RayBio CaspGLOW TM Fluorescein Active Caspase-3 Staining Kit

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Table of Contents. Experiment: Apoptosis Assay using Caspase 3/7 with Hoechst... 2

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RayBio CaspGLOW TM Fluorescein Active Caspase-3 Staining Kit User Manual Version 1.0 May 10 th, 2015 RayBio Caspase-3 Fluorometric Assay Kit Protocol (Cat#: 68FLS-Casp3-S) RayBiotech, Inc. We Provide You With Excellent Support And Service Tel:(Toll Free)1-888-494-8555 or 770-729-2992; Fax:770-206-2393; Web: www.raybiotech.com Email: info@raybiotech.com

RayBiotech, Inc. Staining Kit TABLE OF CONTENTS I. Introduction. 1 II. Reagents. 2 III. Caspase-3 Assay Protocol..... 2 IV. General Troubleshooting Guide. 4 I. INTRODUCTION Activation of caspases plays a central role in apoptosis. The CaspGLOW TM Fluorescein Active Caspase-3 Staining Kit provides a convenient and sensitive means for detecting activated caspases in living cells. The assay utilizes the caspase-3 inhibitor, DEVD-FMK, conjugated to FITC (FITC-DEVD-FMK) as a marker. FITC-DEVD-FMK is cell permeable, nontoxic, and irreversibly binds to activated caspase-3 in apoptotic cells. The FITC label allows for direct detection of activated caspases in apoptotic cells by fluorescence microscopy, flow cytometry, or fluorescence plate reader. 1

II. REAGENTS Store kit at -20⁰C Components 68FLS-Casp3-S25 68FLS-Casp3-S100 Part Number 25 assays 100 assays FITC-DEVD-FMK 25 µl 100 µl Part A Wash Buffer 50 ml 2 x 100 ml Part B Z-VAD-FMK 10 µl 10 µl Part C III. CASPASE-ASSAY PROTOCOL A. Staining Procedure: 1. Induce apoptosis in cells (1 x 10 6 /ml) by desired method. At the same time, also incubate a control culture without apoptosis induction. An additional negative control can be prepared by adding the caspase inhibitor Z-VAD-FMK at 1 µl/ml to an induced culture to inhibit caspase activation. 2. Aliquot 300 µl each of the induced and control cultures into eppendorf tubes. 3. Add 1 µl of FITC-DEVD-FMK into each tube and incubate for 0.5-1 hour at 37 C incubator with 5 % CO 2. 4. Centrifuge cells at 3000 rpm for 5 minutes and remove supernatant. 5. Resuspend cells in 0.5 ml of Wash Buffer, and centrifuge again. 6. Repeat Step 5. Proceed to B, C, or D depending on methods of analysis. B. Quantification by Flow Cytometry: For flow cytometric analysis, resuspend cells in 300 µl of Wash buffer. Put samples on ice until ready. Analyze samples by flow cytometry using the FL-1/FITC channel. 2

C. Detection by Fluorescence Microscopy: For fluorescence microscopic analysis, resuspend cells in 100 µl Wash buffer. Add one drop of the cell suspension onto a microslide and cover with a coverslip. Observe cells under a fluorescence microscope using FITC filter. Caspase positive cells appear to have brighter green signals, whereas caspase negative control cells show much weaker signal. D. Analysis by Fluorescence Plate Reader: For analysis with fluorescence plate reader, resuspend cells in 100 µl Wash Buffer and then transfer the cell suspension to each well of the black microtiter plate. Measure the fluorescence intensity at Ex/Em = 485/535 nm. For control, use wells containing unlabeled cells. 3

IV. GENERAL TROUBLESHOOTING GUIDE Problems Cause Solution High background Cell density is higher than recommended Refer to datasheet and use the suggested cell number Cells were not washed well with wash buffer after staining Cells were Incubated for extended period of time Use the wash buffer provided, and as instructed in the datasheet Refer to datasheets for proper incubation time Use of extremely confluent cells Perform assay when cells are at 70-95% confluency Cells were contaminated Check for bacteria/ yeast/ mycoplasma contamination Lower signal level Cells did not initiate apoptosis Determine the optimal time and dose for apoptosis induction (time-course experiment) Very few cells were used for analysis Refer to data sheet for appropriate cell number Incorrect setting of the equipment or wavelength used to read samples Use of expired kit or improperly stored reagents Refer to datasheet and use the recommended filter setting Always check the expiry date and store the components appropriately Erratic results Old (unhealthy) cells used Seed healthy cells and make sure cells are healthy prior to induction of apoptosis Adherent cells were dislodged and washed away prior to assaying Incorrect incubation times or temperatures Collect all cells (both attached and dislodged) after induction for accurate results Refer to datasheet & verify correct incubation times and temperatures Incorrect volumes used Use calibrated pipettes and aliquot correctly Note: The most probable cause is listed under each section. Causes may overlap with other sections. 4

This product is for research use only. 2004 RayBiotech, Inc. 5