Protein Level Quantification Across Fluorescence-based Platforms
Biological processes are dependent on protein concentration and there is an inherent variability among cells even in environment-controlled conditions. Determining the amount of protein of interest in a cell is relevant to quantitatively relate it with the cells (patho)physiology. Previous studies u...
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Veröffentlicht in: | Bio-protocol 2023-10, Vol.13 (19), p.e4834-e4834 |
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Sprache: | eng |
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Zusammenfassung: | Biological processes are dependent on protein concentration and there is an inherent variability among cells even in environment-controlled conditions. Determining the amount of protein of interest in a cell is relevant to quantitatively relate it with the cells (patho)physiology. Previous studies used either western blot to determine the average amount of protein per cell in a population or fluorescence intensity to provide a relative amount of protein. This method combines both techniques. First, the protein of interest is purified, and its concentration determined. Next, cells containing the protein of interest with a fluorescent tag are sorted into different levels of intensity using fluorescence-activated cell sorting, and the amount of protein for each intensity category is calculated using the purified protein as calibration. Lastly, a calibration curve allows the direct relation of the amount of protein to the intensity levels determined with any instrument able to measure intensity levels. Once a fluorescence-based instrument is calibrated, it is possible to determine protein concentrations based on intensity.
Key features
• This method allows the evaluation and comparison of protein concentration in cells based on fluorescence intensity.
• Requires protein purification and fluorescence-activated cell sorting.
• Once calibrated for one protein, it allows determination of the levels of this protein using any fluorescence-based instrument.
• Allows to determine subcellular local protein concentration based on combining volumetric and intensity measurements. |
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ISSN: | 2331-8325 2331-8325 |
DOI: | 10.21769/BioProtoc.4834 |