1995
DOI: 10.1089/ten.1995.1.361
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Cold-Storage of Synthetic Human Epidermis in HypoThermosol

Abstract: There is a growing need for engineered tissues in a wide variety of medical applications and as alternatives to animal tissues for in vitro toxicology testing. While techniques for the preparation of a variety of synthetic tissue constructs have been devised, little attention has been focused upon the optimum conditions necessary for storage and shipping of these tissue devices. This study investigates the effects of hypothermic storage on synthetic human epidermis (EpiDerm, MatTek Corp., Ashland, MA) and spec… Show more

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Cited by 16 publications
(14 citation statements)
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“…These features facilitate preservation of cell homeostasis, which is not achievable when using just culture medium as a preservation formulation. For example, normal human epidermal keratinocytes can be maintained for periods exceeding 1 week at 4°C in HTS and only 24 hours in normal growth medium at 4°C [21]. Currently, the incorporation of protective agents, including antioxidants, ion chelators, and membrane stabilizers, in preservation media has been reported to markedly improve preservation efficacy.…”
Section: Discussionmentioning
confidence: 99%
See 1 more Smart Citation
“…These features facilitate preservation of cell homeostasis, which is not achievable when using just culture medium as a preservation formulation. For example, normal human epidermal keratinocytes can be maintained for periods exceeding 1 week at 4°C in HTS and only 24 hours in normal growth medium at 4°C [21]. Currently, the incorporation of protective agents, including antioxidants, ion chelators, and membrane stabilizers, in preservation media has been reported to markedly improve preservation efficacy.…”
Section: Discussionmentioning
confidence: 99%
“…A variety of preservation solutions, such as ViaSpan (University of Wisconsin solution), Celsior, Custodiol histidine‐tryptophan‐ketoglutarate solution and, more recently, HypoThermosol (HTS), were developed taking these factors into consideration [15] and are commercially available today. These solutions showed to be effective for hypothermic storage of a large diversity of cells, tissues, and organs (including neonatal rat ventricular cardiomyocytes [16], renal cells [17], hepatocytes [18, 19], liver tissue [20], synthetic human epidermis tissue [21], kidney [22], pancreas [23], liver [20], and heart [24, 25]). Importantly, some of these formulations can be directly administered into patients, avoiding additional poststorage culture manipulations/costs and washing steps.…”
Section: Introductionmentioning
confidence: 99%
“…This assay, which yields a colorimetric change in proportion to cellular respiration, has been used to evaluate cell viability following hypothermic exposure (Acker and McGann, 2002;Cook et al, 1995). Organ samples were transferred 60·min after thawing to a 1.5-ml centrifuge tube containing 90·l alamarBlue diluted (1:10) with PBS, or PBS containing 80·mmol·l -1 urea, and incubated at 15°C with gentle orbital agitation for 120·min.…”
Section: Organ Cryoprotection By Ureamentioning
confidence: 99%
“…Storage at 4 °C is only utilised over relatively short time periods: hours for organs prior to transplantation; or days to weeks for tissue‐engineered products prior to application (Cook et al , ). Maintaining a cold chain at 4 °C is considerably simpler than maintaining one at cryogenic temperatures without a requirement for specialised equipment, and so it is conceivable that a cold chain from clinic (where tissue could be harvested), to tissue bank or cleanroom (where tissue could be stored or reconstructed tissue produced), to theatre (where transplant could be performed) could be devised without much complication.…”
Section: Discussionmentioning
confidence: 99%