Hypothermic storage of isolated human hepatocytes: a comparison between University of Wisconsin solution and a hypothermosol platform

Ostrowska, Alina; Gu, Kenan; Bode, Donald C.; Buskirk, Robert G. Van

doi:10.1007/s00204-009-0419-x

Cited by 38 publications

(32 citation statements)

References 45 publications

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“…Trolox is also known to have a significant iron-chelating capacity [28]; iron chelators have been found to be one of the key elements to enable high attachment efficiency of preserved cells after long term hypothermic storage of rat hepatocytes [27,28]. The importance of Trolox for cold storage of human hepatocytes beyond 48 hours was shown by Ostrowska and co-workers [29] where they compared HTS-FRS against UW and HTS-Base (without Trolox) and found that HTS-FRS was the only solution to prevent damages beyond 48 hours. While ROS generation during short static cold storage at +4 o C has been shown to be low [30] and the lipid peroxidation to be slow [31], similar data does not exist for long storage during cold storage or supercooling.…”

Section: Discussionmentioning

confidence: 99%

Supercooling as a Viable Non-Freezing Cell Preservation Method of Rat Hepatocytes

et al. 2013

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Supercooling preservation holds the potential to drastically extend the preservation time of organs, tissues and engineered tissue products, and fragile cell types that do not lend themselves well to cryopreservation or vitrification. Here, we investigate the effects of supercooling preservation (SCP at -4oC) on primary rat hepatocytes stored in cryovials and compare its success (high viability and good functional characteristics) to that of static cold storage (CS at +4oC) and cryopreservation. We consider two prominent preservation solutions a) Hypothermosol (HTS-FRS) and b) University of Wisconsin solution (UW) and a range of preservation temperatures (-4 to -10 oC). We find that there exists an optimum temperature (-4oC) for SCP of rat hepatocytes which yields the highest viability; at this temperature HTS-FRS significantly outperforms UW solution in terms of viability and functional characteristics (secretions and enzymatic activity in suspension and plate culture). With the HTS-FRS solution we show that the cells can be stored for up to a week with high viability (~56%); moreover we also show that the preservation can be performed in large batches (50 million cells) with equal or better viability and no loss of functionality as compared to smaller batches (1.5 million cells) performed in cryovials.

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Section: Discussionmentioning

confidence: 99%

Supercooling as a Viable Non-Freezing Cell Preservation Method of Rat Hepatocytes

et al. 2013

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“…Oxidative stress has been ascribed a significant role in cellular damage because it alters the functional properties of cell membranes through lipid peroxidation (Vara et al 1995; Meng 2003). Therefore, recent preservation solution development has focused on a few critical topics including the maintenance of ionic and osmotic balance, the prevention of cell swelling and blebbing, the control of free radical formation and the development of serum-free media (Ostrowska et al 2009). Consequently, cold storage solutions containing antioxidants, iron chelators and/or membrane stabilizers have been developed to protect cells from such damages (Meng 2003; Pless et al 2012).…”

Section: Liver In Vitro Models In Pharmacology Toxicology and Basic mentioning

confidence: 99%

Recent advances in 2D and 3D in vitro systems using primary hepatocytes, alternative hepatocyte sources and non-parenchymal liver cells and their use in investigating mechanisms of hepatotoxicity, cell signaling and ADME

Hewitt²,

et al. 2013

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This review encompasses the most important advances in liver functions and hepatotoxicity and analyzes which mechanisms can be studied in vitro. In a complex architecture of nested, zonated lobules, the liver consists of approximately 80 % hepatocytes and 20 % non-parenchymal cells, the latter being involved in a secondary phase that may dramatically aggravate the initial damage. Hepatotoxicity, as well as hepatic metabolism, is controlled by a set of nuclear receptors (including PXR, CAR, HNF-4α, FXR, LXR, SHP, VDR and PPAR) and signaling pathways. When isolating liver cells, some pathways are activated, e.g., the RAS/MEK/ERK pathway, whereas others are silenced (e.g. HNF-4α), resulting in up- and downregulation of hundreds of genes. An understanding of these changes is crucial for a correct interpretation of in vitro data. The possibilities and limitations of the most useful liver in vitro systems are summarized, including three-dimensional culture techniques, co-cultures with non-parenchymal cells, hepatospheres, precision cut liver slices and the isolated perfused liver. Also discussed is how closely hepatoma, stem cell and iPS cell–derived hepatocyte-like-cells resemble real hepatocytes. Finally, a summary is given of the state of the art of liver in vitro and mathematical modeling systems that are currently used in the pharmaceutical industry with an emphasis on drug metabolism, prediction of clearance, drug interaction, transporter studies and hepatotoxicity. One key message is that despite our enthusiasm for in vitro systems, we must never lose sight of the in vivo situation. Although hepatocytes have been isolated for decades, the hunt for relevant alternative systems has only just begun.Electronic supplementary materialThe online version of this article (doi:10.1007/s00204-013-1078-5) contains supplementary material, which is available to authorized users.

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“…• C for up to 72 hours was high (∼70%), the metabolic function of the cells was approximately half that of freshly isolated cells (Ostrowska et al, 2009). It may be that 'paused' cells would also benefit from a period of recovery after rewarming.…”

Section: Can the Cell Therapy Be Preserved And If So How?mentioning

confidence: 99%

From production to patient: challenges and approaches for delivering cell therapies

Coopman

Medcalf

2014

StemBook

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Hypothermic storage of isolated human hepatocytes: a comparison between University of Wisconsin solution and a hypothermosol platform

Cited by 38 publications

References 45 publications

Supercooling as a Viable Non-Freezing Cell Preservation Method of Rat Hepatocytes

Supercooling as a Viable Non-Freezing Cell Preservation Method of Rat Hepatocytes

Recent advances in 2D and 3D in vitro systems using primary hepatocytes, alternative hepatocyte sources and non-parenchymal liver cells and their use in investigating mechanisms of hepatotoxicity, cell signaling and ADME

From production to patient: challenges and approaches for delivering cell therapies

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