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Glucose Uptake Assay Kit (Colorimetric) (ab136955)

Reviews (1)Q&A (11)References (145)
Standard curve and example data.
  • Functional Studies - Glucose Uptake Assay Kit (ab136955)
  • Assay Procedure

Key features and details

  • Assay type: Cell-based (quantitative)
  • Detection method: Colorimetric
  • Platform: Microplate reader
  • Assay time: 3 hr
  • Sample type: Adherent cells, Suspension cells
  • Sensitivity: 0.01 nmol/well

Overview

  • Product name

    Glucose Uptake Assay Kit (Colorimetric)
    See all Glucose uptake kits

  • Detection method

    Colorimetric

  • Sample type

    Adherent cells, Suspension cells

  • Assay type

    Cell-based (quantitative)

  • Sensitivity

    <= 0.01 nmol/well

  • Assay time

    3h 00m

  • Species reactivity

    Reacts with: Mammals, Other species

  • Product overview

    Glucose Uptake Assay Kit (Colorimetric) (ab136955) is a highly sensitive and easy to use non-radioactive assay kit which can detect glucose uptake as low as 10 pmol/well in a variety of cell types.


    2-deoxyglucose (2-DG) is used in glucose uptake assay protocols because of its structural similarity to glucose. 2-DG is taken up by glucose transporters and metabolized to 2-DG-6-phosphate (2-DG6P). 2-DG6P cannot be further metabolized, and thus accumulates within cells. The accumulated 2-DG6P is directly proportional to 2-DG (or glucose) uptake by cells. In this assay, the 2-DG6P is oxidized to generate NADPH, the level of which can be determined by an enzymatic recycling amplification reaction.


    Glucose uptake assay protocol summary:
    - prepare cells with suitable glucose starvation / uptake stimulation depending on experimental set-up
    - add 2-DG to cells and incubate for 20 mins at 37ºC
    - wash cells with PBS to remove exogenous 2-DG
    - lyse cells with extraction buffer and repeated pipetting
    - freeze/thaw lysates and heat at 85ºC for 40 min
    - cool on ice for 5 min
    - add neutralizing buffer, spin and transfer supernatant to new tubes
    - add supernatants and standards to wells
    - add reaction mix A and incubate for 1 hr at 37ºC
    - add extraction buffer and heat to 90ºC for 40 min
    - cool on ice for 5 min and add neutralizing buffer
    - add reaction mix B
    - analyze every 2-3 mins on microplate reader in kinetic mode at 37ºC

  • Notes

    This product is manufactured by BioVision, an Abcam company and was previously called K676 Glucose Uptake Colorimetric Assay Kit. K676-100 is the same size as the 100 test size of ab136955.

    Review our 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.

  • Platform

    Microplate reader

Properties

Associated products

Images

  • Standard curve and example data.
    Standard curve and example data.
    2-DG6P Standard curve (a) and 2-DG uptake in 3T3-L1 cells (b), Human adipocytes (c) and HeLa cells (d) respectively. I=Insulin; P=Phloretin.
  • Functional Studies - Glucose Uptake Assay Kit (ab136955)
    Functional Studies - Glucose Uptake Assay Kit (ab136955)

    Glucose uptake in 3T3-L1 adipocytes stimulated with insulin (I). 3T3-L1 adipocytes were differentiated using:

     

    Dexamethasone ab120743 (1mM, 1:1000)

    IBMX ab120840 (11.5 mg/mL, 1:100)

    Insulin ab123768 (1 mg/mL, 1:1000)

  • Assay Procedure
    Assay Procedure
    Step A: 2-DG oxidation to generate NADPH; Step B: NADPH recycling amplification Reaction.

References (145)

Publishing research using ab136955? Please let us know so that we can cite the reference in this datasheet.

ab136955 has been referenced in 145 publications.

  • Liu M  et al. MYB proto-oncogene like 2 promotes hepatocellular carcinoma growth and glycolysis via binding to the Optic atrophy 3 promoter and activating its expression. Bioengineered 13:5344-5356 (2022). PubMed: 35176941
  • Wu G  et al. FSH mediates estradiol synthesis in hypoxic granulosa cells by activating glycolytic metabolism through the HIF-1a-AMPK-GLUT1 signaling pathway. J Biol Chem 298:101830 (2022). PubMed: 35300979
  • Wen YC  et al. Pyruvate kinase L/R links metabolism dysfunction to neuroendocrine differentiation of prostate cancer by ZBTB10 deficiency. Cell Death Dis 13:252 (2022). PubMed: 35306527
  • Yi B  et al. Circular RNA PLCE1 promotes epithelial mesenchymal transformation, glycolysis in colorectal cancer and M2 polarization of tumor-associated macrophages. Bioengineered 13:6243-6256 (2022). PubMed: 35349390
  • Guo Y  et al. Bmi-1 directly upregulates glucose transporter 1 in human gastric adenocarcinoma. Open Life Sci 17:261-271 (2022). PubMed: 35415241
View all Publications for this product

Customer reviews and Q&As

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1-10 of 12 Abreviews or Q&A

Glucose uptake assay of C. elegans

 Excellent Excellent 5/5 (Ease of Use)
Abreviews
This kit worked well for C. elegans assay. We tried several 1) worm amount, 2) 2DG concentrations and uptake time, 3) sample dilutions. Here we provide the optimal protocol that we found in our trial.

1. Collect 50 ul of young adult worms for each sample in 1.5 mL tube (about 1/2 worms on 9 cm dish)
2. Resuspend worms in M9 buffer (or other saline for worm) and incubate for 1 hrs
3. Remove buffer and incubate worms in 0.5 mM 2DG in M9 buffer for 2 hr
4. Wash worms with ice-cold PBST for 3 times
5. Add 80 ul of Extraction buffer, pipette up and down, and freeze
6. Thaw samples at 85 C for 40 min
7. Add 10 ul Neutralization buffer and spin briefly
8. Dilute supernatant 1/8 times with Assay buffer
9. Add 10 ul Reaction mix A, incubate at 37 C for 1 hr
10. Add 90 ul Extraction buffer and heat at 85 C for 40 min
11. Add 12 ul Neutralization buffer
12. Transfer standards and samples to a 96 well plate
13. Add 38 ul Reaction mix B, pipette up and down
14. Measure absorbance at OD412 nm at 37 C every 5 min until 100pmol/well standard reaches OD412 nm = 1.5 - 2.0
The reviewer received a reward from Abcam’s Loyalty Program in thanks for submitting this Abreview and for helping the scientific community make better-informed decisions.

Shun Kitaoka

Verified customer

Submitted Mar 12 2014

Question

When using this kit I would like to split the protocol into two stages on different days. Would this be possible?

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Answer

We would not recommend storing samples or stopping and storing samples during the assay procedure. However, if absolutely necessary the samples can be stored as cells at -80C before the addition of the extraction buffer to avoid any complications due to storage.

This kit is a very sensitive and multi-step assay using several enzymes. It is not recommended to stop and store cells in the middle of the assay since the enzymes might not work well after freezing and thawing. Once the cells are lysed using the extraction buffer, the entire assay must be completed to ensure best results.

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Question

We would like to use C2C12 and 3T3-L1cell lines which are both mouse cell lines. Would this kit work in mouse samples?

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Answer

We have only tested this kit with human sample. However, we predict that this kit can work with a wide range of mammals including mouse.

Read More

Question

Would you be able to tell us if ab136955 can be used in bacteria samples?

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Answer

Even though this kit has not been tested on bacterial samples, in principle it should work with samples from a wide range of mammals and bacteria. The method of detection is based on a biochemical reaction rather than an immunological reaction.

Read More

Question

What kind of diluent would you recommend to reconstitute 2-DG for this assay, as we are planning to perform it on a bigger scale than 96-well plates and therefore need an increased amount of 2-DG than that provided with the ab136955 kit.

Read More
Answer

Thank you for your enquiry.

I can confirm that the 2DG in the kit can be dissolved in water and is soluble up to 100 mM in water.

I hope this will be helpful. If you have any further questions, please do not hesitate to contact me.

Read More

Question

I'm using 3T3-L1 adipocytes with this kit and I just have a couple questions;
1. What is the purpose of a starvation with serum free medium, if it is then followed by starvation with glucose free buffer?
2. I culture the cells for growth with 1% insulin. Should the insulin be removed duing either the serum starvation stage and/or the glucose starvation stage?
Thanks!

Read More
Answer

Serum starvation is required because serum can provide carbon source from which the cells can make glucose.

There should be no insulin in the media during starvation. After starvation, cells are stimulated with insulin to uptake glucose via the GLUT transporters.

Read More

Question

Want to use this kit but wish to differentiate cells in flask rather than in microtiter wells. Do you have any suggestions on best way to do this? My cells lose ability to adhere once differentiated so differentiating in a flask reduces chance for cross well contamination and sample loss. However I'm not sure what the best method would be to get the cells from the flask into the microtiter plat wells? And also how many cells should I add to each well?

Read More
Answer

To do the differentiation in the flask, the washing steps after differentiation will have to be done in tubes which can be spun down to collect cells. Then the starvation step has to be done again in a flask and the following washes in a tube, spinning down the tube after each wash to collect cells. Subsequent steps of stimulation with insulin, 2DG incubation have to be done in the tubes. Finally, cell aliquots can be added to each well, then assay reagents can be added and measured. Optimization might be necessary to carry out all the steps in flasks/tubes without loss of material and to get the best, most accurate measurements.

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Question

Our spectrophotometer can only detect 405 nm not 412nm. Do you think it should be fine?

Read More
Answer

The kit is based on the fact that DTNB is converted with enzyme to TNB which has absorption maxima at 412. As all the dyes have bell shaped curves so wavelengths higher or lower than maxima should also be suitable; individual absorption maxima curves can be checked for selections of instruments.

Read More

Question

I have some questions about your glucose uptake colorimetric assay kit (ref ab136955). I'm working on human myotubes and I would to know if it's possible to start from 3.5cm petri dish and then continue into 96-well plate after the lysis step? If yes, do you have an idea on volumes of buffers/reagents that I need to use ?

Read More
Answer



You need to increase the volumes of all reagents used such that the cells are covered and are not exposed to the air to dry out. For example, for the serum starvation, instead of using the 100 µl media for covering cells in the 96 well plate, I would use about 2 ml media for the 3.5 cm plate.

Read More

Question

Does this kit need to be used within one go, or can we perform more than one experiment?

Read More
Answer

I am happy to confirm that this kit can be used multiple times.

I recommend to store all the kit components at the recommended temps and in aliquots when possible.

Please take note that repeated freeze/thaw cycles will damage the components.

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1-10 of 12 Abreviews or Q&A

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