Quantitative Immunofluorescence to Measure Global Localized Translation

Jonathan Bergeman; Marc-&#201;tienne Huot

doi:10.3791/55909

Quantitative Immunofluorescence to Measure Global Localized Translation

JoVE Journal
Biochemistry

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JoVE Journal Biochemistry

Quantitative Immunofluorescence to Measure Global Localized Translation

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09:13 min

August 22, 2017

DOI: 10.3791/55909-v

Jonathan Bergeman¹, Marc-Étienne Huot^1,2

¹Centre de Recherche sur le Cancer de l’Université Laval, Faculté de Médecine, Département de Biologie moléculaire, biochimie médicale et pathologie,Université Laval, ²CRCHU de Québec: L’Hôtel-Dieu de Québec

Overview

This manuscript describes a method to visualize and quantify localized translation events in subcellular compartments during cell adhesion. The approach is rapid, cost-effective, and requires only basic confocal imaging systems and specific reagents.

Key Study Components

Area of Science

Neuroscience
Cell Biology
Imaging Techniques

Background

Localized translation events are crucial for understanding cellular processes.
Cell adhesion is a key step in various biological functions.
Existing methods may lack efficiency or accessibility.
This study aims to provide a straightforward alternative.

Purpose of Study

To visualize compartmentalized translation events.
To quantify translation during cell adhesion.
To develop a method that is easy and cost-effective.

Methods Used

Use of puromycin to label newly synthesized proteins.
Application of antibodies directed against puromycin.
Utilization of a standard confocal imaging system.
Preparation of MRC-5 cell suspensions for experimentation.

Main Results

The method allows for rapid assessment of translation events.
It demonstrates effectiveness in analyzing cell migration and adhesion.
Results indicate a clear visualization of localized translation.
The technique is applicable in early drug response studies.

Conclusions

This method offers a practical approach to study translation in cells.
It enhances understanding of cellular responses during adhesion.
The technique is beneficial for various research applications.

Frequently Asked Questions

What is the main advantage of this method?

The method is easy, rapid, and cost-effective.

What reagents are required for this technique?

Only puromycin and specific antibodies are needed.

Can this method be used for drug response studies?

Yes, it is applicable for analyzing early drug responses.

What type of imaging system is necessary?

A standard confocal imaging system is sufficient.

Which cell type is used in this study?

MRC-5 cells are used for the experiments.

Is this method suitable for studying cell migration?

Yes, it can be used to analyze cell migration events.

This manuscript describes a method to visualize and quantify localized translation events in subcellular compartments. The approach proposed in this manuscript requires a basic confocal imaging system and reagents and is rapid and cost-effective.

The overall goal of this experiment is to visualize and quantify compartmentalized translation events taking place during the initial steps of cell adhesion. This method has broad application. Use it whenever rapid specific translation response might be assay such as when analyzing cell migration, adhesion, or early drug response.

The main advantage of this technique are that, it is easy, rapid, and cost-effective. It only requires puromycin, antibodies directed against puromycin, and the standard confocal scan imaging system. To begin, make a suspension of MRC-5 cells.

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Quantitative Immunofluorescence Localized Translation Cell Adhesion Puromycin Anti-puromycin Antibody Fluorophore-conjugated Secondary Antibodies Cell Migration Cell Adhesion Early Drug Response MRC-5 Cells Cycloheximide Formaldehyde Fixation Triton X-100 Permeabilization BSA Blocking Tween-20 Washing