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NovaFluor dyes, including NovaFluor Red 725 dye, are built using Phiton technology and are compatible with both spectral flow cytometry and traditional flow cytometry. NovaFluor dyes exhibit narrow emission spectra and minimal cross-laser excitation, which helps reduce spectral spillover for better marker resolution. In addition, their unique spectral signatures can provide the opportunity to detect additional markers in flow cytometry panels by opening up previously unusable channels.
NovaFluor Red 725 dye has a unique emission spectrum when excited by the 637nm laser, which fits in a spectral space that is currently not accessible by other spectral dyes. Adding spectrally unique dyes may allow for building out larger panels with minimal loss of resolution. NovaFluor Red 725 dye should generally be paired with moderately to lowly expressed antigens to minimize spectral spillover in complex multicolor panels. The macromolecule-based NovaFluor Red 725 dye produces highly stable fluorescence, and stained samples retain their fluorescence intensity and spectral signature when stored at 4°C.
Use NovaFluor dyes with CellBlox Blocking Buffer to reduce background and to block non-specific binding of NovaFluor labels, PE and APC tandems observed with macrophages and monocytes.
Initial brightness | The NovaFluor Red 725 dye, excited by the red laser is optimized for use for cell surface applications. Can be used for spectral and conventional flow cytometry applications. | ||
Photostability in buffer | |||
637 | 720/30 | 636 | 725 | ||
Laser line | Common filter set | Excitation max | Emission max |
We offer NovaFluor dyes conjugated to primary antibodies for use in flow cytometry, as well as NovaFluor Antibody Conjugation Kits, NovaFluor CD4 Label Characterization Kits, and custom conjugation services.
Figure 1. Absorption and fluorescence emission spectra of NovaFluor Red 725 dye.
Figure 2. Spectral signature of NovaFluor Red 725 dye. Normal human peripheral blood cells stained with anti-CD4 antibodies (clone SK3) conjugated to NovaFluor Red 725 dye were used for analysis. Data was acquired on a 5-laser Cytek Aurora system.
Figure 3. C57BL/6 mouse splenocytes were stained with CD3e monoclonal antibody, eFluor 450 dye (Cat. No. 48-0037-42) only (left) or along with CD45R monoclonal antibody, NovaFluor Red 725 dye (Cat. No. H029T03R05) (right). Viable cells were used for analysis, as determined by LIVE/DEAD Fixable Blue Dead Cell Stain Kit (Cat. No. L34962).
Figure 4. Normal human peripheral blood cells were stained with CD19 monoclonal antibody, eFluor 450 dye (Cat. No. 48-0199-42) only (left) or with CD4 monoclonal antibody, NovaFluor Red 725 dye (Cat. No. H001T03R05) (right). Cells in the lymphocyte gate were used for analysis.