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1、Hotline: 400-820-3792Inhibitors Agonists Screening Librarieswww.MedChemENile Blue A sulfateCat. No.: HY-101900CAS No.: 3625-57-8Synonyms: Nile blue sulfate分式: CHNOS.分量: 366.42作靶点: Others作通路: Others储存式: 4C, protect from light* In solvent : -80C, 6 months; -20C, 1 month (protect fromlight)溶解性数据体外实验 DM
2、SO : 150 mg/mL (409.37 mM)* means soluble, but saturation unknown.Mass Solvent1 mg 5 mg 10 mg Concentration制备储备液1 mM 2.7291 mL 13.6455 mL 27.2911 mL5 mM 0.5458 mL 2.7291 mL 5.4582 mL10 mM 0.2729 mL 1.3646 mL 2.7291 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,并请注意储备液的保存式和期限。BIOLOGICAL ACTIVITY物活性 Nile Blue A可于区分素
3、和脂褐素。它也可于脂染,以及制备电流葡萄糖传感器。体外研究Nile blue A is a basic oxazine dye which is soluble in water and ethyl alcohol. Nile blue A is a satisfactorystain for PHB granules in bacteria and is in fact superior to Sudan black B for this purpose. Poly-p3-hydroxybutyrate granules exhibits a strong orange fluorescen
4、ce when stained with Nile blue A. Nile blue Aappears to stain many more PHB granules than Sudan black B does and is not as easily ished from the cell1/2 Master of Small Molecules 您边的抑制剂师www.MedChemEby decolorization procedures 1. Nile blue A is used as a stain for polyhydroxyalkanoic acid-accumulati
5、ngmicroorganisms or to detect polyhydroxyalkanoic acids in microorganisms. Escherichia coli cells that do notaccumulate detectable polyhydroxyalkanoic acids can be stained with Nile blue A and that this staining issufficient for identifying these cells in fluorescence-activated cell sorting (FACS) e
6、xperiments. Nile blue Astaining does not affect either surface display of peptides or specific labeling of these peptides by a secondfluorescence. Staining E. coli for flow cytometry using Nile blue A is an easy-to-handle and low-costalternative to other fluorescent dyes or the intracellular express
7、ion of, for example, green fluorescent protein2. Nile blue A is one of the most studied benzophenoxazine dyes, as a potent photosensitizer forphotodynamic therapy. The dye when administered intravenously disperses throughout the body bycirculating through blood and is taken up by most cells that emp
8、hasize its interaction with variousbiomolecule 3.PROTOCOLCell Assay 123 1% aqueous solution of Nile blue A is prepared and filtered before use. Mild heating may be necessary tofully dissolve the stain. Heat-fixed smears of bacterial cells are stained with the Nile blue A solution at 55Cfor 10 min in
9、 a coplin staining jar. After being stained, the slides are washed with tap water to remove excessstain and with 8% aqueous acetic acid for 1 min. The stained smear is washed and blotted dry with bibulouspaper, remoistened with tap water, and covered with a no. 1 glass cover slip. The preparation is
10、 examinedwith a Nikon Labphot microscope with an episcopic fluorescence attachment 1. The PHA strainEscherichia coli UT5600(DE3) is stained with Nile blue A. In an Erlenmeyer flask, 20 mL of LuriaBertani(LB) broth is inoculated with one colony of UT5600(DE3) and incubated for 14 h at 37 C and 200 rp
11、m.Subsequently, 20 mL of LB broth containing Nile blue A in a final concentration of 0.5 g/mL is inoculatedwith 200 L of the 14-h culture and cultured to an optical density at 578 nm (OD578) of 0.6. As a control, 20mL of LB broth (without Nile blue A) is inoculated with 200 L of the 14-h culture and
12、 is also cultured to anoptical density at OD578 of 0.6. Every 20 min, the OD578 is determined for both cultures to verify whetherthere is any influence of the dye on the growth of the bacteria 2. Nile blue A stock solution is prepared usingethanol as the solvent. The concentration of NB is maintaine
13、d at 5 M for all the studies. The solutions areleft for 1 h to achieve equilibrium before spectral measurements. The absorption spectra are recorded usingShimadzu Spectrophotometer (UV-1800) and the emission spectra are recorded using JobinYvonSpectrofluorimeter. A 450 nm nano-LED is used as the lig
14、ht source and the fluorescence lifetime is collectedat em=672 nm 3.MCE has not independently confirmed the accuracy of these methods. They are for reference only.REFERENCES1. Ostle AG, et al. Nile blue A as a fluorescent stain for poly-beta-hydroxybutyrate. Appl Environ Microbiol. 1982 Jul;44(1):238
15、-41.2. Betscheider D, et al. Nile blue A for staining Escherichia coli in flow cytometer experiments. Anal Biochem. 2009 Jan 1;384(1):194-6.3. Mishra SS, et al. Spectroscopic investigation of interaction of Nile Blue A, a potent photosensitizer, with bile salts in aqueous medium. JPhotochem Photobiol B. 2014 Dec;141:67-75.McePdfHeight2/2 Master
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