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      Alginate Hydrogel Microencapsulation Inhibits Devitrification and Enables Large-Volume Low-CPA Cell Vitrification

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          Abstract

          Cryopreservation of stem cells is important to meet their ever-increasing demand by the burgeoning cell-based medicine. The conventional slow freezing for stem cell cryopreservation suffers from inevitable cell injury associated with ice formation and the vitrification (i.e., no visible ice formation) approach is emerging as a new strategy for cell cryopreservation. A major challenge to cell vitrification is intracellular ice formation (IIF, a lethal event to cells) induced by devitrification (i.e., formation of visible ice in previously vitrified solution) during warming the vitrified cells at cryogenic temperature back to super-zero temperatures. Consequently, high and toxic concentrations of penetrating cryoprotectants (i.e., high CPAs, up to ~8 M) and/or limited sample volumes (up to ~2.5 μl) have been used to minimize IIF during vitrification. We reveal that alginate hydrogel microencapsulation can effectively inhibit devitrification during warming. Our data show that if ice formation were minimized during cooling, IIF is negligible in alginate hydrogel-microencapsulated cells during the entire cooling and warming procedure of vitrification. This enables vitrification of pluripotent and multipotent stem cells with up to ~4 times lower concentration of penetrating CPAs (up to 2 M, low CPA) in up to ~100 times larger sample volume (up to ~250 μl, large volume).

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          Most cited references45

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          Dripping to jetting transitions in coflowing liquid streams.

          A liquid forced through an orifice into an immiscible fluid ultimately breaks into drops due to surface tension. Drop formation can occur right at the orifice in a dripping process. Alternatively, the inner fluid can form a jet, which breaks into drops further downstream. The transition from dripping to jetting is not understood for coflowing fluid streams, unlike the case of drop formation in air. We show that in a coflowing stream this transition can be characterized by a state diagram that depends on the capillary number of the outer fluid and the Weber number of the inner fluid.
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            Ice-free cryopreservation of mouse embryos at −196 °C by vitrification

            W Rall, G Fahy (1985)
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              Cryobiology: The Freezing of Biological Systems

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                Author and article information

                Journal
                Advanced Functional Materials
                Adv. Funct. Mater.
                Wiley
                1616301X
                November 2015
                November 2015
                October 15 2015
                : 25
                : 44
                : 6839-6850
                Affiliations
                [1 ]Department of Biomedical Engineering; The Ohio State University; Columbus OH 43210 USA
                [2 ]Department of Mechanical Engineering; The Ohio State University; Columbus OH 43210 USA
                [3 ]Davis Heart and Lung Research Institute; The Ohio State University; Columbus OH 43210 USA
                [4 ]Center for Biomedical Engineering; Department of Electronic Science and Technology; University of Science and Technology of China; Hefei Anhui 230027 P.R. China
                [5 ]Comprehensive Cancer Center; The Ohio State University; Columbus OH 43210 USA
                Article
                10.1002/adfm.201503047
                4667367
                26640426
                bbaeccf6-cb08-483b-a96b-137091a38eb7
                © 2015

                http://doi.wiley.com/10.1002/tdm_license_1.1

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