Primary cultures of rabbit renal proximal tubule cells: I. Growth and biochemical characteristics |
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Authors: | Michael D. Aleo Mary L. Taub Peter A. Nickerson Paul J. Kostyniak |
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Affiliation: | (1) Department of Pharmacology & Therapeutic, Toxicology Research Center, State University of New York at Buffalo, 102 Faber Hall, 14214 Buffalo, New York;(2) Department of Biochemistry, State University of New York at Buffalo, 102 Farber Hall, 14214 Buffalo, New York;(3) Department of Pathology, State University of New York at Buffalo, 102 Farber Hall, 14214 Buffalo, New York |
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Abstract: | Summay Before the usefulness of a new in vitro model can be ascertained, the model must be properly defined and characterized. This study presents the growth rate and biochemical characteristics of rabbit renal proximal tubule cells in primary culture over a 2-wk culture period. When grown in a hormonally defined, antibiotic-free medium these cells form confluent monolayer cultures within 7 d after plating. Multicellular done formation, an indicator of transepithelial solute transport, was expressed after confluent cultures were formed. The activity of the cytosolic enzyme, lactate dehydrogenase, and the lysosomal enzyme,N-acetyl-glucosaminidase, increased 14- and 2-fold during the first 8 d of culture. respectively. In contrast, the activity of a brush border enzyme, alkaline phosphatase, decreased 85% within the first 8 d of culture. Release of these enzyme markers into the culture medium, which are routinely used to measure cytoxicity, stabilized after 8 d in culture. The ratio of cellular protein to DNA changed according to the state of cellular growth. Values rose from 0.035 mg protein/μg DNA in preconfluent cultures to 0.059 mg protein/μg DNA in confluent cultures. These results document the characteristics of a primary proximal tubule cell culture system for future studies in in vitro toxicology. This paper was resented at a Symposium on the Physiology and Toxicology of the Kidney In Vitro co-sponsored by The Society of Toxicology (SOT) and the Tissue Culture Association held at the 27th annual meeting of the SOT in Dallas, Texas in 1988. This work was supported by grants GM 07145, The Johns Hopkins Center for Alternatives to Animal Testing, and a Sigma Xi Grants-in-Aid of Research Award. |
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Keywords: | proximal tubules primary culture hormonally defined medium lactate dehydrogenase N-acetyl-glucosaminidase alkaline phosphosphatase deoxyribonucleic acid |
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