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2-NBDG

Catalog No. T14017Cas No. 186689-07-6

2-NBDG is a fluorescent indicator for direct glucose uptake measurement. It is an indicator of cell viability.

2-NBDG

2-NBDG

Purity: 98.05%
Catalog No. T14017Cas No. 186689-07-6
2-NBDG is a fluorescent indicator for direct glucose uptake measurement. It is an indicator of cell viability.
Pack SizePriceAvailabilityQuantity
1 mg$37In Stock
5 mg$97In Stock
10 mg$155In Stock
25 mg$313In Stock
50 mg$471In Stock
100 mg$710In Stock
500 mg$1,490In Stock
1 mL x 10 mM (in DMSO)$98In Stock
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Purity:98.05%
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Product Introduction

Bioactivity
Description
2-NBDG is a fluorescent indicator for direct glucose uptake measurement. It is an indicator of cell viability.
In vitro
METHODS: Flow cytometry was used to detect glucose uptake:
1, Cells were seeded at 1*104/well in 96-well plates, and the experiment was performed within 24-48 h. The cells were incubated at 37 ℃ for 10-180 min.
2, Remove the cell culture medium, add fresh medium containing 2-NBDG (5-40 µM), and incubate for 10-180 min at 37 ℃.
3. Remove the medium and wash twice with pre-cooled PBS to stop the 2-NBDG uptake reaction. Resuspend in fresh medium and perform flow cytometry within 30 min. [1]
In vivo
METHODS: Glucose uptake by circulating breast cancer cells was detected by fluorescent microscopy:
1. A mouse blood sample (100 µL/mouse) was collected by puncturing the mouse saphenous vein.
2. Incubate the blood sample containing circulating breast cancer cells with 2-NBDG (5 µg/100 µL blood) for 30 min at 37℃ in a dark incubator.
3. Add the magnetic bead suspension (1µL 1%) to 100 µL of blood sample and incubate for 30 min at 4°C with gentle shaking to promote binding of the magnetic beads to the circulating breast cancer cells.
4. Separate the circulating breast cancer cells from the blood using a magnetic separation rack, wash with PBS 3 times, resuspend in 100 µL PBS and transfer to a 96-well cell plate.
5. 2-NBDG uptake by circulating breast cancer cells was examined under a fluorescence microscope equipped with a 488 nm filter. Large cells with a fluorescent signal derived from fluorescent 2-NBDG uptake by cells were counted as hypermetabolic circulating breast cancer cells, and small-sized normal mouse blood cells (lymphocytes and RBCs) showed no or little 2-NBDG fluorescent signal. [2]
Chemical Properties
Molecular Weight342.26
FormulaC12H14N4O8
Cas No.186689-07-6
Storage & Solubility Information
Storagestore at low temperature,keep away from direct sunlight | Powder: -20°C for 3 years | In solvent: -80°C for 1 year | Shipping with blue ice.
Solubility Information
H2O: 5 mg/mL (14.61 mM), Sonication and heating to 60℃ are recommended.
Solution Preparation Table
H2O
1mg5mg10mg50mg
1 mM2.9218 mL14.6088 mL29.2176 mL146.0878 mL
5 mM0.5844 mL2.9218 mL5.8435 mL29.2176 mL
10 mM0.2922 mL1.4609 mL2.9218 mL14.6088 mL

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TargetMol | Animal experimentsFor example, your dosage is 10 mg/kg Each animal weighs 20 g, and the dosage volume is 100 μL . TargetMol | Animal experiments A total of 10 animals were administered, and the formula you used is 5% TargetMol | reagent DMSO+30% PEG300+5% Tween 80+60% ddH2O. So your working solution concentration is 2 mg/mL。
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Preparation method for in vivo formula: Take 50 μL DMSOTargetMol | reagent main solution, add 300 μLPEG300TargetMol | reagent mix well and clarify, then add 50 more μL Tween 80, mix well and clarify, then add 600 more μLddH2OTargetMol | reagent mix well and clarify
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