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dc.contributor.authorKyffin, Jonathan A.
dc.contributor.authorCox, Christopher R.
dc.contributor.authorLeedale, Joseph
dc.contributor.authorColley, Helen E.
dc.contributor.authorMurdoch, Craig
dc.contributor.authorMistry, Pratibha
dc.contributor.authorWebb, Steven D.
dc.contributor.authorSharma, Parveen
dc.date.accessioned2019-10-02T01:30:57Z
dc.date.available2019-10-02T01:30:57Z
dc.date.issued2019-09-13
dc.identifierhttps://chesterrep.openrepository.com/bitstream/handle/10034/622663/CP%20Toxicology%20-%20Kyffin%20-%20Preparation%20of%20Primary%20Rat%20Hepatocyte%20Spheroids.pdf?sequence=2
dc.identifier.citationKyffin, J. A., Cox, C. R., Leedale, J., Colley, H. E., Murdoch, C., Mistry, P., Webb, S. D., & Sharma, P. (2019). Preparation of primary rat hepatocyte spheroids utilizing the liquid-overlay technique. Current Protocols in Toxicology, 81(1), e87. https://doi.org/10.1002/cptx.87
dc.identifier.issn1934-9254
dc.identifier.doi10.1002/cptx.87
dc.identifier.urihttp://hdl.handle.net/10034/622663
dc.description.abstractHerein, we describe a protocol for the preparation and analysis of primary isolated rat hepatocytes in a 3D cell culture format described as spheroids. The hepatocyte cells spontaneously self-aggregate into spheroids without the need for synthetic extracellular matrices or hydrogels. Primary rat hepatocytes (PRHs) are a readily available source of primary differentiated liver cells and therefore conserve many of the required liver-specific functional markers, and elicit the natural in vivo phenotype when compared with common hepatic cells lines. We describe the liquid-overlay technique which provides an ultra-low attachment surface on which PRHs can be cultured as spheroids. © 2019 The Authors. Basic Protocol 1: Preparation of agarose-coated plates Basic Protocol 2: Primary rat hepatocyte isolation procedure Basic Protocol 3: Primary rat hepatocyte spheroid culture Basic Protocol 4: Immunofluorescent analysis of PRH spheroids. [Abstract copyright: © 2019 The Authors.]
dc.languageeng
dc.publisherWiley-Blackwell
dc.relation.urlhttps://currentprotocols.onlinelibrary.wiley.com/doi/10.1002/cptx.87
dc.rights.urihttps://creativecommons.org/licenses/by/4.0/
dc.sourceeissn: 1934-9262
dc.subjectbile canaliculi
dc.subjectimmunofluorescence
dc.subjectliquid-overlay technique
dc.subjectliver spheroids
dc.subjectprimary rat hepatocytes
dc.titlePreparation of Primary Rat Hepatocyte Spheroids Utilizing the Liquid-Overlay Technique
dc.typeArticle
dc.identifier.eissn1934-9262
dc.contributor.departmentUniversity of Liverpool; University of Chester; University of Sheffield; Syngenta Ltd; Liverpool John Moores University
dc.identifier.journalCurrent Protocols in Toxicology
dc.date.updated2019-10-02T01:30:57Z
rioxxterms.funderBBSRC; Grant(s): BB/M503435/1
rioxxterms.funderMRC Skills Development Fellowship; Grant(s): MR/S019332/1
rioxxterms.funderUniversity of Liverpool
rioxxterms.funderMRC
rioxxterms.funderLiverpool Centre for Mathematics in Healthcare
rioxxterms.funderEPSRC; Grant(s): EP/N014499/1
rioxxterms.versionofrecordhttps://doi.org/10.1002/cptx.87


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