials it would be highly beneficial to cryopreserve committed mDA neural precursors cells in a ready-to-use format. In terms of cell manufacturing for PD CRT trials, a cryopreserved transplantation-ready mDA cell product would provide a critical opportunity for quality control, efficacy testing, and safety assessments. To address this challenge, we have compared six (6) different clinical-grade cryopreservation media and different freezing conditions for mDA neural precursor cells differentiated from two human embryonic stem cell (ESC) lines, MasterShef7 and RC17. Significant differences in cell viability were observed at 24h post-thawing, but no differences were observed immediately upon thawing. This highlights the need to check cell viability over the first 24h after thawing, and that viability of freshly thawed cells is insufficient to gauge the success of a cryopreservation protocol. Considerable apoptosis occurs in the first 24h post-thawing, and significant differences between cryopreservation procedures were only revealed during this time period. The presence of ROCK inhibitors improved cell viability at 24h for all conditions tested. A faster cooling rate of 1-2°C/min was significantly better than 0.5°C/min for all conditions tested, while rapid thawing at 37°C was not always superior to slow thawing at 4°C. Indeed, the optimal cryopreservation and thawing conditions in this study, as determined by 24h post-thaw viability, were cells frozen in PSC Cryopreservation medium at a cooling rate of 1°C/min and slow thawing at 4°C. These conditions permitted recovery of 60%-70% live cells at 24h with respect to the starting number of cryopreserved cells. Importantly, cryopreservation of mDA neural precursor cells did not alter their potential to resume differentiation into mDA neurons. Highlights:• First systematic comparison of multiple clinical-grade cryopreservation media for human ESC-derived mDA neural precursor cells• Differences in cell viability were observed at 24h after thawing, but not immediately upon thawing• Cooling rates of 1°C/min or 2°C/min were significantly better than 0.5°C/min for all cryopreservation conditions tested • A slow thawing condition at 4°C was significantly better than quick thawing at 37°C for cells frozen in PSC Cryopreservation medium • Cryopreservation of mDA cells does not significantly alter their potential to differentiate into mDA neurons

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The effect of Me 2 SO overexposure during cryopreservation on HOS TE85 and hMSC viability, growth and quality

Cited by 15 publications

References 35 publications

The Impact of Varying Cooling and Thawing Rates on the Quality of Cryopreserved Human Peripheral Blood T Cells

The Impact of Varying Cooling and Thawing Rates on the Quality of Cryopreserved Human Peripheral Blood T Cells

Icariin Improves the Viability and Function of Cryopreserved Human Nucleus Pulposus-Derived Mesenchymal Stem Cells

Cryopreservation of midbrain dopaminergic neural cells differentiated from human embryonic stem cells

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