Alexa Fluor® 647 anti-mouse/human CD324 (E-Cadherin) Antibody

Product Details

Verified Reactivity

Mouse, Human

Reported Reactivity

Cynomolgus, Dog, Pig

Antibody Type

Monoclonal

Host Species

Rat

Immunogen

E-Cadherin extracellular domain

Formulation

Phosphate-buffered solution, pH 7.2, containing 0.09% sodium azide.

Preparation

The antibody was purified by affinity chromatography and conjugated with Alexa Fluor® 647 under optimal conditions.

Concentration

0.5 mg/mL

Storage & Handling

The antibody solution should be stored undiluted between 2°C and 8°C, and protected from prolonged exposure to light. Do not freeze.

Application

FC - Quality tested
ICC, IHC-F, 3D IHC - Verified

SB - Reported in the literature, not verified in house

Recommended Usage

Each lot of this antibody is quality control tested by immunofluorescent staining with flow cytometric analysis. For flow cytometric staining, the suggested use of this reagent is ≤ 1.0 µg per million cells in 100 µL volume. For immunocytochemistry, a concentration range of 2.0 - 10 μg/mL is recommended. For immunohistochemical staining on frozen tissue sections, a concentration range of 5.0 - 10 µg/mL is suggested. For 3D immunohistochemistry on formalin-fixed tissues, a concentration of 5.0 µg/mL is suggested. It is recommended that the reagent be titrated for optimal performance for each application.

It is also recommended using EDTA-based solutions for dissociating attachment-dependent cell lines.

* Alexa Fluor® 647 has a maximum emission of 668 nm when it is excited at 633 nm / 635 nm.

Alexa Fluor® and Pacific Blue™ are trademarks of Life Technologies Corporation.

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Excitation Laser

Red Laser (633 nm)

Application Notes

Additional reported applications (for relevant formats) include: immunoprecipitation¹, Western Blotting¹, immunomicroscopy³, biological function^1,2, and spatial biology (IBEX)^4,5.

Additional Product Notes

Iterative Bleaching Extended multi-pleXity (IBEX) is a fluorescent imaging technique capable of highly-multiplexed spatial analysis. The method relies on cyclical bleaching of panels of fluorescent antibodies in order to image and analyze many markers over multiple cycles of staining, imaging, and, bleaching. It is a community-developed open-access method developed by the Center for Advanced Tissue Imaging (CAT-I) in the National Institute of Allergy and Infectious Diseases (NIAID, NIH).

Application References

(PubMed link indicates BioLegend citation)

1. Vestweber D, et al. 1985. EMBO. 4:3393. (IP, WB, FA)
2. Nakagawa M, et al. 2001. J. Cell Sci. 114:1829. (FA in canine cells)
3. Mohamet L, et al. 2010. PLoS ONE. 5:e12921. (IF)
4. Radtke AJ, et al. 2020. Proc Natl Acad Sci U S A. 117:33455-65. (SB) PubMed
5. Radtke AJ, et al. 2022. Nat Protoc. 17:378-401. (SB) PubMed

Product Citations

1. Smolen JA, et al. 2022. PNAS Nexus. 1:pgac235. PubMed
2. Jeon Y, et al. 2022. Cancers (Basel). 14:. PubMed
3. Vereertbrugghen A, et al. 2023. J Neuroinflammation. 20:120. PubMed
4. Khodeer S, et al. 2022. J Cell Sci. 135: . PubMed
5. Law NC, et al. 2019. Nat Commun. 10:2787. PubMed
6. Rodríguez E, et al. 2022. Commun Biol. 5:41. PubMed
7. Pitarresi JR, et al. 2021. Cancer Discov. 11:1774. PubMed
8. Cohen SB et al. 2018. Cell host & microbe. 24(3):439-446 . PubMed
9. Stefkovich ML, et al. 2021. Curr Protoc. 1:e139. PubMed
10. Gentek R, et al. 2018. Immunity. 48:1160. PubMed
11. Han S, et al. 2019. Cell Stem Cell. 25:342. PubMed
12. Rosàs-Canyelles E, et al. 2020. Sci Adv. 6:eaay1751. PubMed
13. Emily A Thompson et al. 2019. Cell reports. 26(11):2859-2867 . PubMed
14. Steele NG, et al. 2021. Clin Cancer Res. 27:2023. PubMed
15. Gawronska-Kozak B, et al. 2016. PLoS One. 11: 0150635. PubMed
16. Norgard RJ, et al. 2021. EMBO Rep. 22:e51872. PubMed
17. Malenica I, et al. 2021. Nat Commun. 12:5209. PubMed
18. Radke J, et al. 2022. Nat Commun. 13:7304. PubMed

RRID

AB_2563954 (BioLegend Cat. No. 147307)
AB_2563954 (BioLegend Cat. No. 147308)

Antigen Details

Structure

Member of the cadherin superfamily. Calcium-dependent, transmembrane cell-cell adhesion glycoprotein composed of four extracellular cadherin repeats and a highly conserved cytoplasmic tail region.

Distribution

Widely expressed in epithelial cells in the colon, uterus, liver, keratinocytes, brain, heart, muscle, kidney, and pancreas as well as erythroid cells.

Function

Cell adhesion molecule involved in development, bacterial pathogenesis, and tumor invasion. The ectodomain of CD324 mediates bacterial adhesion to mammalian cells, while the cytoplasmic domain is required for internalization.

Interaction

Interacts with a variety of proteins including erbin, ezrin, caspase-3, caspase-8, EGF receptor, β-catenin, presenilin 1, casein kinase II, and others.

Ligand/Receptor

αEβ7 integrin.

Cell Type

Embryonic Stem Cells

Biology Area

Cell Adhesion, Cell Biology, Immunology, Innate Immunity, Neuroscience, Stem Cells, Synaptic Biology

Molecular Family

Adhesion Molecules, CD Molecules

Antigen References

1. Overduin M, et al. 1995. Science 267:386.
2. Boggon TJ, et al. 2002. Science 296:1308.
3. Berx G, et al. 1995. EMBO J. 14:6107.
4. Perl AK, et al. 1998. Nature 392:190.

Gene ID

999 View all products for this Gene ID 12550 View all products for this Gene ID

UniProt

View information about CD324 on UniProt.org

Documentation

• Technical data sheet
• Certificate of Analysis
• Safety Data Sheet

Reviews

Related Protocols

• Immunohistochemistry Protocol for Frozen Sections
• Cell Surface Flow Cytometry Staining Protocol
• Immunocytochemistry Staining Protocol
• Ce3D™ Tissue Clearing Kit

Related Pages & Pathways

Related FAQs

If an antibody clone has been previously successfully used in IBEX in one fluorescent format, will other antibody formats work as well?

It’s likely that other fluorophore conjugates to the same antibody clone will also be compatible with IBEX using the same sample fixation procedure. Ultimately a directly conjugated antibody’s utility in fluorescent imaging and IBEX may be specific to the sample and microscope being used in the experiment. Some antibody clone conjugates may perform better than others due to performance differences in non-specific binding, fluorophore brightness, and other biochemical properties unique to that conjugate.

Will antibodies my lab is already using for fluorescent or chromogenic IHC work in IBEX?

Fundamentally, IBEX as a technique that works much in the same way as single antibody panels or single marker IF/IHC. If you’re already successfully using an antibody clone on a sample of interest, it is likely that clone will have utility in IBEX. It is expected some optimization and testing of different antibody fluorophore conjugates will be required to find a suitable format; however, legacy microscopy techniques like chromogenic IHC on fixed or frozen tissue is an excellent place to start looking for useful antibodies.

Are other fluorophores compatible with IBEX?

Over 18 fluorescent formats have been screened for use in IBEX, however, it is likely that other fluorophores are able to be rapidly bleached in IBEX. If a fluorophore format is already suitable for your imaging platform it can be tested for compatibility in IBEX.

The same antibody works in one tissue type but not another. What is happening?

Differences in tissue properties may impact both the ability of an antibody to bind its target specifically and impact the ability of a specific fluorophore conjugate to overcome the background fluorescent signal in a given tissue. Secondary stains, as well as testing multiple fluorescent conjugates of the same clone, may help to troubleshoot challenging targets or tissues. Using a reference control tissue may also give confidence in the specificity of your staining.

How can I be sure the staining I’m seeing in my tissue is real?

In general, best practices for validating an antibody in traditional chromogenic or fluorescent IHC are applicable to IBEX. Please reference the Nature Methods review on antibody based multiplexed imaging for resources on validating antibodies for IBEX.

Other Formats

Certificate of Analysis