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Oil Red O Staining: A Technique for Staining Neutral Lipids in Hepatocytes for Detecting Hepatic Steatosis In Vitro

作者：

简介：

Overview

This article discusses hepatic steatosis, a condition marked by fat accumulation in liver cells. It details a method for visualizing lipid droplets using Oil-red-O staining.

Key Study Components

Area of Science

Neuroscience
Cell Biology
Pathology

Background

Hepatic steatosis involves excessive fat in hepatocytes.
Lipid droplets are composed of triglycerides and cholesterol esters.
Understanding fat accumulation is crucial for liver disease research.
Oil-red-O is a dye used to visualize lipid deposits.

Purpose of Study

To demonstrate a method for staining lipid droplets in hepatocytes.
To provide a protocol for researchers studying hepatic steatosis.
To enhance understanding of fat metabolism in liver cells.

Methods Used

Culture hepatocytes in a multi-well plate.
Induce lipid accumulation with a steatogenic medium.
Fix cells with paraformaldehyde and stain with Oil-red-O.
Observe stained cells under a microscope.

Main Results

Lipid droplets appear red after Oil-red-O staining.
The method effectively visualizes fat accumulation in hepatocytes.
Staining allows for assessment of steatosis severity.
Protocol can be replicated for further studies on liver fat metabolism.

Conclusions

Oil-red-O staining is a reliable method for visualizing lipid droplets.
This technique aids in the study of hepatic steatosis.
Understanding lipid accumulation is vital for liver health research.

Frequently Asked Questions

What is hepatic steatosis?

Hepatic steatosis is the accumulation of fats in liver cells, which can lead to liver disease.

How is Oil-red-O used in this study?

Oil-red-O is used to stain lipid droplets in hepatocytes, allowing visualization under a microscope.

What are the key steps in the staining protocol?

The protocol includes fixing cells, staining with Oil-red-O, and observing under a microscope.

Why is it important to study lipid accumulation?

Studying lipid accumulation helps understand metabolic disorders and liver diseases.

What type of cells are used in this experiment?

HepG2 cells, a human liver cancer cell line, are used for the experiment.

What does the red coloration indicate?

The red coloration indicates the presence of lipid droplets within the hepatocytes.

Hepatic steatosis is a pathological condition characterized by an excessive accumulation of fats in hepatocytes - a prominent liver cell type. The fats deposit in the form of lipid droplets of varying sizes in the cytoplasm of the hepatocytes.

Structurally, a lipid droplet contains a core of neutral, hydrophobic fats such as triglycerides and cholesterol esters. The core is surrounded by a phospholipid monolayer decorated with various proteins.

To visualize fat deposition, take a multi-well plate containing an adherent hepatocyte culture. The cells are pretreated with a steatogenic medium to induce lipid droplet accumulation inside them.

Add the desired concentration of paraformaldehyde, which diffuses into the cells, and cross-links the proteins. This step deactivates proteases and preserves the hepatocyte structure. Discard the paraformaldehyde and add the Oil-red-O solution containing the organic dye dissolved in isopropanol.

The isopropanol acts as a carrier solvent for the sparingly soluble Oil-red-O molecules. This helps the dye molecules to enter fixed hepatocytes and eventually reach the lipid droplets. Once inside, the dye transfers from the isopropanol to neutral lipids due to its higher affinity, forming the dye-lipid complex. This result in red coloration of lipid droplets.

Discard the excess dye and observe the cells under a microscope. The intracellular lipid droplets appear intensely red.

Put a cell culture coverslip in every well in a 24-well plate, and seed HepG2 cells, as described in the text manuscript. After the appropriate incubation, wash the cells with 1 milliliter of PBS, and discard the supernatant. Fix them with 1 milliliter of 4% paraformaldehyde in PBS, and incubate for 1 hour at room temperature. Discard the excess paraformaldehyde, and rinse the cells with 1 milliliter of distilled water.

Then, add 1 milliliter of 70% isopropanol, and incubate for 5 minutes. Discard the excess isopropanol, and add 1 milliliter of Oil-red O solution, and incubate for 30 minutes. Discard the excess Oil-red O solution, and then, rinse with 1 milliliter of distilled water. Observe the cells under the microscope at a magnification of 400x.

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