Hepatic stellate cells are a
significant type of cell which causes liver fibrosis in fibrogenic myofibroblast
cells. It is followed by activation in conditions such as chronic alcohol
abuse, hepatitis B, hyperlipidemia, obesity, and diabetes. Renewable cell
culture models are increasingly needed to faithfully encapsulate there in vivo
phénotype, particularly for clinical trials.
Much of the current knowledge of
stellate cell behavior is acquired through animal studies and primary culture
studies, especially from rats. Cultivated on uncoated plastic, star cells are
spontaneously triggered strongly linked to their reaction in vivo.
However, pathways elucidated by
mouse models of human hepatic stellate
cells must be tested to show their importance to human disease.
Structure
Gold chloride can exclusively stain
endothelial cells, but its distinguishing characteristic in standard x-ray
preparations is the inclusion of multiple adipocytes in their cytoplasm.
Some Other Names
Before we proceed to explore more
about human hepatic stellate cells, let’s
first, know some other names of these cells.
·
Perisinusoidal Cells
·
Ito Cells
·
Hepatic Lipocytes
·
Hepatic Pericytes
Limitations of Human Hepatic
Stellate Cells
The unusual and unexpected amount
of human tissue suitable for cell isolation and the small yield and often
impurities that characterize these isolates has been a significant limitation
of the use of human stellate cells.
One Possible Solution
One solution to solving these
problems was to transfer fibroblast-like outgrowths from whole tissue regions,
typically representing a heterogeneous mixture of HSCs stimulated with certain
forms of hepatic cells which include large endothelial and vascular smooth
muscle cells.
In addition to variability, the
effectiveness of explant outgrowths is restricted by the finite amount of
passages that cells experience until immortalized. Besides, human liver
isolates differ from ready to prepared, rendering clear comparisons between
findings challenging.
Isolation Methods
An accurate way of separating HSC
and explicitly classifying HSCs is crucial for a complete knowledge of its
human liver physiology and liver disease function. Two primary methods to
isolate HSCs from human liver have been described so far: one is to develop
smooth musculature-like cells from liver tissue explants and the other is to
use density gradient centrifugation similar to HSC isolation in rodents.
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