LIVE/DEAD™ Cell Imaging Kit (488/570)
LIVE/DEAD™ Cell Imaging Kit (488/570)
Invitrogen™

LIVE/DEAD™ Cell Imaging Kit (488/570)

The LIVE/DEAD® Cell Imaging Kit is a sensitive two-color fluorescence cell viability assay optimized for FITC and Texas Red™ filters.Read more
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Catalog NumberQuantity
R376011 mL kit
Catalog number R37601
Price (CNY)
2,485.00
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Ends: 31-Dec-2025
3,347.00
Save 862.00 (26%)
Each
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Quantity:
1 mL kit
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Price (CNY)
2,485.00
Online Exclusive
Ends: 31-Dec-2025
3,347.00
Save 862.00 (26%)
Each
Add to cart
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The LIVE/DEAD® Cell Imaging Kit is a sensitive two-color fluorescence cell viability assay optimized for FITC and Texas Red™ filters. Quick and easy to use, the kit allows discrimination between live and dead cells with two probes that measure recognized parameters of cytotoxicity and cell viability—intracellular esterase activity and plasma membrane integrity.

Contains Calcein, AM, cell permeant dye as live cell indicator and BOBO-3 Iodide as dead cell indicator.

See other Ready Probes ready-to-use imaging reagents and accessories ›

The LIVE/DEAD® Cell Imaging Kit *488/570* offers:

Fast, simple determination of live and dead cells

• Accuracy with convenience
• Sensitive probes ideal for FITC and Texas Red filters


Dual Probe-Based Assay for Imaging Platforms
Just like our popular LIVE/DEAD® Viability/Cytotoxicity assay, the new LIVE/DEAD® Cell Imaging Kit is based on a cell-permeable dye for staining of live cells and a cell-impermeable dye for staining of dead and dying cells, which are characterized by compromised cell membranes. To adapt this important assay for imaging platforms, the LIVE/DEAD® Cell Imaging Kit components were optimized for the common green and red imaging filters used with FITC and Texas Red. The live cell component produces an intense, uniform green fluorescence in live cells (ex/em 488 nm/515 nm). The dead cell component produces a predominantly nuclear red fluorescence (ex/em 570nm/602 nm) in cells with compromised cell membranes, a strong indicator of cell death and cytotoxicity (Fig 1).

Quick, Exact Determination of Viability and Cytotoxicity
The LIVE/DEAD® Cell Imaging kit provides very sensitive detection of key measures of cell health: viability, live/dead ratio, and cytotoxicity. The components of the LIVE/DEAD® Cell Imaging kit are configured for ease of use with minimal dilutions.

Assay Principle
With the LIVE/DEAD® Cell Imaging Kit, live cells are distinguished by the presence of ubiquitous intracellular esterase activity as determined by the enzymatic conversion of the virtually non-fluorescent cell-permeant calcein AM to the intensely fluorescent calcein, which is well-retained within live cells. The red component of the LIVE/DEAD® Cell Imaging Kit is cell-impermeant and therefore only enters cells with damaged membranes. In dying and dead cells a bright red fluorescence is generated upon binding to DNA. Background fluorescence levels are inherently low with this assay technique because the dyes are virtually non-fluorescent before interacting with cells. The fluorophores in the LIVE/DEAD® Cell Imaging Kit were selected for their brightness, spectral properties (FITC and Texas Red filters), and ease of use. Packaged for workflow convenience, they allow for effortless and quick determination of the fractions of live and dead cells in a population.

See other Molecular Probes imaging tools and reagents
Specifications
Cell TypeMammalian Cells
DescriptionLIVE/DEAD™ Cell Imaging Kit (488/570)
Detection MethodFluorescence
Dye TypeOther Label(s) or Dye(s)
FormFrozen
FormatTube(s)
Incubation Time15 min
Quantity1 mL kit
Shipping ConditionDry Ice
ColorRed, Green
Emission515/602
Excitation Wavelength Range488, 570 nm
For Use With (Application)Viability Assay
For Use With (Equipment)Floid Cell Imaging System, Fluorescence Microscope
Product LineLIVE/DEAD, Molecular Probes
Product TypeCell Imaging Kit
Unit SizeEach
Contents & Storage
• Component A: 10 x 1 mL vials
• Component B: 1 x 10 vials (dried down)

Store at -20°C
PG2624-PJT8477-COL022341-Media-Promo-Pod-Graphic-Global-F-278x123
four-plex-image-COS7-live-cell zoomed
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Certificates

Lot #Certificate TypeDateCatalog Number(s)
3080150Certificate of AnalysisMay 18, 2025R37601
3079938Certificate of AnalysisApr 03, 2025R37601
3080142Certificate of AnalysisApr 03, 2025R37601
3079927Certificate of AnalysisDec 29, 2024R37601
3079918Certificate of AnalysisDec 22, 2024R37601
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Safety Data Sheets

Frequently asked questions (FAQs)

Heat killing is commonly used. Place your cells in a tube in buffer and heat at 60oC for 20 minutes. You can also kill your cells by fixing them with ice cold 70% ethanol for 15 minutes. The ethanol-killed cells can then be stored at -20oC until needed, at which point you wash out the ethanol and replace with buffer.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

The LIVE/DEAD Cell Imaging Kit (488/570) (Cat. No. R37601) is used for identifying live and dead cells using fluorescence-based staining. It cannot be used with fixed cells.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

The formulation of the solution as well as the amount and concentration of Calcein, AM provided in the LIVE/DEAD Cell Imaging Kit (488/570) (Cat. No. R37601) is proprietary information.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

Once the Live Green (Component A) and Dead Red (Component B) are mixed, this solution should be used immediately for one-time use and should not be stored.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

The nuclear stain in the LIVE/DEAD Cell Imaging Kit (488/570) is BOBO-3. The amount, concentration, and formulation is proprietary.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

Citations & References (26)

Citations & References
Abstract
A novel microfluidic platform for high-resolution imaging of a three-dimensional cell culture under a controlled hypoxic environment.
Authors:Funamoto K, Zervantonakis IK, Liu Y, Ochs CJ, Kim C, Kamm RD,
Journal:Lab Chip
PubMed ID:23023115
'Low oxygen tensions experienced in various pathological and physiological conditions are a major stimulus for angiogenesis. Hypoxic conditions play a critical role in regulating cellular behaviour including migration, proliferation and differentiation. This study introduces the use of a microfluidic device that allows for the control of oxygen tension for the ... More
Saikosaponin-d Enhances the Anticancer Potency of TNF-a via Overcoming Its Undesirable Response of Activating NF-Kappa B Signalling in Cancer Cells.
Authors:Wong VK, Zhang MM, Zhou H, Lam KY, Chan PL, Law CK, Yue PY, Liu L,
Journal:Evid Based Complement Alternat Med
PubMed ID:23573150
'Tumor necrosis factor-alpha (TNF- a ) was reported as anticancer therapy due to its cytotoxic effect against an array of tumor cells. However, its undesirable responses of TNF- a on activating NF- ? B signaling and pro-metastatic property limit its clinical application in treating cancers. Therefore, sensitizing agents capable of ... More
Aryl hydrocarbon receptor protects against bacterial infection by promoting macrophage survival and reactive oxygen species production.
Authors:Kimura A, Abe H, Tsuruta S, Chiba S, Fujii-Kuriyama Y, Sekiya T, Morita R, Yoshimura A,
Journal:
PubMed ID:24343818
'Aryl hydrocarbon receptor (AhR) is crucial for various immune responses. The relationship between AhR and infection with the intracellular bacteria Listeria monocytogenes (LM) is poorly understood. Here, we show that in response to LM infection, AhR is required for bacterial clearance by promoting macrophage survival and reactive oxygen species (ROS) ... More
Circulating fibrocytes stabilize blood vessels during angiogenesis in a paracrine manner.
Authors:Li J, Tan H, Wang X, Li Y, Samuelson L, Li X, Cui C, Gerber DA,
Journal:
PubMed ID:24300950
'Accumulating evidence supports that circulating fibrocytes play important roles in angiogenesis. However, the specific role of fibrocytes in angiogenesis and the underlying mechanisms remain unclear. In this study, we found that fibrocytes stabilized newly formed blood vessels in a mouse wound-healing model by inhibiting angiogenesis during the proliferative phase and ... More
Characterizing natural hydrogel for reconstruction of three-dimensional lymphoid stromal network to model T-cell interactions.
Authors:Kim J, Wu B, Niedzielski SM, Hill MT, Coleman RM, Ono A, Shikanov A,
Journal:
PubMed ID:25649205
'Hydrogels have been used in regenerative medicine because they provide a three-dimensional environment similar to soft tissues, allow diffusion of nutrients, present critical biological signals, and degrade via endogenous enzymatic mechanisms. Herein, we developed in vitro system mimicking cell-cell and cell-matrix interactions in secondary lymphoid organs (SLOs). Existing in vitro ... More
26 total citations

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