AI Article Synopsis
- Alternative methods for detecting proteins in polyacrylamide gels are outlined, which do not require fixation before or during staining.
- Skipping the fixation step allows for easier retrieval of proteins for further analysis, though these non-fixation methods generally have lower sensitivity compared to fixation methods.
- Several techniques for protein detection are detailed, including SDS precipitation, contact blots, imidazole-zinc staining, fluorescent labels, as well as additional methods like tryptophan fluorescence and minimal protein staining.
Article Abstract
A number of alternative methods are described for detecting proteins in polyacrylamide gels that do not require fixation of the protein either prior to staining or in conjunction with staining. The primary advantage of avoiding fixation is that this makes it easier to remove proteins of interest from the gels for subsequent analysis. In general, the sensitivity of protein detection methods that avoid fixation is lower than for detection methods using fixation. For any given method, sensitivity is dependent on the volume of the protein band within the gel; hence, sensitivity is highest for sharp, narrow bands. Techniques described in this unit include protocols for protein detection in gels by SDS precipitation, preparation of contact blots, staining with imidazole-zinc, and use of the fluorescent labels IAEDANS and fluorescamine. Several additional methods, including the use of tryptophan fluorescence, guide strips, and minimal protein staining, are discussed in the Commentary.
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| http://dx.doi.org/10.1002/0471140864.ps1006s48 | DOI Listing |
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