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The hepatocyte proteome in organotypic rat liver models and the influence of the local microenvironment
Authors:Lucas T Vu  Sophia M Orbach  W Keith Ray  Margaret E Cassin  Padmavathy Rajagopalan  Richard F Helm
Institution:1.Department of Chemical Engineering,Virginia Tech,Blacksburg,USA;2.Department of Biochemistry,Virginia Tech,Blacksburg,USA;3.School of Biomedical Engineering and Sciences,Virginia Tech,Blacksburg,USA;4.ICTAS Center for Systems Biology and Engineered Tissues,Virginia Tech,Blacksburg,USA
Abstract:

Background

Liver models that closely mimic the in vivo microenvironment are useful for understanding liver functions, capabilities, and intercellular communication processes. Three-dimensional (3D) liver models assembled using hepatocytes and liver sinusoidal endothelial cells (LSECs) separated by a polyelectrolyte multilayer (PEM) provide a functional system while also permitting isolation of individual cell types for proteomic analyses.

Methods

To better understand the mechanisms and processes that underlie liver model function, hepatocytes were maintained as monolayers and 3D PEM-based formats in the presence or absence of primary LSECs. The resulting hepatocyte proteomes, the proteins in the PEM, and extracellular levels of urea, albumin and glucose after three days of culture were compared.

Results

All systems were ketogenic and found to release glucose. The presence of the PEM led to increases in proteins associated with both mitochondrial and peroxisomal-based β-oxidation. The PEMs also limited production of structural and migratory proteins associated with dedifferentiation. The presence of LSECs increased levels of Phase I and Phase II biotransformation enzymes as well as several proteins associated with the endoplasmic reticulum and extracellular matrix remodeling. The proteomic analysis of the PEMs indicated that there was no significant change after three days of culture. These results are discussed in relation to liver model function.

Conclusions

Heterotypic cell-cell and cell-ECM interactions exert different effects on hepatocyte functions and phenotypes.
Keywords:
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