ProStain™ Protein Quantification Kit

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Determining the protein concentration of cell extracts is an essential step in many modern cell biology procedures, such as Western blot and ELISA. Not surprisingly, there are numerous photometric and fluorescent methods for quantifying cell extract protein levels. Photometric methods have traditionally been based either on intrinsic absorbance at 280 nm or on reagent-based methods such as the Bradford and Lowry assays. However, these classical approaches tend to be time consuming, have limited sensitivity and may be influenced by the presence of contaminating substances. Fluorescent-based detection methods, while generally more sensitive, have also tended to suffer from limitations, such as the requirement for toxic co-factors, high rates of hydrolysis or unsuitable spectral properties. The ProStain Kit offers significant improvements in sensitivity, assay robustness and convenience when compared with existing methods.

ProStain™ advantages

• Large Stokes shift and increased quantum yield of bound dye improve sensitivity and eliminate background
• Robust – limited effect from contaminating substances found in cell lysis buffers
• Fast and simple procedure for cell extract protein concentration determination
• ProStain dye has only one reactive group, preventing crosslinking-related issues
• Supplied ready to use, eliminating the need for activation steps prior to conjugation

Figure 1: Standard curves of BSA in various contaminants.

Increasing amounts of BSA protein were quantified using the ProStain Protein Quantification Kit in the presence of a variety of contaminants, demonstrating that ProStain is not influenced by these compounds.