Products
Rhod-2 AM

CAS:145037-81-6

Storage:Powder:-20℃,2 years;Insolvent(Mother Liquid):-20℃,6 months;-80℃,1 year

Purity:≥95%

Appearance:Solid

Rhod-2 AM
Cat.No:
IR1880
Brand:
Solarbio
SKU Tongzhou Beijing Haidian Beijing Wuhan Guangzhou
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Calcium ion fluorescence probe Rhod-2, AM is a reagent for calcium flux determination, which is the preferred method in drug discovery for screening G-protein-coupled receptors (GPCR).

Rhod-2 is a Ca2+ fluorescence probe with high affinity to visible light excitation wavelength. Rhod-2 AM is an acetyl methyl derivative of Rhod-2 and has cell membrane permeability. Once inside the cell, it is cleaved by its lactase enzyme to produce membraneless permeable Rhod-2, which remains in the cell to perform its corresponding physiological functions. Maximum excitation/emission wavelength: 549/578 nm.

Fluorescence microscope(for reference only)

Excitation TRITC filter set

Emission TRITC filter set

Recommended plate Black wall/clear bottom

Fluorescence microplate reader(for reference only)

Excitation 540

Emission 590

Cutoff 570

Recommended plate Black wall/clear bottom

Instrument specification(s) Bottom read mode/Programmable liquid handling

Example protocol(For reference only)

Rhod-2 AM Stock Solution

Prepare a 2 to 5 mM stock solution of Rhod-2 AM in high-quality, anhydrous DMSO.

If it is necessary to prepare a stock solution, it is recommended to store in aliquots to avoid product failure caused by repeated freezing and thawing.

Rhod-2 AM Working Solution

For most cell lines, Rhod-2 AM at a final concentration of 4-5 μM is recommended. The exact concentration of indicators required for cell loading must be determined empirically.

Note The nonionic detergent Pluronic F-127 is sometimes used to increase the aqueous solubility of Rhod-2 AM.

Note If your cells contain organic anion-transporters, probenecid (1-2 mM) may be added to the dye working solution (final in well concentration will be 0.5-1 mM) to reduce leakage of the de-esterified indicators.

SAMPLE EXPERIMENTAL PROTOCOL(For reference only)

Following is our recommended protocol for loading AM esters into live cells. This protocol only provides a guideline and should be modified according to your specific needs.

Prepare cells in growth medium overnight.

On the next day, add 1X Rhod-2 AM working solution into your cell plate.

Note If your compound(s) interfere with the serum, replace the growth medium with fresh HHBS buffer before dye-loading.

Incubate the dye-loaded plate in a cell incubator at 37 ℃ for 30 to 60 minutes.

Note Incubating the dye for longer than 1 hour can improve signal intensities in certain cell lines.

Replace the dye working solution with HHBS or buffer of your choice (containing an anion transporter inhibitor, such as 1 mM probenecid, if applicable) to remove any excess probes.

Add the stimulant as desired and simultaneously measure fluorescence using either a fluorescence microscope equipped with a TRITC filter set or a fluorescence plate reader containing a programmable liquid handling system such as an FDSS, FLIPR, or FlexStation, at Ex/Em = 540/590 nm cutoff 570 nm.

Remark:
These protocols are for reference only. Solarbio does not independently validate these methods.

Note:
1. The products are all for scientific research use only. Do not use it for medical, clinical diagnosis or treatment, food and cosmetics, etc. Do not store them in ordinary residential areas.
2. For your safety and health, please wear laboratory clothes, disposable gloves and masks.
3. The experimental results may be affected by many factors, after-sale service is limited to the product itself and does not involve other compensation.
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