These studies demonstrate that the MH1C1 strain of rat hepatoma cells has the ability to take up and conjugate bilirubin and then excrete the conjugated pigment into the culture medium. On incubation with unconjugated bilirubin, the average rate of appearance of conjugated bilirubin in the medium was 4.4 ± 0.20 µg per mg of cell protein per hour (mean ± SE). The products formed from bilirubin by MH1C1 cells were chromatographically identical to those found in normal rat bile. Assay of bilirubin UDP glucuronyl transferase activity in homogenates of MH1C1 cells gave a value of 3.3 ± 0.50 µg of conjugated pigment formed per mg protein per hour, only moderately less than the enzyme activity of liver from normal rats. Rat fibroblasts in culture did not conjugate bilirubin, nor did they contain bilirubin UDP-glucuronyl transferase activity. As in living animals, flavaspidic acid inhibited bilirubin metabolism by MH1C1 cells, suggesting that the mechanism for bilirubin uptake is similar to that of normal liver. In contrast to the findings in animals, however, preincubation of MH1C1 cells with phenobarbital led to only minimal enhancement of pigment conjugation. MH1C1 cells represent the first example of a clonal strain of cells in culture in which many of the pathways of hepatic bilirubin metabolism remain intact. They should, therefore, serve as a useful model for studies of bile pigment metabolism which are not easily performed in the living animal.
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1 December 1970
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December 01 1970
METABOLISM OF BILIRUBIN BY A CLONAL STRAIN OF RAT HEPATOMA CELLS
Hans E. Rugstad,
Hans E. Rugstad
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
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Stephen H. Robinson,
Stephen H. Robinson
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
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Claudine Yannoni,
Claudine Yannoni
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
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Armen H. Tashjian, Jr.
Armen H. Tashjian, Jr.
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
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Hans E. Rugstad
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
Stephen H. Robinson
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
Claudine Yannoni
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
Armen H. Tashjian, Jr.
From the Pharmacology Department, Harvard School of Dental Medicine; the Department of Pharmacology, Harvard Medical School; and the Department of Medicine, Beth Israel Hospital and Harvard Medical School, Boston, Massachusetts 02115
Received:
April 20 1970
Revision Received:
June 15 1970
Online ISSN: 1540-8140
Print ISSN: 0021-9525
Copyright © 1970 by The Rockefeller University Press
1970
J Cell Biol (1970) 47 (3): 703–710.
Article history
Received:
April 20 1970
Revision Received:
June 15 1970
Citation
Hans E. Rugstad, Stephen H. Robinson, Claudine Yannoni, Armen H. Tashjian; METABOLISM OF BILIRUBIN BY A CLONAL STRAIN OF RAT HEPATOMA CELLS . J Cell Biol 1 December 1970; 47 (3): 703–710. doi: https://doi.org/10.1083/jcb.47.3.703
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