Cell Explorer™ Live Cell Tracking Kit Deep Red Fluorescence

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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
Shipping	Standard overnight for United States, inquire for international

Storage, safety and handling

H-phrase	H303, H313, H333
Hazard symbol	XN
Intended use	Research Use Only (RUO)
R-phrase	R20, R21, R22
UNSPSC	12352200

Alternative formats

Cell Explorer™ Live Cell Tracking Kit *Blue Fluorescence*

Cell Explorer™ Live Cell Tracking Kit *Orange Fluorescence*

Cell Explorer™ Live Cell Tracking Kit *Red Fluorescence*

Overview SDS Protocol

Platform

Flow cytometer

Excitation	640 nm laser
Emission	660/20 nm filter
Instrument specification(s)	APC channel

Fluorescence microscope

Excitation	Cy5 filter
Emission	Cy5 filter
Recommended plate	Black wall/clear bottom

Components

Example protocol

AT A GLANCE

Protocol summary

Prepare samples
Add 10X Track It™ Deep Red working solution (10 µL/well)
Stain the cells at 37 ^oC for 15 minutes to 1 hour
Wash the cells
Examine the specimen under fluorescence microscope with Cy5 filter or flow cytometer with 660/20 nm filter (APC channel)

Important notes
Thaw all the components to room temperature. Centrifuge the component A briefly before opening.

PREPARATION OF WORKING SOLUTION

Dilute 500X Track It™ Deep Red DMSO stock solution (Component A) into Assay Buffer (Component B) to make a 10 to 25X Track It™ Deep Red working solution. The working solution should be prepared enough for all the wells at 10 µL/well with the appropriate concentration. For example, to get a 10X final concentration of Track It™ Deep Red for one 96-well microplate, dilute 20 µL of 500X Track It™ Deep Red DMSO stock solution into 1 mL of Assay Buffer (Component B) to make 1 mL of 10X Track It™ Deep Red working solution. Note: The final concentration of the Track It™ Deep Red working solution should be empirically determined for different cell types and/or experimental conditions. It is recommended to test at the concentrations at least over a ten fold range. Note: The unused portion of the Track It™ Deep Red stock solution should be stored at -20^oC. Avoid repeated freeze/thaw cycles.

For guidelines on cell sample preparation, please visit
https://www.aatbio.com/resources/guides/cell-sample-preparation.html

SAMPLE EXPERIMENTAL PROTOCOL

Add 10X Track It™ Deep Red working solution to the cell wells which should be equal to 1/10 of the volume of cell culture medium. For example, for a 96-well plate, add 10 µL/well of 10X Track It™ Deep Red working solution into the cells.
Incubate the cells in a 37°C, 5% CO₂ incubator for 15 minutes to 1 hour.
Wash cells with Hanks and 20 mM Hepes buffer (HHBS) or an appropriate buffer.
Fill the cell wells with growth medium.
Analyze the cells using a fluorescence microscope with Cy5 filter or flow cytometer with 660/20 nm filter (APC channel).

Images

Figure 1. Image of HeLa cells stained with Cell Explorer™ Live Cell Tracking Kit (Cat#22624)in a Costar black wall/clear bottom 96-well plate. Cells were stained with Track It™ Deep Red for 15 minutes and image was aquired with fluorescence microscope using Cy5 filter.

Citations

View all 3 citations: Citation Explorer

Autophagy proteins are not universally required for phagosome maturation
Authors: Cemma, Marija and Grinstein, Sergio and Brumell, John H
Journal: Autophagy (2016): 1440--1446

Differential detection of tumor cells using a combination of cell rolling, multivalent binding, and multiple antibodies
Authors: Myung, Ja Hye and Gajjar, Khyati A and Chen, Jihua and Molokie, Robert E and Hong, Seungpyo
Journal: Analytical chemistry (2014): 6088--6094

Versatile fabrication of nanoscale sol--gel bioactive glass particles for efficient bone tissue regeneration
Authors: Lei, Bo and Chen, Xiaofeng and Han, Xue and Zhou, Jiaan
Journal: Journal of Materials Chemistry (2012): 16906--16913

References

View all 26 references: Citation Explorer

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A pharmaceutical company user's perspective on the potential of high content screening in drug discovery
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Journal: Methods Mol Biol (2007): 19

Optimizing the integration of immunoreagents and fluorescent probes for multiplexed high content screening assays
Authors: Giuliano KA., undefined
Journal: Methods Mol Biol (2007): 189

Past, present, and future of high content screening and the field of cellomics
Authors: Taylor DL., undefined
Journal: Methods Mol Biol (2007): 3

High-content fluorescence-based screening for epigenetic modulators
Authors: Martinez ED, Dull AB, Beutler JA, Hager GL.
Journal: Methods Enzymol (2006): 21

Application of laser-scanning fluorescence microplate cytometry in high content screening
Authors: Bowen WP, Wylie PG.
Journal: Assay Drug Dev Technol (2006): 209

High-content screening of known G protein-coupled receptors by arrestin translocation
Authors: Hudson CC, Oakley RH, Sjaastad MD, Loomis CR.
Journal: Methods Enzymol (2006): 63

Evaluation of a high-content screening fluorescence-based assay analyzing the pharmacological modulation of lipid homeostasis in human macrophages
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Journal: Cytometry A (2006): 200

Automated high content screening for phosphoinositide 3 kinase inhibition using an AKT 1 redistribution assay
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High concordance of drug-induced human hepatotoxicity with in vitro cytotoxicity measured in a novel cell-based model using high content screening
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