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JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry) (ab112133)

Submit a review Q&A (5)References (10)
Flow Cytometry - JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry) (ab112133)

    Key features and details

    • Assay type: Direct
    • Detection method: Fluorescent
    • Platform: Flow cytometer
    • Assay time: 20 min
    • Sample type: Adherent cells, Suspension cells

    製品の概要

    • 製品名

      JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry)
      Mitochondrial Membrane Potential キット 製品一覧

    • 検出方法

      Fluorescent

    • サンプルの種類

      Adherent cells, Suspension cells

    • アッセイタイプ

      Direct

    • 全工程の試験時間

      0h 20m

    • 製品の概要

      JC-10 Mitochondrial Membrane Potential Assay Kit ab112133 is designed for use with flow cytometry, and it provides the most robust assay method for monitoring changes in mitochondrial membrane potential.


      The assay is based on the detection of the mitochondrial membrane potential changes in cells by the cationic, lipophilic JC-10 dye. In normal cells, JC-10 concentrates in the mitochondrial matrix where it forms red fluorescent aggregates. However, in apoptotic and necrotic cells, JC-10 diffuses out of mitochondria, changes to a monomeric form and stains cells with green fluorescence. 


      Although JC-1 is widely used in many labs, its poor water solubility causes great inconvenience. Even at 1 µM concentration, JC-1 tends to precipitate in aqueous buffer. Compared to JC-1, JC-10 has much better water solubility.


      JC-10 selectively enters mitochondria, and reversibly changes its color from green to orange-red as membrane potentials increase. This property is due to the reversible formation of JC-10 aggregates upon membrane polarization which cause a shifts in emitted light from 520 nm (the emission of JC-10 monomeric form) to 570 nm (the emission of JC-10-aggregate form). When excited at 490 nm, the color of JC-10 changes reversibly from green to greenish orange as the mitochondrial membrane becomes more polarized. 


      In normal cells, JC-10 concentrates in the mitochondrial matrix where it forms red fluorescent aggregates. However, in apoptotic and necrotic cells, JC-10 exists in monomeric form and stains cells green. The green emission can be analyzed in fluorescence channel 1 (FL1) and greenish orange emission in channel 2 (FL2). Both colors can be detected using the filters commonly mounted in all flow cytometers. Besides its use in flow cytometry, it can also be used in fluorescence imaging and fluorescence microplate platform.


      JC-10 assay protocol summary:
      - add JC-10 staining solution to experimentally treated cells
      - incubate cells for 15-60 min
      - analyze wth flow cytometer

    • 特記事項

      If you would like to use JC-10 on a microplate reader, we recommend JC-10 Mitochondrial Membrane Potential Assay Kit (Microplate) (ab112134).

      Related assays

      Review the cell health assay guide to learn about kits to perform a cell viability assaycytotoxicity assay and cell proliferation assay

      Review the metabolism assay guide to learn about assays for metabolites, metabolic enzymes, mitochondrial function, and oxidative stress, and also about how to assay metabolic function in live cells using your plate reader.

    • 試験プラットフォーム

      Flow cytometer

    製品の特性

    画像

    • Flow Cytometry - JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry) (ab112133)
      Flow Cytometry - JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry) (ab112133)

      JC-10 Mitochondrial Membrane Potential Assay Kit (Flow Cytometry) (ab112133) was used to measure the effect of FCCP induced mitochondria membrane potential change in Jurkat cells by Flow Cytometry. Jurkat cells were dye loaded with JC-10 dye-loading solution along with DMSO (Top) or 5 µM FCCP (Low) for 10 minutes. The fluorescent intensities for both J-aggregates and monomeric forms of JC-10 were measured with a flow cytometer using FL1 and FL2 channels. Uncompensated data (left column) were compared with compensated data (right column).

    参考文献 (10)

    ab112133 を使用した論文を発表された方は、こちらまでお知らせください。データシートに掲載させていただきます。

    ab112133 は 10 報の論文で使用されています。

    • Wang J  et al. Optimized allotopic expression of mitochondrial ND6 transgene restored complex I and apoptosis deficiencies caused by LHON-linked ND6 14484T > C mutation. J Biomed Sci 30:63 (2023). PubMed: 37537557
    • Tong L  et al. Mutational burden of XPNPEP3 leads to defects in mitochondrial complex I and cilia in NPHPL1. iScience 26:107446 (2023). PubMed: 37599822
    • Santos SS  et al. Effects of the PARP Inhibitor Olaparib on the Response of Human Peripheral Blood Leukocytes to Bacterial Challenge or Oxidative Stress. Biomolecules 12:N/A (2022). PubMed: 35740913
    • Mohiuddin M & Kasahara K Cisplatin Activates the Growth Inhibitory Signaling Pathways by Enhancing the Production of Reactive Oxygen Species in Non-small Cell Lung Cancer Carrying an EGFR Exon 19 Deletion. Cancer Genomics Proteomics 18:471-486 (2021). PubMed: 33994369
    • Bellanti F  et al. Inhibition of nuclear factor (erythroid-derived 2)-like 2 promotes hepatic progenitor cell activation and differentiation. NPJ Regen Med 6:28 (2021). PubMed: 34039998
    • Mohiuddin M & Kasahara K Paclitaxel Impedes EGFR-mutated PC9 Cell Growth via Reactive Oxygen Species-mediated DNA Damage and EGFR/PI3K/AKT/mTOR Signaling Pathway Suppression. Cancer Genomics Proteomics 18:645-659 (2021). PubMed: 34479917
    • Jan MW  et al. Characterization of Pathogenesis and Inflammatory Responses to Experimental Parechovirus Encephalitis. Front Immunol 12:753683 (2021). PubMed: 34899705
    • Condelli V  et al. Targeting TRAP1 as a downstream effector of BRAF cytoprotective pathway: a novel strategy for human BRAF-driven colorectal carcinoma. Oncotarget 6:22298-309 (2015). PubMed: 26084290
    • Khurana S  et al. Antiapoptotic actions of methyl gallate on neonatal rat cardiac myocytes exposed to H2O2. Oxid Med Cell Longev 2014:657512 (2014). Flow Cyt ; Rat . PubMed: 24672637
    • Liu Z  et al. Potent Half-Sandwich Iridium(III) Anticancer Complexes Containing C(?)N-Chelated and Pyridine Ligands. Organometallics 33:5324-5333 (2014). PubMed: 25328266

    レビューと Q&A

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    1-5 of 5 Abreviews or Q&A

    Question

    To whom it may concern,
    All our FACS samples are fix using BD cytofix/ctyoperm, I just want to make sure that the JC-10 mitochondrial membrane potential Assay kit (Ab112133) is compatible with fixation/permeabilization.

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    Answer





    This kit is for live cells only.



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    Question

    I was having troubles with the JC-10 kit I had ordered from your company when using it for flow cytometry.

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    Answer

    Based on the data, it looks like the way your customer treated the cells probably is the reason for the problem. It most likely when detaching the cells (trypsinized?), the mitochondria membrane potential changes. If you have to use flow, might try EDTA (which at least make the membrane intake, but I am not 100% sure if it will also cause the same problem) to lift the cells from plate. The best way for the adherent cell mitochondria membrane potential measurement will be the plate format (you do need have a bottom read mode fluorescent plate reader though). In this way, one can keep the cell intake before the experiment.
    Also, due to the great solubility of the JC-10, the sensitivity of the JC-10 on mitochondria membrane potential is very high, especially for the the cells which are very sensitive to environment. It is probably also one of the causes of these "unexpected" results. The following links are some examples that people use JC-10 in cardiomyocytes. Attached please also find a JC-10 paper published last Nov.

    http://www.cellulardynamics.com/products/lit/CDI_appnote_Cardiomyocytes_mitochondrial.pdf


    http://www.moleculardevices.com/Documents/general-documents/scientific-posters/imaging-posters/2011Poster_SBS%20Cardiotoxicity%20Imaging.pdf

    Here are some tips for flow cytometry:
    1. Lift cells with EDTA only (no trypsin), hopefully this procedure will not change the mitochondria membrane potential.
    2. treat FCCP for 15 min in growth medium first.
    3. remove the FCCP.
    4. Resuspend cells in growth medium,
    5. add equal volume of JC-10 dye-loading solution.
    6. incubate for 15 min
    7. analyze with flow.

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    Question

    I chose 10uM FCCP because in your protocol given it says to use between 2-10UM of CCCP or FCCP. I decided to try 10uM because I have previously done JC-1 experiments with an Invitrogen kit and they recommended a concentration of 50uM so I just chose the highest concentration you suggested...

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    Answer



    The concentration of CCCP or FCCP required as a positive control will vary based on cell line. Perhaps it would be useful to try 50uM FCCP as this has worked for you in the past.

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    Question

    I apologize for the late email but I have attached data from my JC-10 experiment. My main question is why CCCP is giving a greater FL2/FL1 ratio than my stained control? I thought the reverse was true?

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    Answer

    Thank you for providing that extra information.

    I have talked to the lab again, to see if they have any other thoughts on this and they think it is probably due to using the different "gating method", attached please find a copy of the method that was used for gating.

    Yes, you can dye load for 30 min first, and then treat with CCCP for 15 min, we have used FCCP for our positive control.

    If changing the gating does not prove to be successful for you, then I would be happy to either replace or refund the kit for you.

    Please let me know if there is anything I can help you with.

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    Question

    I apologize for the late email but I have attached data from my JC-10 experiment. My main question is why CCCP is giving a greater FL2/FL1 ratio than my stained control? I thought the reverse was true?

    Read More
    Answer

    Thank you for providing that information.

    I have talked to our supplier about your concerns and they have told me that your results are most likely due to the method of preparing the cells. Physically scraped the cells may damage the cell membrane already. You can tell there are two populations from Control, one with much lower F1 intensity which I believe is more healthy cells, and after CCCP treatment, that population is gone. I recommend you use EDTA (without trypsin) to dissociated the cells from plate.

    Please let me know if there is anything else I can help you with.

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