Brilliant Violet™ 786 Dye | Thermo Fisher Scientific

Brilliant Violet 786 excitation shown as dotted line and emission shown as solid red histogram


3	405	780/60, 750 LP	406	788	(in buffer) 3	flow cytometry

Invitrogen Brilliant Violet™ 786 (BV786) is a tandem dye excited by the 405 nm violet laser and emits at 786 nm. This dye has a medium relative brightness and can be used for cell surface, intracellular, and nuclear staining.

When using two or more Super Bright, Brilliant Violet™, Brilliant Ultra Violet™, or other polymer dye- conjugated antibodies in a staining panel, we recommend using Super Bright Complete Staining Buffer or Brilliant Stain Buffer to minimize any non-specific polymer interactions.

We offer BV786 dye conjugated to primary antibodies for use in flow cytometry.

Search Brilliant Violet™ 786 primary antibodies

Additional products

Control antibodies for flow cytometry

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Experimental data using Brilliant Violet™ 786

Graph of fluorescence intensity vs Channel for Brilliant Violet dye 786

Click image to enlarge

Spectral signature of Brilliant Violet™ 786 dye. Data acquired on a 5-laser Cytek Aurora and normal human peripheral blood cells stained with CD8a Monoclonal Antibody, Brilliant Violet™ 786 were used for analysis.

Dot plot of Ki-67 BV786 vs CD45R (B220) FITC in unstimulated and stimulated cells

Intracellular staining of mouse splenocytes using Brilliant Violet™ 786. C57BL/6 mouse splenocytes were unstimulated (left) or stimulated for 48 hours with CD3e Monoclonal Antibody, Functional Grade (right). Cells were then surface-stained with CD45R (B220) Monoclonal Antibody, FITC and stained intracellularly, using the Foxp3/Transcription Factor Staining Buffer Set and protocol, with 1.0 µg of Ki-67 Monoclonal Antibody (SolA15), Brilliant Violet™ 786. Viable cells in the lymphocyte gate were used for analysis, as determined by LIVE/DEAD™ Fixable Blue Dead Cell Stain Kit, for UV excitation.

Dot plot of samples stained with IgG2a control vs CD4-FITC and CD8a-BV786 vs CD4-FITC

Cell surface staining of mouse splenocytes using Brilliant Violet™ 786. C57BL/6 mouse splenocytes were stained with CD4 Monoclonal Antibody, FITC and 0.25 µg of Rat IgG2a kappa Isotype Control, Brilliant Violet™ 786 (left) or 0.25 µg of CD8a Monoclonal Antibody, Brilliant Violet™ 786 (right). Viable cells in the lymphocyte gate were used for analysis, as determined by 7-AAD Viability Staining Solution.

Brilliant Ultra Violet™ dye background

Brilliant Ultra Violet dyes are a polymer dye-based technology and compatible with both spectral flow cytometry as well as traditional flow cytometry. The UV laser has unique channels far from heavily occupied detectors, allowing for larger panels.