Screening for Chemical Toxicity Using Cryopreserved Precision Cut Lung Slices
Author(s) -
Christa Watson,
F Damiani,
Sumati RamMohan,
Sylvia Rodrigues,
Priscila de Moura Queiroz,
Thomas C. Donaghey,
Jamie H. Rosenblum Lichtenstein,
Joseph D. Brain,
Ramaswamy Krishnan,
Ramon M. Molina
Publication year - 2015
Publication title -
toxicological sciences
Language(s) - Uncategorized
Resource type - Journals
SCImago Journal Rank - 1.352
H-Index - 183
eISSN - 1096-6080
pISSN - 1096-0929
DOI - 10.1093/toxsci/kfv320
Subject(s) - cryopreservation , viability assay , toxicity , in vivo , chemistry , glutathione , cell , andrology , biology , microbiology and biotechnology , biochemistry , embryo , medicine , enzyme , organic chemistry
To assess chemical toxicity, current high throughput screening (HTS) assays rely primarily on in vitro measurements using cultured cells. Responses frequently differ from in vivo results due to the lack of physical and humoral interactions provided by the extracellular matrix, cell-cell interactions, and other molecular components of the native organ. To more accurately reproduce organ complexity in HTS, we developed an organotypic assay using the cryopreserved precision cut lung slice (PCLS) from rats and mice. Compared to the never-frozen PCLS, their frozen-thawed counterpart slices showed viability or metabolic activity that is decreased to an extent comparable to that observed in other cryopreserved cells and tissues, but shows no differences in further changes in cell viability, mitochondrial integrity, and glutathione activity in response to the model toxin zinc chloride (ZnCl2). Notably, these measurements were successfully miniaturized so as to establish HTS capacity in a 96-well plate format. Finally, PCLS responses correlated with common markers of lung injury measured in lavage fluid from rats intratracheally instilled with ZnCl2. In summary, we establish that the cryopreserved PCLS is a feasible approach for HTS investigations in predictive toxicology.
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