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Rhod-2 AM
本产品不向个人销售,仅用作科学研究,不用于任何人体实验及非科研性质的动物实验。
Rhod-2 AM图片
CAS NO:145037-81-6
包装与价格:
包装价格(元)
1mg电议
5mg电议
10mg电议

产品介绍
Rhod-2 是一种高亲和可见光激发波长的 Ca2+荧光探针,Rhod-2 AM 是 Rhod-2 的乙酰甲酯衍生物,具有细胞膜通透性,简单培养即可轻松进入细胞。一旦进入细胞,被其乳糖酶剪切产生无膜渗透性的 Rhod-2,留在细胞内执行相应的生理功能。最大激发/发射波长: 549/578 nm。
生物活性

Rhod-2 is a high-affinity visiblelightexcitation wavelength CaCa2+fluorescent probe, Rhod-2, AM is an acetyl methyl ester derivative of Rhod-2, which has cell membrane permeability and can easily enter cells with simple culture. Once it enters the cell, it is sheared by its lactesterase to produce Rhod-2 without membrane permeability, which remains in the cell to perform the corresponding physiological functions. Maximum excitation/emission wavelength: 549/578 nm[1].

体外研究
(In Vitro)

1.Rhod-2 AM 工作液的配制
1.1 制备储存液
用 无水DMSO 配制 5 mM 的 Rhod-2 AM。
1.2 工作液的配制
用预热好的无血清细胞培养基或 PBS 稀释储存液,配制成 1-10 μM 的 Rhod-2 AM 工作液。
注:请根据实际情况调整 Rhod-2 AM 工作液浓度,且现用现配。
2. 细胞染色(悬浮细胞)
2.1 悬浮细胞:在 4℃ 下 1000 g 离心 3-5 分钟,然后丢弃上清液。加入 PBS 洗涤两次,每次 5 分钟。细胞密度在 1×106/mL。
2.2 加入 1 mL Rhod-2 AM 工作液,室温孵育 5-30 分钟。
2.3 400 g,离心 3-4 分钟,弃去上清。
2.4 加入 PBS 洗涤细胞两次,每次 5 分钟。
2.5 用 1 mL 无血清培养基或 PBS 重悬细胞后,使用荧光显微镜或流式细胞仪进行观察。
3. 细胞染色(贴壁细胞)
3.1 将贴壁细胞培养于无菌盖玻片上。
3.2 从培养基中移出盖玻片,吸除多余培养基。
3.3 加入 100 μL 染料工作液,轻轻晃动使其完全覆盖细胞,室温孵育 5-30 分钟。
3.4 吸去染料工作液,用培养基洗 2-3 次,每次 5 分钟 ,使用荧光显微镜或流式细胞仪进行观察。

分子量

1123.94

性状

Oil

Formula

C52H59BrN4O19

CAS 号

145037-81-6

运输条件

Room temperature in continental US; may vary elsewhere.

储存方式

-20°C, sealed storage, away from moisture and light

*In solvent : -80°C, 6 months; -20°C, 1 month (sealed storage, away from moisture and light)

染色示例
  • Description: Rhod-2 AM is a mitochondrial probe, it can be used to detect mitochondrial Ca2+levels with red fluorescence.
    Method: For mitochondrial potential assessment.
    1. After treatment, cells are incubated at 37℃ in dark with 4 μM Rhod-2 AM for 20 min.
    2. Wash cells for three times and re-suspended in Hank’s Balanced Salt Solution without Ca2+and Mg2+.
    3. Treat cells with REE NPs and additionally stained with 20 nM TMRM, then analysed by flow cytometry (FACS) for mitochondrial membrane assessment. FACS analysis is performed using an LSR II flow cytometer (Becton Dickinson, Mountain View, CA) equipped with a single 488 nm argon laser. Rhod-2 fluorescence are examined using the PE channel; and both forward and side scatters are used to eliminate cellular fragments.
    4. Following treatment, a portion of cells are also fixed with 10% PBS-buffered formaldehyde with 0.1% Triton X-100 for 10 min, then stained with 4’ 6-diamidino-2-phenylindole (DAPI) (blue) and Fluo-3/AM (green) or Rhod-2 (red). Fluorescent images are visualized through confocal laser scanning microscopy.
  • Description: Rhod-2 AM is a mitochondrial probe, it can be used to detect mitochondrial Ca2+levels with red fluorescence.
    Method: For measurement of mitochondrial Ca2+levels.
    1. Cells are incubated with Rhod-2 AM (10 μM; 2 h; dark).
    2. Wash cells twice with PBS, and then resuspended in PBS.
    3. Fluorescence is determined by flow cytometry, and fluorescence photomicrographs are taken using a fluorescence microscope.
  • Description: Rhod-2 AM is a Ca2+fluorescence probe that specifically aggregates in mitochondria because of its positive charge, it can be used to track mitochondrial Ca2+uptake in cells.
    Method: For measurement of mitochondrial Ca2+uptake in oocytes.
    1. Around 40 oocytes are incubated with Rhod-2 AM (6 μM) in the KSOM medium for 30 min at 37℃.
    2. After three quick washes with the KSOM medium, the oocytes are imaged using a Nikon fluorescence microscope (Nikon, Tokyo, Japan).