2-NBDG Glucose Uptake Assay Kit
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- Specifications
Product Description
2-NBDG Glucose Uptake Assay Kit provides a sensitive and non-radioactive assay for measuring glucose uptake in cultured cells. The fluorescence signal can be monitored by fluorescence microscope or flow cytometer with a 488 nm laser and 530/30 nm emission filter (FITC channel). This Assay Kit is the most robust tool for monitoring glucose transporters.
Suitable Sample
Cultured Cells.
Detection Method
Fluorimetric
Platform
Instrument: Flow cytometer
Excitation: 488 nm laser
Emission: 530/30 nm filter
Instrument specification(s): FITC channel
Instrument: Fluorescence microscope
Excitation: FITC filter
Emission: FITC filter
Recommended plate: Black wall/clear bottomRegulatory Status
For research use only (RUO)
Storage Instruction
Store the kit at -20°C and avoid from light.
Note
Example Data Analysis and Figures.
- Applications
Functional Study
Flow Cytometry
Flow cytometry of 2-NBDG uptake in CHO-K1 cells using the 2-NBDG Glucose Uptake Assay Kit. CHO-K1 cells were treated with or without 100 uM Phloretin at 37°C for 1 hour, then incubated with 100 uM 2-NBDG staining solution for 20 minutes. To prepare adherent CHO-K1 cells for flow cytometry, EDTA was used to detach cells after staining. Fluorescence intensity was measured using ACEA NovoCyte flow cytometer in FITC channel. - Publication Reference
- Respiratory syncytial virus co-opts hypoxia-inducible factor-1α-mediated glycolysis to favor the production of infectious virus.
Li-Feng Chen, Jun-Xing Cai, Jing-Jing Zhang, Yu-Jun Tang, Jia-Yi Chen, Si Xiong, Yao-Lan Li, Hong Zhang, Zhong Liu, Man-Mei Li.
mBio 2023 Oct; 14(5):e0211023.
Application:Func, Human, Hep-2 cells.
- SNHG15 promotes chemoresistance and glycolysis in colorectal cancer.
Min Li, Shengbai Sun, Zehua Bian, Surui Yao, Meng Liu, Xiaohong You, Min Li.
Pathology, Research and Practice 2023 Jun; 246:154480.
Application:Func, Human, DLD1, HTC8 cells.
- Respiratory syncytial virus co-opts hypoxia-inducible factor-1α-mediated glycolysis to favor the production of infectious virus.