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2-macroglobulin by the
interaction between hepatocytes and endothelial cells in
coculture
Departments of 1 Surgery and 2 Physiology, Johns Hopkins University School of Medicine, Baltimore, Maryland 21287; and 3 Department of Surgery, Washington University School of Medicine, St. Louis, Missouri 63110
The interaction between distinct cell types
within the liver seems to be important in regulating hepatic function.
However, these interactions have not been well characterized because of difficulty in reproducing the hepatic environment in an ex vivo model.
In the present study a coculture system of hepatocytes and endothelial
cells was established to investigate the communication between
parenchymal and nonparenchymal cells. Freshly isolated rat hepatocytes
were placed onto a monolayer of primary aortic rat endothelial cells.
Analysis of the proteins secreted into the extracellular medium after
pulse labeling with radioactive amino acids revealed the presence of a
180,000-apparent molecular weight glycoprotein, BBB-180, which was not
detected in the extracellular medium of hepatocytes or endothelial
cells when they were cultured separately. This glycoprotein was
identified as
2-macroglobulin after sequencing of the proteolytic peptides derived from the purified
protein. This finding was confirmed by Northern and Western blotting,
immunoprecipitation, and RT-PCR. The expression of
2-macroglobulin required direct
contact between hepatocytes and viable endothelial cells. These
findings suggest that endothelial cells modulate hepatocyte gene
expression by direct cellular interactions.
acute phase; liver; cellular communication
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