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AB140359

MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent)

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(3 Publications)

MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) is a Cell-based (quantitative) ELISA for the measurement of MitoBiogenesis™ In-Cell (Fluorescent) in in Cell/Tissue Extracts samples from a wide range of species.

View Alternative Names

SDH2, SDHF, SDHA, Flavoprotein subunit of complex II, Malate dehydrogenase [quinone] flavoprotein subunit, Fp

4 Images
Immunocytochemistry - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)
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Supplier Data

Immunocytochemistry - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)

Antibody specificity demonstrated by immunocytochemistry. Two-color immunocytochemical labeling of cultured cells with the two primary monoclonal antibodies specific for COX-I and SDH-A. The two antibodies exhibit striking and specific co-localization in the mitochondria, consistent with the known mitochondrial expression of both proteins.

Functional Studies - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)
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Supplier Data

Functional Studies - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)

Quantitative measurement of the COX-I/SDH-A protein expression ratio. At all cell concentrations, a consistent ratio of mtDNA-encoded protein expression COX-I (HRP signal) to nuclear DNA-encoded mitochondrial protein expression SDH-A (AP signal) is observed in untreated cells. Therefore, normalizing COX-I levels to SDH-A levels simplifies data analysis and eliminates the need to perform all tests at the same cell concentration.

Inhibition Assay - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)
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Supplier Data

Inhibition Assay - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)

Inhibition of mitochondrial biogenesis by chloramphenicol. The IC50 of a drug’s effect on mitochondrial protein translation can be determined quickly using the MitoBiogenesis™ ICE Kit. In this example, cells were seeded at 6,000 cells/well, allowed to grow for 6 days in a drug dilution series and then relative amounts of COX-I (HRP signal), and SDH-A (AP-signal) were measured in each well. Chloramphenicol inhibits mtDNA-encoded (HRP signal) COX-I protein synthesis relative to nuclear DNA-encoded (AP signal) SDH-A protein synthesis by 50% at 8.1 µM, %CV = 4.33% for HRP (COX-1) signal and 3.13% for AP (SDH-A) signal.

Western blot - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)
  • WB

Supplier Data

Western blot - MitoBiogenesis™ In-Cell ELISA Kit (Fluorescent) (AB140359)

Antibody specificity demonstrated by Western blot.

A Western blot of total cell protein (10 μg) from Human or rat cultured cells was probed with the primary and secondary antibodies and scanned with a LI-COR® Odyssey® imager. The two mitochondrial proteins targeted by the two primary mAbs were labeled and visualized specifically despite the presence of thousands of other proteins. Furthermore, reduction of mtDNA levels in human Rho0 (mtDNA-depleted) cells, or inhibition of mitochondrial protein translation by chloramphenicol in rat cells result in specific reduction of COX-I protein while nuclear DNA-encoded SDH-A is unaffected.

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Key facts

Detection method

Fluorescent

Sample types

Cell culture extracts

Reacts with

Mouse, Rat, Cow, Human

Assay type

Cell-based (quantitative)

Assay Platform

Microplate

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Reactivity data

{ "title": "Reactivity Data", "filters": { "stats": ["", "Reactivity", "Dilution Info", "Notes"] }, "values": { "ELISA": { "reactivity":"TESTED_AND_REACTS", "dilution-info":"", "notes":"<p></p>" } } }
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Product details

ab140359 is an In-Cell ELISA (ICE) assay kit that uses quantitative immunocytochemistry to measure levels of COX1 and SDHA levels in cultured cells. Cells are fixed in a microplate and targets of interest are detected with highly specific, well-characterized antibodies. Relative target levels are quantified using secondary antibodies conjugated to either horseradish peroxidase (HRP) or alkaline phosphatase (AP) which generate signal through the use of two spectrally distinct fluorogenic substrates. Fluorescence is measured using a standard fluorescent spectrophotometer and relative levels of target proteins are quantified. Optionally, antibody signal intensity can be normalized to the total cell amount using Janus Green stain. In-Cell ELISA (ICE) technique generates quantitative data with specificity similar to Western blotting, but with much greater quantitative precision and higher throughput due to the greater dynamic range and linearity of fluorescence detection and the ability to run up to 96 samples in parallel. This method rapidly fixes the cells in situ, stabilizing the in vivo levels of proteins and their post-translational modifications, and thus essentially eliminates changes during sample handling, such as preparation of protein extracts.

Plates are available in our ICE (In-Cell ELISA) Support Pack (ab111542) which can be bought separately.

"Cytochrome c oxidase is the component of the respiratory chain that catalyzes the reduction of oxygen to water. Subunits 1-3 form the functional core of the enzyme complex. CO I is the catalytic subunit of the enzyme. Electrons originating in cytochrome c are transferred via the copper A center of subunit 2 and heme A of subunit 1 to the bimetallic center formed by heme A3 and copper B. Catalytic activity carries out the following reaction; 4 ferrocytochrome c + O2 + 4 H+ = 4 ferricytochrome c + 2 H2O.Flavoprotein (FP) subunit of succinate dehydrogenase (SDH) that is involved in complex II of the mitochondrial electron transport chain and is responsible for transferring electrons from succinate to ubiquinone (coenzyme Q). Can act as a tumor suppressor. Catalytic activity carries out following reaction; Succinate + ubiquinone = fumarate + ubiquinol.**Related products**Review the , or the full to learn about more assays for metabolites, metabolic enzymes, mitochondrial function, and oxidative stress, and also how to assay metabolic function in live cells using your plate reader.

REACH authorisation
Abcam has not and does not intend to apply for the REACH Authorisation of customers' uses of products that contain European Authorisation list (Annex XIV) substances.
It is the responsibility of our customers to check the necessity of application of REACH Authorisation, and any other relevant authorisations, for their intended uses.

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Precision

[ { "reproducibilityType": "Intra", "sample": "COX-1 (HRP)", "replicates": 0, "mean": null, "standardDeviation": null, "coefficientOfVariability": "4.62" }, { "reproducibilityType": "Intra", "sample": "SDH-A (AP)", "replicates": 0, "mean": null, "standardDeviation": null, "coefficientOfVariability": "6.02" } ]
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What's included?

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Properties and storage information

Shipped at conditions
Blue Ice
Appropriate short-term storage conditions
+4°C
Appropriate long-term storage conditions
+4°C
Storage information
+4°C
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Product protocols

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Target data

Flavoprotein (FP) subunit of succinate dehydrogenase (SDH) that is involved in complex II of the mitochondrial electron transport chain and is responsible for transferring electrons from succinate to ubiquinone (coenzyme Q) (PubMed : 10746566, PubMed : 24781757). SDH also oxidizes malate to the non-canonical enol form of oxaloacetate, enol-oxaloacetate (By similarity). Enol-oxaloacetate, which is a potent inhibitor of the succinate dehydrogenase activity, is further isomerized into keto-oxaloacetate (By similarity). Can act as a tumor suppressor (PubMed : 20484225).
See full target information SDHA

Additional targets

MT-CO1
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Publications (3)

Recent publications for all applications. Explore the full list and refine your search

Cancer & metabolism 12:24 PubMed39113152

2024

The polyunsaturated fatty acid docosahexaenoic affects mitochondrial function in prostate cancer cells.

Applications

Unspecified application

Species

Unspecified reactive species

Guilherme Henrique Tamarindo,Caroline Fidalgo Ribeiro,Alana Della Torre Silva,Alex Castro,Ícaro Putinhon Caruso,Fátima Pereira Souza,Sebastião Roberto Taboga,Massimo Loda,Rejane Maira Góes

Nature communications 12:487 PubMed33473105

2021

BNIP3L/NIX-mediated mitophagy protects against glucocorticoid-induced synapse defects.

Applications

Unspecified application

Species

Unspecified reactive species

Gee Euhn Choi,Hyun Jik Lee,Chang Woo Chae,Ji Hyeon Cho,Young Hyun Jung,Jun Sung Kim,Seo Yihl Kim,Jae Ryong Lim,Ho Jae Han

Genes 11: PubMed32867169

2020

Leigh Syndrome in a Pedigree Harboring the m.1555A>G Mutation in the Mitochondrial 12S rRNA.

Applications

Unspecified application

Species

Unspecified reactive species

Mouna Habbane,Laura Llobet,M Pilar Bayona-Bafaluy,José E Bárcena,Leticia Ceberio,Covadonga Gómez-Díaz,Laura Gort,Rafael Artuch,Julio Montoya,Eduardo Ruiz-Pesini
View all publications
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