Amersham CyDye DIGE Fluors, Cytiva

Supplier: Cytiva
CY™
RPK0273 25-8010-83 25-8010-85 RPK0275 RPK0272 25-8010-82 25-8008-61 25-8010-82 RPK0273 RPK0272 25-8010-85 RPK0275 25-8008-60 25-8010-83 25-8008-62
CA89129-270EA 2724.17 CAD
CA89129-270 89129-272 89129-270 CA89129-244 CA89129-242 89129-244 CA89129-274 89129-242 CA89129-240 CA89129-262 CA89129-272 89129-274 89129-240 CA89129-260 CA89129-258
Amersham CyDye DIGE Fluors, Cytiva
Protein Linking and Labeling Systems
CyDye™ DIGE fluors are available as minimal and saturation labeling dyes. The minimal dyes are intended for general 2-D application use where sufficient amounts of sample are available. The saturation dyes from the Scarce Sample Labeling Kit are designed to be used for applications where only small amounts of sample are available, for example in Laser Capture Microdissection.

  • Allow detection of up to three prelabelled protein samples and standards on the same 2-D electrophoresis gel
  • Size- and charge-matched dyes enable co-migration of labelled samples within the gel
  • Bright and highly sensitive dyes allow the use of the minimal labelling technique
  • Minimal loss of signal during labelling, separation, and scanning
  • No change in signal over wide pH range used during first-dimension (IEF) separation
  • Discrete signal from each fluor with minimal cross-talk contributes to high accuracy
  • Soluble in cold and hot water (solid)

CyDye™ DIGE fluors are exceptional dyes for multicolour analysis, offering bright and intense colours with narrow excitation and emission bands. The fluors are spectrally distinct, making them ideal for multicolour detection.

CyDye™ DIGE fluor minimal dyes:
Protein samples and the internal standard are each labeled with one CyDye™ DIGE fluor minimal dye. These labelled samples are then combined, run on an isoelectric focusing gel in the first dimension, and separated by SDS-PAGE in the second dimension.

The ability to multiplex different CyDye™ DIGE fluor minimal dye-labelled samples on the same gel means that the different samples will be subjected to exactly the same first- and second-dimension running conditions. Consequently, the same protein labelled with any of the CyDye™ DIGE fluor minimal dyes and separated on the same gel will migrate to the same position on the 2-D gel and overlay. This limits experimental variation and ensures accurate within-gel matching.

CyDye™ DIGE fluor labeling kits for scarce samples:
Protein samples and the internal standard are each labelled with one CyDye™ DIGE fluor minimal dye. These labelled samples are then combined, run on an isoelectric focusing gel in the first dimension, and separated by SDS-PAGE in the second dimension.

The NHS ester reactive group of CyDye™ DIGE fluor minimal dyes covalently attaches to the epsilon amino group of lysine of proteins via an amide linkage. The ratio of dye to protein has been designed to ensure the dyes are limiting in the reaction. As a result, approximately 3% of the available proteins are labelled and then only on a single lysine per protein (one dye per protein, or minimal labelling).

The amino acid lysine in proteins carries an intrinsic single positive charge at neutral or acidic pH. CyDye™ DIGE fluor minimal dyes also carry a single positive charge which, when coupled to the lysine, replaces the single positive charge of the lysine with its own, ensuring that the pI of the protein is not significantly altered when compared with the same unlabelled protein.

The fluors are spectrally distinct, making them highly suitable for multicolor detection. CyDye DIGE fluors utilize these benefits but are also size- and charge-matched for 2-D DIGE using Ettan DIGE system.
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