Albumin promotes proliferation of G1 arrested serum starved hepatocellular carcinoma cells

Badr Ibrahim; Jan Stange; Adrian Dominik; Martin Sauer; Sandra Doss; Martin Eggert

doi:10.7717/peerj.8568

PeerJ (Mar 2020)

Albumin promotes proliferation of G1 arrested serum starved hepatocellular carcinoma cells

Badr Ibrahim,
Jan Stange,
Adrian Dominik,
Martin Sauer,
Sandra Doss,
Martin Eggert

Affiliations

Badr Ibrahim: Division of Nephrology/ Department of Internal Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany
Jan Stange: Division of Nephrology/ Department of Internal Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany
Adrian Dominik: Division of Nephrology/ Department of Internal Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany
Martin Sauer: Department of Anaesthesiology and Intensive Care Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany
Sandra Doss: Division of Nephrology/ Department of Internal Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany
Martin Eggert: Division of Nephrology/ Department of Internal Medicine, University Hospital Rostock, Rostock, Mecklenburg Verpommern, Germany

DOI: https://doi.org/10.7717/peerj.8568
Journal volume & issue: Vol. 8
p. e8568

Abstract

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Albumin is the most abundant plasma protein and functions as a transport molecule that continuously interacts with various cell types. Because of these properties, albumin has been exploited by the pharmaceutical industry to improve drug delivery into target cells. The immediate effects of albumin on cells, however, require further understanding. The cell interacting properties and pharmaceutical applications of albumin incentivises continual research into the immediate effects of albumin on cells. The HepG2/C3A hepatocellular carcinoma cell line is used as a model for studying cancer pathology as well as liver biosynthesis and cellular responses to drugs. Here we investigated the direct effect of purified albumin on HepG2/C3A cell proliferation in the absence of serum, growth factors and other serum originating albumin bound molecules. We observed that the reduced cell counts in serum starved HepG2/C3A cultures were increased by the inclusion of albumin. Cell cycle analysis demonstrated that the percentage of cells in G1 phase during serum starvation was reduced from 86.4 ± 2.3% to 78.3 ± 3.2% by the inclusion of albumin whereas the percentage of cells in S phase was increased from 6.5 ± 1.5% to 14.3 ± 3.6%. A significant reduction in the cell cycle inhibitor protein, P21, accompanied the changes in the proportions of cell cycle phases upon treatment with albumin. We have also observed that the levels of dead cells determined by DNA fragmentation and membrane permeabilization caused by serum starvation (TUNEL: 16.6 ± 7.2%, ethidium bromide: 13.8 ± 4.8%) were not significantly altered by the inclusion of albumin (11.6 ± 10.2%, ethidium bromide: 16.9 ± 8.9%). Therefore, the increase in cell number was mainly caused by albumin promoting proliferation rather than protection against cell death. These primary findings demonstrate that albumin has immediate effects on HepG2/C3A hepatocellular carcinoma cells. These effects should be taken into consideration when studying the effects of albumin bound drugs or pathological ligands bound to albumin on HepG2/C3A cells.

Published in PeerJ

ISSN: 2167-8359 (Online)
Publisher: PeerJ Inc.
Country of publisher: United States
LCC subjects: Medicine; Science: Biology (General)
Website: https://peerj.com/

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