Annexin V

iFluor® 750

Annexins are a family of proteins that bind to phospholipid membranes in the presence of calcium. Annexin V is a valuable tool for studying cell apoptosis. It is used as a probe to detect cells which have expressed phosphatidylserine on the cell surface, a feature found in apoptosis as well as other forms of cell death. There are a variety of parameters that can be used for monitoring cell viability. Annexin V-dye conjugates are widely used to monitor cell apoptosis through measuring the translocation of phosphatidylserine (PS). In apoptosis, PS is transferred to the outer leaflet of the plasma membrane. The appearance of phosphatidylserine on the cell surface is a universal indicator of the initial/intermediate stages of cell apoptosis and can be detected before morphological changes can be observed. This fluorescent Annexin V conjugate has spectral properties similar to Alexa Fluor® 750 (Alexa Fluor® 750 is the trademark of Invitrogen) and Cy7® (Cy7® is the trademark of GE Healthcare).

Example protocol

AT A GLANCE

Protocol Summary

Prepare cells with test compounds (200 µL/sample).
Add Annexin V conjugate assay solution.
Incubate at room temperature for 30-60 minutes.
Analyze with a flow cytometer or a fluorescence microscope.

Storage and Handling Conditions

The fluorescent annexin V conjugates are stored in a PBS buffer solution containing 0.1% bovine serum albumin (BSA) with a pH of 7.4. To ensure their stability, it is recommended that the solutions be stored at a temperature of -20°C and protected from light. Avoid exposing the fluorescent conjugates to repeated freeze-thaw cycles as this can have a negative effect on their integrity. These solutions can be stored for at least 6 months under the recommended conditions.

SAMPLE EXPERIMENTAL PROTOCOL

Prepare and Incubate Cells with Annexin V Conjugate

Prepare an Annexin V-binding assay buffer: 10 mM HEPES, 140 mM NaCl, and 2.5 mM CaCl2, pH 7.4.
Treat cells with test compounds for a desired period of time (e.g., 4-6 hours for Jurkat cells treated with staurosporine) to induce apoptosis.
Centrifuge the cells to get 1-5×10⁵ cells/tube.
Resuspend cells in 200 μL of the Annexin V-binding assay buffer from Step 1.
Add 2 μL of the Annexin V conjugate to the cells.

Optional: Add a dead cell stain such as Nuclear Green™ DCS1 (Cat No. 17550) into the cells for necrosis cells.
Incubate at room temperature for 30 to 60 minutes, protected from light.
Add 300 μL of the Annexin V-binding assay buffer (from Step 1) to increase volume before analyzing the cells with
a flow cytometer or fluorescence microscope.
Monitor the fluorescence intensity by using a flow cytometer or a fluorescence microscope.

Flow Cytometer Protocol

Quantify Annexin V conjugates binding by using a flow cytometer with appropriate filters.

Note: It is not common to perform Annexin V binding flow cytometric analysis on adherent cells due to the possibility of membrane damage during cell detachment or harvesting. However, previous studies by Casiola-Rosen et al. and van Engelend et al. (refer to Refs 1 and 2) have demonstrated methods for using Annexin V in flow cytometry on adherent cell types.

Fluorescence Microscope Protocol

Pipette the cell suspension from Step 6, rinse 1-2 times with Annexin V-binding assay buffer (Step 1), and then resuspend the cells with the Annexin V-binding assay buffer (Step 1).
Add the cells on a glass slide that is covered with a glass cover slip.

Note: For adherent cells, it is recommended to grow the cells directly on a cover slip.
After incubation with Annexin V conjugate (Step 6), rinse 1-2 times with Annexin V-binding assay buffer (Step 1), and add
Annexin V-binding assay buffer (Step 1) back to the cover slip.
Invert the cover slip on a glass slide and visualize the cells. The cells can also be fixed in 2% formaldehyde after incubation with Annexin V conjugate and visualized under a microscope with the appropriate filter set.

APPENDIX

References

Pascal Clerc, Pauline Jeanjean, Nicolas Halalli, Michel Gougeon, Bernard Pipy, Julian Carrey, Daniel Fourmy, Véronique Gigoux. Journal of Controlled Release (2017).
Hanshaw RG, Lakshmi C, Lambert TN, Johnson JR, Smith BD. Chembiochem, 6, 2214. (2005).

Spectrum

Open in Advanced Spectrum Viewer

Product family

Name	Excitation (nm)	Emission (nm)	Extinction coefficient (cm ^-1 M ^-1)	Quantum yield	Correction Factor (260 nm)	Correction Factor (280 nm)
Annexin V-iFluor® 633 conjugate	640	654	250000¹	0.29¹	0.062	0.044
Annexin V-iFluor® 350 conjugate	345	450	20000¹	0.95¹	0.83	0.23
Annexin V-iFluor® 488 conjugate	491	516	75000¹	0.9¹	0.21	0.11
Annexin V-iFluor® 555 conjugate	557	570	100000¹	0.64¹	0.23	0.14
Annexin V-iFluor® 594 conjugate	587	603	200000¹	0.53¹	0.05	0.04
Annexin V-iFluor® 647 conjugate	656	670	250000¹	0.25¹	0.03	0.03
Annexin V-iFluor® 680 conjugate	684	701	220000¹	0.23¹	0.097	0.094
Annexin V-iFluor® 700 conjugate	690	713	220000¹	0.23¹	0.09	0.04

Citations

View all 2 citations: Citation Explorer

Resources-Application Notes Phenotypic and Epigenetic Mechanism of Action Determinations of Histone Methylase and Demethylase Inhibitors using Digital Widefield Microscopy
Authors: Larson, Brad and Banks, Peter
Journal: Experimental Biology (2017)

Targeted Magnetic Intra-Lysosomal Hyperthermia produces lysosomal reactive oxygen species and causes Caspase-1 dependent cell death
Authors: Clerc, Pascal and Jeanjean, Pauline and Halalli, Nicolas and Gougeon, Michel and Pipy, Bernard and Carrey, Julian and Fourmy, Daniel and Gigoux, Véronique
Journal: Journal of Controlled Release (2017)

References

View all 32 references: Citation Explorer

Gold fluorescent annexin A5 as a novel apoptosis detection tool
Authors: Kurschus FC, Pal PP, Baumler P, Jenne DE, Wiltschi B, Budisa N.
Journal: Cytometry A (2009): 626

Glycogen synthase kinase-3 and Omi/HtrA2 induce annexin A2 cleavage followed by cell cycle inhibition and apoptosis
Authors: Wang CY, Lin YS, Su WC, Chen CL, Lin CF.
Journal: Mol Biol Cell (2009): 4153

Evaluation of annexin V and Calcein-AM as markers of mononuclear cell apoptosis during human immunodeficiency virus infection
Authors: Palma PF, Baggio GL, Spada C, Silva RD, Ferreira SI, Treitinger A.
Journal: Braz J Infect Dis (2008): 108

Detection of apoptosis induced by new type gosling viral enteritis virus in vitro through fluorescein annexin V-FITC/PI double labeling
Authors: Chen S, Cheng AC, Wang MS, Peng X.
Journal: World J Gastroenterol (2008): 2174

Measurement of annexin V uptake and lactadherin labeling for the quantification of apoptosis in adherent Tca8113 and ACC-2 cells
Authors: Hu T, Shi J, Jiao X, Zhou J, Yin X.
Journal: Braz J Med Biol Res (2008): 750

Page updated on October 8, 2024

Ordering information

Price
Conjugate
Unit size
Catalog Number	200142001520018200302003120032200652006620067200682006920070200712007220073200742007520076200772008020081200822008520089200902009220096
Quantity

Add to cart

Additional ordering information

Telephone	1-800-990-8053
Fax	1-800-609-2943
Email	sales@aatbio.com
International	See distributors
Bulk request	Inquire
Custom size	Inquire
Technical Support	Contact us
Purchase order	Send to sales@aatbio.com
Shipping	Standard overnight for United States, inquire for international

Request quotation

Physical properties

Molecular weight	~36000
Solvent	Water

Spectral properties

Correction Factor (260 nm)	0.044
Correction Factor (280 nm)	0.039
Correction Factor (565 nm)	0.0250
Correction Factor (650 nm)	0.1413
Extinction coefficient (cm ^-1 M ^-1)	275000¹
Excitation (nm)	757
Emission (nm)	779
Quantum yield	0.12¹

Storage, safety and handling

H-phrase	H303, H313, H333
Hazard symbol	XN
Intended use	Research Use Only (RUO)
R-phrase	R20, R21, R22
Storage	Freeze (< -15 °C); Minimize light exposure
UNSPSC	12352200