TMRM

製品番号: HY-D0984: Data Sheet 取扱説明書
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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, and microorganisms.

It is advisable to consider the salt form (TMRM Perchlorate) that retains the same biological activity.

商品は「研究用試薬」です。人や動物の医療用・臨床診断用・食品用の製品ではありません。
研究用途以外に使用した場合、当社は一切の責任を負いかねます。

CAS 番号 : 115532-49-5

容量		在庫状況
MOQ		Minimum order quantity
50 mg		お問い合わせ
100 mg		お問い合わせ
250 mg		お問い合わせ
Other size		お問い合わせ

* アイテムを追加する前、数量をご選択ください

This product is a controlled substance and not for sale in your territory.

Other 在庫あり Forms of TMRM:

TMRM Perchlorate

Other Forms of TMRM:

TMRM Perchlorate 在庫あり

顧客検証

Cell Imaging/Staining

Flow Cytometry

: TMRM purchased from MedChemExpress. Usage Cited in: ACS Nano. 2025 Mar 11;19(9):9390-9411. [Abstract]; Analysis of mitochondrial membrane potential. The proportion of TMRM positive cells in flow cytometry reflect the high or low mitochondrial membrane potential. Scale bar = 40 μm.

: TMRM purchased from MedChemExpress. Usage Cited in: Bioact Mater. 2024 Oct 30:44:447-460. [Abstract]; images of 4T1 cells stained with TMRM fluorescence probe after different treatments. The red fluorescence indicates the mitochondrial membrane potential. Scale bar: 50 μm. G1: PBS; G2: PBS + L; G3: AuNCs@PDA; G4: AuNCs@PDA + L; G5: AuNCs@PDA-Mn; G6: AuNCs@PDA-Mn + L, in which the symbols “L”, indicated the presence of NIR.

: TMRM purchased from MedChemExpress. Usage Cited in: J Adv Res. 2025 Aug:74:609-620. [Abstract]; Effects of silencing and overexpression of vimentin on apoptosis of MH7A cells. TMRM/DAPI staining (n = 4).

: TMRM purchased from MedChemExpress. Usage Cited in: Adv Mater. 2024 May;36(22):e2211609. [Abstract]; TMRM (25 nM, 30 min) fluorescence analysis of mitochondrial membrane potential in MEFs, iPSCs, or cells undergoing reprogramming on day 5 and 7.

: TMRM purchased from MedChemExpress. Usage Cited in: Endocrinology. 2020 Sep 1;161(9):bqaa119. [Abstract]; Mitochondrial membrane potential detected by TMRE. TMRM staining reveals a decreased signal in the Immp2l knockdown granulosa cells compared to control cells, suggesting mitochondrial membrane potential depolarization. Melatonin treatment prevented the membrane depolarization in Immp2l knockdown granulosa cells.

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製品説明	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, and microorganisms^[1].
体外実験	Guide (Following is our recommended protocol. This protocol only provides a guideline, and should be modified according to your specific needs). 1.Preparation of TMRM working solution 1.1Preparation of the stock solution Dissolve 1 mg TMRM in 525 μL DMSO to obtain 5 mM of stock solution. 1.2Preparation of TMRM working solution Dilute the stock solution in serum-free cell culture medium or PBS to obtain 1-20 μM of working solution. Note: Please adjust the concentration of TMRM working solution according to the actual situation. 2. Cell staining (Suspension cells) 2.1 Centrifuge at 1000 g at 4°C for 3-5 minutes and then discard the supernatant. Wash twice with PBS, 5 minutes each time. The cell density is 1×10⁶/mL. 2.2 Add 1 mL of working solution, and then incubate at room temperature for 5-30 minutes. 2.3 Centrifuge at 400 g at 4°C for 3-4 minutes and then discard the supernatant. 2.4 Wash twice with PBS, 5 minutes each time. 2.5 Resuspend cells with serum-free cell culture medium or PBS. Observation by fluorescence microscopy or flow cytometry. 3. Cell staining (Adherent cells) 3.1 Culture adherent cells on sterile coverslips. 3.2 Remove the coverslip from the medium and aspirate excess medium. 3.3 Add 100 μL of working solution, gently shake it to completely cover the cells, and then incubate at room temperature for 5-30 minutes. 3.4 Wash twice with medium, 5 minutes each time. Observation by fluorescence microscopy or flow cytometry. MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only. TMRM 関連抗体
分子量	401.48
分子式	C₂₅H₂₅N₂O₃
Emission (Em)	576
Excitation (Ex)	550
CAS 番号	115532-49-5
SMILES	O=C(C1=CC=CC=C1C2=C3C=CC(N(C)C)=CC3=[O+]C4=C2C=CC(N(C)C)=C4)OC
輸送条件	Room temperature in continental US; may vary elsewhere.
保管条件	Please store the product under the recommended conditions in the Certificate of Analysis.
純度とドキュメンテーション	データシート (277 KB) 取扱説明書 (2659 KB)
Dyeing Example	Description: TMRM 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 and/or drugs for 1 h at 37°C (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°C. 3. Use a confocal laser scanning microscope for image. Description: TMRM 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 (20 μM; 30 min; 37°C; dark). 3. Subsequently, the 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 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 fluorescent dye is formulated into 50 nM/L with PBS. Incubate cells with TMRM (50 μL; 25 min; 37°C; 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.
参考文献	[1]. Crowley LC, et al. Measuring Mitochondrial Transmembrane Potential by TMRE Staining. Cold Spring Harb Protoc. 2016 Dec 1;2016(12):pdb.prot087361. [Content Brief] [2]. Chowdhury SR, et al. Simultaneous evaluation of substrate-dependent oxygen consumption rates and mitochondrial membrane potential by TMRM and safranin in cortical mitochondria. Biosci Rep. 2015 Dec 8;36(1):e00286. [Content Brief] [3]. Monteith A, et al. Imaging of mitochondrial and non-mitochondrial responses in cultured rat hippocampal neurons exposed to micromolar concentrations of TMRM. PLoS One. 2013;8(3):e58059. [Content Brief]

細胞実験
^[1]

Cultures are exposed to Millipore-filtered solutions (0.22 µm) containing TMRM and/or drugs for 1 hr at 37°C (except the experiment involving different durations of exposure to TMRM). After treatment, solutions are removed and growth media reapplied under sterile conditions, and cultures are post-incubated for 18 hours at 37°C (except for the experiment involving analysis at different time points after exposure). Cells are then stained with 2 mg/mL bisbenzimide for 20 min at room temperature. Coverslips are subsequently washed in saline and imaged using 2P microscopy. Apoptotic cells are identified as brightly fluorescent nuclei under UV excitation indicating DNA fragmentation. Cell survivability is calculated as the percentage of live, unstained cells (±SD) in five microscopic fields per treatment^[1].

MedChemExpress (MCE) はこれらの方法の精度を確認していません。こちらは参照専用です。

参考文献

[1]. Crowley LC, et al. Measuring Mitochondrial Transmembrane Potential by TMRE Staining. Cold Spring Harb Protoc. 2016 Dec 1;2016(12):pdb.prot087361. [Content Brief]

[2]. Chowdhury SR, et al. Simultaneous evaluation of substrate-dependent oxygen consumption rates and mitochondrial membrane potential by TMRM and safranin in cortical mitochondria. Biosci Rep. 2015 Dec 8;36(1):e00286. [Content Brief]

[3]. Monteith A, et al. Imaging of mitochondrial and non-mitochondrial responses in cultured rat hippocampal neurons exposed to micromolar concentrations of TMRM. PLoS One. 2013;8(3):e58059. [Content Brief]

TMRM Related Classifications

Inflammation/Immunology

Molarity Calculator
Dilution Calculator

The molarity calculator equation

Mass (g) = Concentration (mol/L) × Volume (L) × Molecular Weight (g/mol)

質量		濃度		体積		分子量 *
	=		×		×

The dilution calculator equation

Concentration _(start) × Volume _(start) = Concentration _(final) × Volume _(final)

一般には略語で表示されます：C₁V₁ = C₂V₂

濃度 _（開始）	×	体積 _（開始）	=	濃度 _（終了）	×	体積 _（終了）
	×		=		×
C1		V1		C2		V2

Help & FAQs

Do most proteins show cross-species activity?
Species cross-reactivity must be investigated individually for each product. Many human cytokines will produce a nice response in mouse cell lines, and many mouse proteins will show activity on human cells. Other proteins may have a lower specific activity when used in the opposite species.

Keywords:

TMRM115532-49-5Fluorescent DyeInhibitorinhibitorinhibit

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TMRM

Other Forms of TMRM:

TMRM 関連抗体

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おすすめ

•関連小分子:

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生物活性

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