Home
Our Research
Education
Shared Resources
Patient Care
You Are Here:
Shared Resources
Registration
Biorepository and Tissue Technology
Biostatistics
Flow Cytometry
Genomics and Computational Biology
In Vivo Imaging
Microscopy
Radiation Medicine
Transgenic Mouse
Biobehavioral Shared Resource
Clinical Trials Resources for Researchers
Skip to Main Navigation
Skip to Main Content
Search this site
Search all sites
Search
Toggle navigation
Search
Search this site
Search all sites
Home
Our Research
Centers and Select Labs
Patel Lab
San Diego Center for Precision Immunotherapy (SDCPI)
Education
Cancer Therapeutics Training (CT2) Program
Program Overview
CT2 Program Faculty
Requirements
Application Information
Contact
CT2 Lecture Series
Current Fellows
OPTIMUS
Program Details
Apply
Meet the Team
Contact Us
Alumni
Donate
Our Supporters
Events Calendar
Shared Resources
Currently selected
Registration
Biorepository and Tissue Technology
Tissue Technology Shared Resource
Service Profile
How to request
Policies
Forms
Recharges
Biostatistics
Flow Cytometry
Service Details
Protocols
Rates
Bibliography
Genomics and Computational Biology
In Vivo Imaging
Computed Tomography
Positron Emission Tomography
Optical Imaging
BioSpace Gamma Imager
High-Resolution Ultrasound
High-Resolution Tissue Imaging
Image Processing / Kinetic Modeling
Radiochemistry
Magnetic Resonance Imaging
Fluorescence Imaging
Photoacoustic Imaging - Ultrasound Imaging
Microscopy
Scheduling
Rates
Equipment and Services
Protocols
Publications
Microscopy Links
Radiation Medicine
Transgenic Mouse
Getting Started
Services and Rates
Helpful Links
Biobehavioral Shared Resource
Clinical Trials Resources for Researchers
Patient Care
Moores Cancer Center
Research and Training
School of Medicine
/
Research
/
Moores Cancer Center
/
Shared Resources
/
Flow Cytometry
/
Protocols
/
Ethidium Monoazide (EMA)
Additional Navigation
Shared Resources
Registration
Biorepository and Tissue Technology
Tissue Technology Shared Resource
Service Profile
How to request
Policies
Forms
Recharges
Biostatistics
Flow Cytometry
Service Details
Protocols
7-AAD on Fixed Cells
DNA Content of Adherent Cells
Basic Antibody Staining
Apoptosis with PI Only
Cell Cycle with PI
DNAse I
Ethidium Monoazide (EMA)
Currently selected
GFP and DNA
Isolated Nuclei DNA Staining
Nuclear Antigens and DNA
Surface Antigens and DNA
Sorting Checklist
Antibody Titration
SYTOX Green
SYBR Green I
20X Phosphate Buffered Saline (PBS)
Erythrocyte Lysis
Dextran Sedimentation of Erythrocytes
Paraformaldehyde Fixative
Rates
Bibliography
Genomics and Computational Biology
In Vivo Imaging
Computed Tomography
Positron Emission Tomography
Optical Imaging
BioSpace Gamma Imager
High-Resolution Ultrasound
High-Resolution Tissue Imaging
Image Processing / Kinetic Modeling
Radiochemistry
Magnetic Resonance Imaging
Fluorescence Imaging
Photoacoustic Imaging - Ultrasound Imaging
Microscopy
Scheduling
Rates
Equipment and Services
Protocols
Publications
Microscopy Links
Radiation Medicine
Transgenic Mouse
Getting Started
Forms and Protocols
Services and Rates
Service Descriptions
Helpful Links
Biobehavioral Shared Resource
Clinical Trials Resources for Researchers
Ethidium Monoazide (EMA)
Page Content
Adapted from Kathrine A. Muirhead
Zynaxis Cell Science, Inc.
Use ethidium monoazide (EMA) that has been titered (0.5 ug/ml - 10 ug/ml) and compared to trypan blue exclusion and/or propidium iodide (PI = 0.5 ug/ml). Viable cells should have low background EMA staining.
Wash cells twice in phosphate buffered saline (PBS) containing 0.5% to 5% bovine serum albumin (BSA) and 0.1% sodium azide (NaN
3
).
Resuspend cells to 10
7
per ml.
Add 50 ul cells and appropriate volume of buffer to give 90 ul in 96-well plate or 12 x 75 mm tubes. Add sufficient EMA stock to each well or tube for the final concentration (as determined above) and mix well. (eg 10 ul of 100 ug/ml EMA in PBS).
Incubate IN THE DARK on ice for 15 minutes to allow uptake of EMA by dead cells.
Continue incubating ON ICE for 15 minutes 30 cm from fluorescenct light source to photoactivate EMA and cause covalent binding.
Add appropriate amount of monoclonal antibodies and incubate 15 - 30 minutes on ice in the dark.
Wash twice with wash buffer (eg PBS-BSA-NaN
3
).
Fix cells with 0.5% final concentration protein-free buffered paraformaldehyde (PFA) and store at 4°C IN DARK.