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钙黄绿素蓝 AM

CAS:No.168482-84-6

英文名称:Calcein Blue AM

分子式:C21H23NO11

分子量:465.41

储存条件:Powder:-20℃,2 years;Insolvent(母液):-20℃,6 months;-80℃,1 year

纯度:≥95%

钙黄绿素蓝 AM
小分子同系列3送1
货号:
ICA10200
品牌:
Solarbio
SKU 北京总部 北京海淀 武汉 广州
ICA10200-1mg 咨询 咨询 咨询 咨询
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Calcein Blue AM是一种细胞可渗透的Calcein Blue。在进入活细胞后,弱荧光Calcein Blue AM被水解为Calcein Blue,其具有类似于DAPI、Hoechst和AMCA的激发/发射最大值。这种与典型的绿色和红色荧光团(如FITC、TMR和Texas red)的特殊光谱分离为多路复用实验提供了额外的选择。由于Calcein Blue AM本身带有荧光,因此可能需要适当的过滤器设置和额外的洗涤步骤来最小化背景荧光。



Flow cytometer(仅供参考
Excitation                                      350 nm or 405 nm laser
Emission                                        450/40 nm filter
Instrument specification(s)           Pacific Blue channel

Fluorescence microscope(仅供参考
Excitation                             DAPI filter set
Emission                              DAPI filter set
Recommended plate           Black wall/clear bottom

Fluorescence microplate reader(仅供参考
Excitation                                      360
Emission                                        450
Cutoff                                            420
Recommended plate                    Black wall/clear bottom
Instrument specification(s)           Bottom read mode

Example protocol(仅供参考
Calcein Blue, AM Stock Solution

Prepare a 2 to 5 mM stock solution of Calcein Blue 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.
Note     The nonionic detergent Pluronic F-127 can be used to increase the aqueous solubility of AM esters.      In the staining buffer, the final Pluronic F-127 concentration should be approximately 0.02%.

Calcein Blue, AM Working Solution
Prepare a Calcein Blue AM working solution of 1 to 10 µM in the buffer of your choice (e.g., Hanks and Hepes buffer).      For most cell lines, Calcein Blue AM at the final concentration of 4 to 5 µM is recommended.      The exact concentration of indicators required for cell loading must be determined empirically.
Note     If your cells contain organic anion-transporters, probenecid (1–2.5 mM) or sulfinpyrazone (0.1–0.25 mM) may be added to the working solution to reduce leakage of the de-esterified indicators.

SAMPLE EXPERIMENTAL PROTOCOL(仅供参考
Prepare cells for imaging.
Remove the cell culture medium and wash cells once with serum-free buffer to remove any remaining media.
Note     Serum in cell culture media may contain esterase activity, which can increase background interference.
Add Calcein Blue AM working solution to the culture.
Incubate cells at 37 ℃ for 30 to 60 minutes.
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.
Measure the fluorescence intensity using either a fluorescence microscope equipped with a DAPI filter set, a flow cytometer equipped with a 450/40 nm filter (Pacific Blue channel), or a fluorescence plate reader at Ex/Em = 360/450 nm cutoff 420 nm.


备注:
以上数据均来自公开文献, Solarbio暂未进行独立验证, 仅供参考。
These protocols are for reference only. Solarbio does not independently validate these methods.

实验图
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