描述
BODIPY 493/503 中性脂滴荧光探针
产品标签
BODIPY 493/503;Nile Red 尼罗红;Neutral lipds 中性脂滴;DiI 细胞膜探针;DiR; CAS NO:121207-31-6
产品信息
|
产品名称 |
产品编号 | 规格 | CAS NO. | 价格(元) |
|
BODIPY 493/503 中性脂滴荧光探针 |
MX5403-5MG | 5mg | 121207-31-6 |
680 |
| BODIPY 493/503 中性脂滴荧光探针 | MX5403-10MG | 10mg | 121207-31-6 |
980 |
产品描述
BODIPY 493/503是一种亲脂性荧光探针,定位在极性脂上,能用于标记细胞中性脂内容物,特别定位在活细胞和固定细胞的脂滴上。BODIPY 493/503与落射荧光显微镜、共聚焦荧光显微镜和双质子荧光显微镜,以及流式细胞仪兼容。最大激发和发射波长分别是493/503nm,适用于活细胞和固定细胞标记。
产品特性
1)CAS NO.:121207-31-6
2)化学名:(T-4)-[2-[1-(3,5-dimethyl-2H-pyrrol-2-ylidene-κN)ethyl]-3,5-dimethyl-1H-pyrrolato-κN]difluoro-boron
3)同义名:4,4-Difluoro-1,3,5,7,8-Pentamethyl-4-Bora-3a,4a-Diaza-s-Indacene
4)分子式:C14H17BF2N2
5)分子量:262.1
6)纯度:≥98%
7)Ex/Em:493/503nm
8)溶解性:溶于DMSO或无水乙醇
9)化学结构式:
保存与运输方法
保存:-20ºC避光干燥保存,至少2年有效。
运输:冰袋运输。
储存液的制备和保存
1)将低温保存的10mg BODIPY 493/503(Mw:262.1)置于室温回温至少20min,低速离心后加入一定量的无水乙醇或无水DMSO配制成适量浓度的母液,比如5mM(往10mg 粉末加入7.63ml DMSO,充分溶解即可)。根据单次用量将储存液分装,≤-20℃避光干燥保存。需注意溶液内湿度的逐渐积累会随着时间引起探针聚集,从而务必干燥保存储存液。
2)如果想长期保存,可以用无水乙醇溶解粉末,之后分装到小量,之后使用真空泵来挥发掉乙醇。之后置于≤-20℃避光干燥保存。
探针的标记(仅作参考)
由于BODIPY 493/503属于疏水染料,难以快速的分散进入水溶性溶液中,为了能均匀稳定的标记细胞,可参考以下方法标记活细胞。
应用示例
图1. 胞内中性LDs的定量和观察。A,A498细胞在含BSA(0.2%)或含BSA的油酸过夜培养。之后根据流式分析的操作步骤进行BODIPY染色;B,A498细胞在含BSA(0.2%)或含BSA的油酸过夜培养。之后根据荧光分析的操作步骤进行BODIPY染色;
BODIPY staining for flow cytometry
- Grow cells under culture conditions relevant for the study. A 35 mm dish/well is sufficient for the cell numbers required in this assay. For our assays, 50,000 A498 cells in 35 mm well were sufficient.
- Overnight incubation of cells with 30 μM oleic acid can serve as a positive control for increased neutral lipid content, as oleic acid is a potent inducer of triglyceride synthesis and storage. Fatty acid free BSA serves as a control.
- At the time-point of interest, prepare 2 μM BODIPY staining solution in PBS. The volume of staining solution required for each sample corresponds to the volume of media used for culturing cells.
- Wash cells with a quick rinse using 3 ml PBS to remove media/serum.
- Incubate on BODIPY staining solution in the dark for 15 min at 37 °C. Include an unstained control for flow cytometry.
Note: From this point, protect samples from light as much as possible.
- Wash cells with a quick rinse using 3 ml PBS to remove staining solution.
- Trypsinize cells to generate a single cell suspension. For the A498 cell line used in this protocol, cells were incubated with Trypsin-EDTA (0.25%) for 5 min at 37 °C.
- Add 5 ml of PBS and transfer cell suspension to a 15 ml conical tube.
- Pellet cells at 250 × g, 5 min, 4 °C.
- Aspirate supernatant, wash the cell pellet with a quick rinse using 3 ml PBS, and pellet cells at 250 × g, 5 min, 4 °C.
- Carefully aspirate the supernatant and resuspend cells in 300 μl 1× flow cytometry buffer.
- Pass cell suspension through a 35 μm filter into a FACS tube.
- Perform flow cytometry. Obtain a minimum of 10,000 events per condition.
- The investigator can analyze data as mean fluorescence (Figure A) or display the data as a histogram (Figure B).
注意事项
1)荧光染料均存在淬灭问题,请尽量注意避光,以减缓荧光淬灭。
2)为了您的安全和健康,请穿实验服并戴一次性手套操作。
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