7-Aminoactinomycin D (7-AAD) (Synonyms: 7-AAD, NSC 239759) |
| رقم الكتالوجGC33577 |
7-Aminoactinomycin D (7-AAD) (7-AAD) وصمة دنا فلورية ، هو مثبط قوي لبوليميراز الحمض النووي الريبي.
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Cas No.: 7240-37-1
Sample solution is provided at 25 µL, 10mM.
7-Aminoactinomycin D (7-AAD) is a fluorescent DNA dye that is commonly used to detect or exclude non-viable cells in flow cytometry analysis because 7-AAD is usually excluded by living cells[1][ 2]. 7-AAD exhibits excitation spectra at 488, 546, and 578 nm and an emission spectrum at 650 nm [3]. Since 7-AAD is detected in the far-red range of the spectrum, it has minimal spectral overlap with commonly used probes and thus can be used in combination with probes such as FITC [1] [3]. 7-AAD has been used to assess apoptosis and cell-mediated cytotoxicity and to stain DNA in cells fixed and permeabilized by various methods [1] [2] [4].
7-AAD is a fluorescent derivative of actinomycin D that selectively binds to the GC region of DNA [5]. Taking advantage of the permeability of the cell membrane and the fact that the fluorescence intensity of 7-AAD is lower in early apoptotic cells and higher in late apoptotic and dead cells, it can be performed in fixed/permeabilized cells by flow cytometry. cycle analysis. Low concentrations (0.5-5μg/ml) of 7-AAD are often used to stain and exclude dead cells in flow cytometry; higher concentrations (10-20μg/ml) of 7-AAD are used to distinguish live cells (7-AAD negative ), apoptotic cells (7-AAD dim bright) and dead cells (7-AAD)[5].
References:
[1].Schmid, I., Uittenbogaart, C.H., Keld, B., et al.A rapid method for measuring apoptosis and dual-color immunofluorescence by single laser flow cytometryJ. Immunol. Methods170(2)145-157(1994)
[2].Coder, D.M.Assessment of cell viabilityCurr. Protoc. Cytom.Suppl. 15(1997)
[3].Stokke, T., Holte, H., and Steen, H.B.In vitro and in vivo activation of B-lymphocytes: A flow cytometric study of chromatin structure employing 7-aminoactinomycin DCancer Res.48(23)6708-6714(1988)
[4].Lecoeur, H., Février, M., Garcia, S., et al.A novel flow cytometric assay for quantitation and multiparametric characterization of cell-mediated cytotoxicityJ. Immunol. Methods253(1-2)177-187(2001)
[5].Nadine C L Zembruski, et al. 7-Aminoactinomycin D for apoptosis staining in flow cytometry. 2012 Oct 1;429(1):79-81. doi: 10.1016/j.ab.2012.07.005. Epub 2012 Jul 14.
This plan only provides a guide, please modify it to meet your specific needs.
1. Prepare 7-Aminoactinomycin D (7-AAD) staining solution
(1) 7-Aminoactinomycin D (7-AAD) dye stock solution: Use 50% DMSO to dissolve 7-AAD into a 1mg/ml stock solution.
Note: Unused storage solution should be aliquoted and stored in the dark at -20°C to avoid repeated freezing and thawing. The prepared storage solution needs to be filtered and sterilized using a 0.22μm nylon filter.
(2) Preparation of working solution: Dilute the storage solution with a suitable sterile buffer (such as serum-free culture medium, HBSS or PBS) to prepare a working solution with a concentration of 0.5-20 μg/ml.
Notice:
① Low concentration (0.5-5μg/ml) 7-AAD is often used for flow cytometry staining or excluding dead cells; higher concentration (10-20μg/ml) 7-AAD is used to distinguish living cells (7-AAD negative ), apoptotic cells (7-AAD dim bright) and dead cells (7-AAD)
② Please adjust the concentration of the working fluid according to the actual situation and prepare it now.
2. Cell suspension staining
(1) Suspension cells: Centrifuge the suspended cells at 4°C and 1000g for 3-5 minutes, discard the supernatant, and wash twice with PBS for 5 minutes each time.
(2) Adherent cells: Discard the culture medium and add trypsin to digest the cells. After centrifugation and discarding the supernatant, add PBS and wash twice, 5 minutes each time.
(3) Resuspend approximately 1 x 106 cells in 0.5-1mL working solution and incubate at 4°C in the dark for 5-30 minutes. The optimal incubation time for different cells is different, please explore by yourself according to the specific experimental needs.
3. Cell adhesion staining
(1) Culture adherent cells on sterile coverslips.
(2) Remove the coverslip from the culture medium, suck out the excess culture medium, and place the coverslip in a humid environment.
(3) Add 100 μL of Hoechst dye working solution from one corner of the coverslip, shake gently to make the dye evenly cover all cells, and incubate at 4°C in the dark for 5-30 minutes.
(4) Aspirate away the dye working solution, wash the coverslip 2 to 3 times with culture solution, and observe with a fluorescence microscope.
4. Fluorescence detection: The maximum absorption wavelength of 7-AAD is 546 nm, and it can be effectively excited using a 543nm helium-neon laser; it can also be excited with a lower efficiency using a 488nm or 514nm argon laser line. The emission of 7-AAD has a very large Stokes shift, maximum in deep red: 647 nm. Therefore, 7-AAD is compatible with most blue and green fluorophores and even many red fluorophores in multicolor applications.
Precautions:
① 7-AAD is a strong carcinogen. In order to avoid skin and eye contact, it is recommended to wear gloves, lab coats and eye masks/face masks during operation;
② Fluorescent dyes all have quenching problems. Please try to avoid light to slow down fluorescence quenching.
| Cas No. | 7240-37-1 | SDF | |
| المرادفات | 7-AAD, NSC 239759 | ||
| Canonical SMILES | O=C(N[C@H](C(N1[C@@](C(N(C)CC(N(C)[C@@H](C(C)C)C(O[C@@H]2C)=O)=O)=O)([H])CCC1)=O)C(C)C)[C@H]2NC(C(C(C(OC3=C(C)C(N)=C4)=C5C)=NC3=C4C(N[C@@H]6C(N[C@H](C(N7[C@@](C(N(C)CC(N(C)[C@@H](C(C)C)C(O[C@@H]6C)=O)=O)=O)([H])CCC7)=O)C(C)C)=O)=O)=C(N)C5=O)=O | ||
| Formula | C62H87N13O16 | M.Wt | 1270.43 |
| الذوبان | DMF: 10 mg/ml,DMF:PBS(pH 7.2)(1:1): 0.5 mg/ml,DMSO: 5 mg/ml | Storage | -20°C, protect from light,unstable in solution, ready to use. |
| General tips | Please select the appropriate solvent to prepare the stock solution according to the
solubility of the product in different solvents; once the solution is prepared, please store it in
separate packages to avoid product failure caused by repeated freezing and thawing.Storage method
and period of the stock solution: When stored at -80°C, please use it within 6 months; when stored
at -20°C, please use it within 1 month. To increase solubility, heat the tube to 37°C and then oscillate in an ultrasonic bath for some time. |
||
| Shipping Condition | Evaluation sample solution: shipped with blue ice. All other sizes available: with RT, or with Blue Ice upon request. | ||
| Prepare stock solution | |||
|
1 mg | 5 mg | 10 mg |
| 1 mM | 0.7871 mL | 3.9357 mL | 7.8714 mL |
| 5 mM | 0.1574 mL | 0.7871 mL | 1.5743 mL |
| 10 mM | 0.0787 mL | 0.3936 mL | 0.7871 mL |
Step 1: Enter information below (Recommended: An additional animal making an allowance for loss during the experiment)
g
μL
Step 2: Enter the in vivo formulation (This is only the calculator, not formulation. Please contact us first if there is no in vivo formulation at the solubility Section.)
Calculation results:
Working concentration: mg/ml;
Method for preparing DMSO master liquid: mg drug pre-dissolved in μL DMSO ( Master liquid concentration mg/mL, Please contact us first if the concentration exceeds the DMSO solubility of the batch of drug. )
Method for preparing in vivo formulation: Take μL DMSO master liquid, next addμL PEG300, mix and clarify, next addμL Tween 80, mix and clarify, next add μL ddH2O, mix and clarify.
Method for preparing in vivo formulation: Take μL DMSO master liquid, next add μL Corn oil, mix and clarify.
Note: 1. Please make sure the liquid is clear before adding the next solvent.
2. Be sure to add the solvent(s) in order. You must ensure that the solution obtained, in the previous addition, is a clear solution before proceeding to add the next solvent. Physical methods such as vortex, ultrasound or hot water bath can be used to aid dissolving.
3. All of the above co-solvents are available for purchase on the GlpBio website.
Quality Control & SDS
- View current batch:
- Purity: >97.00%
- COA (Certificate Of Analysis)
- SDS (Safety Data Sheet)
- Datasheet
Average Rating: 5 (Based on Reviews and 12 reference(s) in Google Scholar.)
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