TY - JOUR
T1 - Assessment of a new cell culture perfusion apparatus for in vitro chronic toxicity testing part 2
T2 - Toxicological evaluation
AU - Jennings, Paul
AU - Koppelstaetter, Christian
AU - Pfaller, Walter
AU - Morin, Jean Paul
AU - Hartung, Thomas
AU - Ryan, Michael P.
PY - 2004
Y1 - 2004
N2 - The goal of replacement, refinement and reduction of animal testing is critically dependent on the development and assessment of novel in vitro methodologies and the further development of existing methodologies. Here, we evaluated the use of a modified perfusion cell culture apparatus for application to chronic in vitro nephrotoxicity testing using DMSO, SDS, paracetamol and cyclosporine A as test compounds. Renal epithelial monolayers were cultured on microporous growth supports and exposed to test compounds under static or perfusion conditions. Alamar Blue reduction, gamma-glutamyl transpeptidase activity (GGT), lactate dehydrogenase activity (LDH) and remnant protein were used to assay cell toxicity. There was no significant difference in IC50 values between static and perfusion cultures up to 72 hours exposure. However, the perfusion system allowed continuous real-time monitoring of plasma membrane damage, which gives important information of time, duration and scale of toxicity. The complexity of the system restrains its use to low-throughput analysis. However the real and theoretical advantages of this and similar systems merit further investigations.
AB - The goal of replacement, refinement and reduction of animal testing is critically dependent on the development and assessment of novel in vitro methodologies and the further development of existing methodologies. Here, we evaluated the use of a modified perfusion cell culture apparatus for application to chronic in vitro nephrotoxicity testing using DMSO, SDS, paracetamol and cyclosporine A as test compounds. Renal epithelial monolayers were cultured on microporous growth supports and exposed to test compounds under static or perfusion conditions. Alamar Blue reduction, gamma-glutamyl transpeptidase activity (GGT), lactate dehydrogenase activity (LDH) and remnant protein were used to assay cell toxicity. There was no significant difference in IC50 values between static and perfusion cultures up to 72 hours exposure. However, the perfusion system allowed continuous real-time monitoring of plasma membrane damage, which gives important information of time, duration and scale of toxicity. The complexity of the system restrains its use to low-throughput analysis. However the real and theoretical advantages of this and similar systems merit further investigations.
KW - Cell culture
KW - Chronic
KW - Cyclosporine A
KW - DMSO
KW - Paracetamol
KW - Perfusion
KW - Toxicity
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M3 - Article
C2 - 15195226
AN - SCOPUS:3242777028
SN - 0946-7785
VL - 21
SP - 61
EP - 66
JO - ALTEX. Alternativen zu Tierexperimenten
JF - ALTEX. Alternativen zu Tierexperimenten
IS - 2
ER -