Protein analysis using real‐time PCR instrumentation: Incorporation in an integrated, inquiry‐based project
Instrumentation for real‐time PCR is used primarily for amplification and quantitation of nucleic acids. The capability to measure fluorescence while controlling temperature in multiple samples can also be applied to the analysis of proteins. Conformational stability and changes in stability due to...
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Veröffentlicht in: | Biochemistry and molecular biology education 2014-03, Vol.42 (2), p.142-151 |
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Sprache: | eng |
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Zusammenfassung: | Instrumentation for real‐time PCR is used primarily for amplification and quantitation of nucleic acids. The capability to measure fluorescence while controlling temperature in multiple samples can also be applied to the analysis of proteins. Conformational stability and changes in stability due to ligand binding are easily assessed. Protein structure studies possible with a real‐time PCR instrument address core topics in biochemistry and have valuable high‐throughput applications in the fields of drug discovery and protein engineering. Protein analysis using real‐time PCR instrumentation has been incorporated in an undergraduate laboratory project based on previously described projects. Students express, purify, and characterize a protein. Based on literature research and analysis using bioinformatics tools, they select a specific mutation to investigate. They then attempt to express, purify, and characterize their mutated protein. Thermal denaturation using a real‐time PCR instrument is the primary tool used to compare the wild‐type and mutated proteins. Alternative means for incorporation of protein analysis by real‐time PCR instrumentation into laboratory experiences and additional modes of analysis are also described. © 2013 by The International Union of Biochemistry and Molecular Biology, 42(2):142–151, 2014 |
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ISSN: | 1470-8175 1539-3429 |
DOI: | 10.1002/bmb.20747 |