Transfecting RAW264.7 Cells with a Luciferase Reporter Gene

作者： Sylvia T. Cheung1,2,3, Soroush Shakibakho1,2, Eva Y. So1,2, Alice L-F Mui1,2,3 1Immunity and Infection Research Centre,Vancouver Costal Health Research Institute, 2Department of Surgery,University of British Columbia, 3Department of Biochemistry and Molecular Biology,University of British Columbia

简介：

Overview

This article presents a robust procedure for transfecting luciferase reporter genes into the RAW264.7 macrophage cell line without triggering the cell's natural defense mechanisms. The method involves careful handling and specific plasmid requirements to ensure successful transfection.

Key Study Components

Area of Science

• Cell Biology
• Transfection Techniques
• Macrophage Research

Background

• RAW264.7 cells are known for their resistance to foreign materials.
• Transfection in these cells is challenging due to their immune response.
• Luciferase reporter genes are commonly used for gene expression studies.
• Endotoxin-free plasmids are crucial for successful transfection.

Purpose of Study

• To develop a gentle transfection method for RAW264.7 cells.
• To enable the study of gene expression without activating immune responses.
• To facilitate the use of luciferase assays in macrophage research.

Methods Used

• Harvesting RAW264.7 cells through gentle pipetting.
• Seeding cells into a 24-well tissue culture plate.
• Cotransfecting Firefly and Renilla luciferase plasmids.
• Assaying luciferase activity after cell lysis.

Main Results

• Successfully transfected RAW264.7 cells without activating them.
• Demonstrated reliable luciferase activity measurement.
• Established a protocol for future studies involving macrophages.
• Provided insights into the transfection process for immune cells.

Conclusions

• The developed method is effective for transfecting RAW264.7 cells.
• This approach can enhance research on macrophage biology.
• Future applications may include various treatments and assays.

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