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  3. Fura-2 AM

Fura-2 AM  (Synonyms: Fura-2 Acetoxymethyl ester)

Art. -Nr.: HY-101897 Reinheit: 98.53%
Handling Instructions Technical Support

Fura-2 AM is a membrane permeable, intracellular, UV light-excitable and ratiometric fluorescent Ca2+ (calcium ion) indicator. Fura-2 AM crosses cell membranes and is converted to Fura-2 (HY-D0110A) via cellular esterases. Fura-2 AM can be used to detect calcium in cells.

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Fura-2 AM

Fura-2 AM Chemische Struktur

CAS. Nr. : 108964-32-5

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Based on 9 publication(s) in Google Scholar

Other Forms of Fura-2 AM:

Top Publications Citing Use of Products
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Beschreibung

Fura-2 AM is a membrane permeable, intracellular, UV light-excitable and ratiometric fluorescent Ca2+ (calcium ion) indicator. Fura-2 AM crosses cell membranes and is converted to Fura-2 (HY-D0110A) via cellular esterases. Fura-2 AM can be used to detect calcium in cells.

In Vitro

Guideline (The following is our recommended protocol. This protocol is for reference only and should be modified according to your specific requirements).
Preparation of Stock Solution
Add anhydrous DMSO to Fura-2 AM, pipette gently or vortex until completely dissolved to prepare a 1 mM stock solution.
Cell Loading
2.1 Preparation of Working Solution (prepare freshly before use):
Preheat serum-free or low-serum medium to 37℃, add the above 1 mM stock solution, and mix by gentle inversion to prepare a 1 μM loading working solution.
(Optional) To facilitate uniform intracellular dye entry, 0.02% Pluronic F-127 or 0.1% BSA can be added.
2.2 Loading Incubation:
Transfer the coverslips with neuronal cells to a 35 mm culture dish containing the working solution.
Incubate at 37℃ for 30 minutes in the dark.
2.3 Post-incubation (De-esterification):
Preheat 2 mL of fresh dye-free culture medium.
Take out the coverslips from the loading solution and transfer them into the fresh medium.
Continue incubation at 37℃ for 20–30 minutes in the dark. This step is critical to remove extracellular residual dye and ensure sufficient intracellular hydrolysis of the dye into free Fura-2 acid.
3. Pre-imaging Preparation
3.1 Washing: Gently rinse the coverslips 1–2 times with prewarmed HBSS or imaging buffer (containing Ca2?/Mg2?) to eliminate background dye.
3.2 Mounting: Mount the coverslip onto the imaging chamber and add 1–2 mL of imaging buffer.
3.3 Stabilization: Place the chamber on a thermostatted microscope stage (37℃), equilibrate for 5–10 minutes before baseline recording.

MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only.

Molekulargewicht

1001.85

Formel

C44H47N3O24

CAS. Nr.
Appearance

Liquid (Density: 1.400±0.06 g/cm3)

Color

Light yellow to green yellow

Emission (Em)

505

Excitation (Ex)

336

SMILES

O=C(C1=CN=C(C2=CC3=CC(OCCOC4=CC(C)=CC=C4N(CC(OCOC(C)=O)=O)CC(OCOC(C)=O)=O)=C(N(CC(OCOC(C)=O)=O)CC(OCOC(C)=O)=O)C=C3O2)O1)OCOC(C)=O

Versand

Room temperature in continental US; may vary elsewhere.

Speicherung

-20°C, protect from light

*The compound is unstable in solutions, freshly prepared is recommended.

Lösungsmittel & Löslichkeit
In Vitro: 

DMSO : 10 mg/mL (9.98 mM; Need ultrasonic; Hygroscopic DMSO has a significant impact on the solubility of product, please use newly opened DMSO)

Preparing
Stock Solutions
Concentration Solvent Mass 1 mg 5 mg 10 mg
1 mM 0.9982 mL 4.9908 mL 9.9815 mL
5 mM 0.1996 mL 0.9982 mL 1.9963 mL
View the Complete Stock Solution Preparation Table

* Please refer to the solubility information to select the appropriate solvent. The compound is unstable in solutions, freshly prepared is recommended.

  • Molaritätsrechner

  • Verdünnungsrechner

Mass (g) = Concentration (mol/L) × Volume (L) × Molecular Weight (g/mol)

Mass
=
Concentration
×
Volume
×
Molecular Weight *

Concentration (start) × Volume (start) = Concentration (final) × Volume (final)

This equation is commonly abbreviated as: C1V1 = C2V2

Concentration (start)

C1

×
Volume (start)

V1

=
Concentration (final)

C2

×
Volume (final)

V2

In Vivo Dissolution Calculator
Please enter the basic information of animal experiments:

Dosage

mg/kg

Animal weight
(per animal)

g

Dosing volume
(per animal)

μL

Number of animals

Recommended: Prepare an additional quantity of animals to account for potential losses during experiments.
Calculation results:
Working solution concentration: mg/mL
Reinheit & Dokumentation

Purity: 99%

Verweise
Zellassay

MCE hat die Genauigkeit dieser Methoden nicht unabhängig bestätigt. Sie dienen nur als Referenz.

Verweise

Complete Stock Solution Preparation Table

* Please refer to the solubility information to select the appropriate solvent. The compound is unstable in solutions, freshly prepared is recommended.

Optional Solvent Concentration Solvent Mass 1 mg 5 mg 10 mg 25 mg
DMSO 1 mM 0.9982 mL 4.9908 mL 9.9815 mL 24.9538 mL
5 mM 0.1996 mL 0.9982 mL 1.9963 mL 4.9908 mL
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Help & FAQs
  • Do most proteins show cross-species activity?

    Species cross-reactivity must be investigated individually for each product. Many human cytokines will produce a nice response in mouse cell lines, and many mouse proteins will show activity on human cells. Other proteins may have a lower specific activity when used in the opposite species.

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Produktname:
Fura-2 AM
Art. -Nr.:
HY-101897
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