罗丹明类染料是一种膜渗透性的阳离子荧光探针,可对线粒体膜电位进行特异性识别,从而附着在线粒体中,并产生明亮荧光,在一定浓度下,罗丹明类染料对细胞具有低毒性,因此普遍用于检测动物细胞、植物细胞以及微生物中的线粒体。
生物活性 | Rhodamine dyes are membrane-permeable cationic fluorescent probes that specifically recognize mitochondrial membrane potentials, thereby attaching to mitochondria and producing bright fluorescence, and at certain concentrations, rhodamine dyes have low toxicity to cells, so they are commonly used to detect mitochondria in animal cells, plant cells, andmicroorganisms[1]. |
体外研究 (In Vitro) | 1.TMRM Perchlorate 工作液的配制 1.1 制备储存液 用 525 μL 无水DMSO 稀释 1mg TMRM Perchlorate 去配制 5 mM 的储备液。 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 1-20 μM 的 TMRM Perchlorate 工作液。 注:请根据实际情况调整 TMRM Perchlorate 工作液浓度,且现用现配。 2. 细胞染色(悬浮细胞) 2.1 离心收集细胞,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 TMRM Perchlorate 工作液,室温孵育 30-60 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,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。
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Emission (Em) | Em 570-590 nm Yellow |
Excitation (Ex) | Ex 495-570 nm Green |
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运输条件 | Room temperature in continental US; may vary elsewhere. |
储存方式 | 4°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) |
溶解性数据 | In Vitro: DMSO : 41.67 mg/mL(83.19 mM;Need ultrasonic) 配制储备液 1 mM | 1.9963 mL | 9.9814 mL | 19.9629 mL | 5 mM | 0.3993 mL | 1.9963 mL | 3.9926 mL | 10 mM | 0.1996 mL | 0.9981 mL | 1.9963 mL |
*请根据产品在不同溶剂中的溶解度选择合适的溶剂配制储备液;一旦配成溶液,请分装保存,避免反复冻融造成的产品失效。 储备液的保存方式和期限:-80℃, 6 months; -20℃, 1 month (sealed storage, away from moisture and light)。-80℃ 储存时,请在 6 个月内使用,-20℃ 储存时,请在 1 个月内使用。 |
染色示例 | Description: TMRM Perchlorate is a rapidly and selectively mitochondrial membrane potential fluorescent probe with red fluorescence.Method: For mitochondrial membrane potential measurement.1. Cultures are exposed to Millipore-filtered solutions (0.22 μM) containing TMRM Perchlorate and/or drugs for 1 h at 37℃ (except the experiment involving different durations of exposure to TMRM).2. After treatment, solutions are removed and growth media reapplied under sterile conditions, and cultures are post-incubated for 18 hours at 37℃.3. Use a confocal laser scanning microscope for image. Description: TMRM Perchlorate is a rapidly and selectively mitochondrial membrane potential fluorescent probe with red fluorescence.Method: For mitochondrial membrane potential measurement.1. Testing cells are pretreated first.2. Incubate cells with TMRM Perchlorate (20 μM; 30 min; 37℃; dark).3. Subsequently, cells are rinsed with PBS for twice and fixed in 10% formaldehyde neutral buffer solution at room temperature for 10 min.4. Cells are imaged under a Zeiss LSM710 Confocal laser-scanning microscope. Description: TMRM Perchlorate is a rapidly and selectively mitochondrial membrane potential fluorescent probe with red fluorescence.Method: For mitochondrial membrane potential measurement.1. Testing cells are pretreated first.2. The TMRM Perchlorate fluorescent dye is formulated into 50 nM/L with PBS. Incubate cells with TMRM Perchlorate (50 μL; 25 min; 37℃; dark).3. The fluorescence intensity of membrane potential measurement is detected by High Content Cell Imaging Analysis System (IN Cell analyzer 2500HS, GE, USA) and use a confocal laser scanning microscope for image.
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