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Cloning and Stem Cells
Human Embryonic Stem Cells Passaged Using Enzymatic Methods Retain a Normal Karyotype and Express CD30

To cite this article:
Alison Thomson, Davina Wojtacha, Zoë Hewitt, Helen Priddle, Virginie Sottile, Alex Di Domenico, Judy Fletcher, Martin Waterfall, Néstor López Corrales, Ray Ansell, Jim McWhir. Cloning and Stem Cells. March 2008, 10(1): 89-106. doi:10.1089/clo.2007.0072.

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Alison Thomson 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Davina Wojtacha 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Zoë Hewitt 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Centre for Stem Cell Biology, The University of Sheffield, Alfred Denny Building, Western Bank, Sheffield, S10 2TN, UK.
Helen Priddle 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
D Floor East Block, Queen's Medical Centre, University of Nottingham, Nottingham, NG7 2UH, UK.
Virginie Sottile 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Institute of Genetics, Queen's Medical Centre, University of Nottingham, Nottingham, NG7 2UH, UK.
Alex Di Domenico 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Judy Fletcher 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Centre for Regenerative Medicine, University of Edinburgh, 49 Little France Crescent, Edinburgh, EH16 4SB, UK.
Martin Waterfall 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Néstor López Corrales 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Public University of Navarra, Department of Agriculture, Edif. Los Olivos, Campus de Arrosadía 31006, Pamplona, Spain.
Ray Ansell 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.
Jim McWhir 
Division of Gene Function and Development, Roslin Institute, Roslin, Midlothian, Scotland.

Human embryonic stem cells (hESCs) are thought to be susceptible to chromosomal rearrangements as a consequence of single cell dissociation. Compared in this study are two methods of dissociation that do not generate single cell suspensions (collagenase and EDTA) with an enzymatic procedure using trypsin combined with the calcium-specific chelator EGTA (TEG), that does generate a single cell suspension, over 10 passages. Cells passaged by single cell dissociation using TEG retained a normal karyotype. However, cells passaged using EDTA, without trypsin, acquired an isochromosome p7 in three replicates of one experiment. In all of the TEG, collagenase and EDTA-treated cultures, cells retained consistent telomere length and potentiality, demonstrating that single cell dissociation can be used to maintain karyotypically and phenotypically normal hESCs. However, competitive genomic hybridization revealed that subkaryotypic deletions and amplifications could accumulate over time, reinforcing that present culture regimes remain suboptimal. In all cultures the cell surface marker CD30, reportedly expressed on embryonal carcinoma but not karyoptically normal ESCs, was expressed on hESCs with both normal and abnormal karyotype, but was upregulated on the latter.

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