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Mutagenesis-based definitions and probes of residue burial in proteins

Bajaj, Kanika and Chakrabarti, Purbani and Varadarajan, Raghavan (2005) Mutagenesis-based definitions and probes of residue burial in proteins. In: Proceedings of The National Academy of Sciences of The United States of America, 102 (45). pp. 16221-16226.

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Every residue of the 101-aa Escherichia, coli toxin CcdB was substituted with Ala, Asp, Glu, Lys, and Arg by using site-directed mutagenesis. The activity of each mutant in vivo was characterized as a function of Controller of Cell Division or Death B protein (CcdB) transcriptional level. The mutation data suggest that an accessibility value of 5% is an appropriate cutoff for definition of buried residues. At all buried positions, introduction of Asp results in an inactive phenotype at all CcdB transcriptional levels. The average amount of destabilization upon substitution at buried positions decreases in the order Asp>Glu>Lys>Arg>Ala. Asp substitutions at buried sites in two other proteins, maltose-binding protein and thioredoxin, also were shown to be severely destabilizing. Ala and Asp scanning mutagenesis, in combination with dose-dependent expression phenotypes, was shown to yield important information on protein structure and activity. These results also suggest that such scanning mutagenesis data can be used to rank order sequence alignments and their corresponding homology models, as well as to distinguish between correct and incorrect structural alignments. With continuous reductions in oligonucleotide costs and increasingly efficient site-directed mutagenesis procedures, comprehensive scanning mutagenesis experiments for small proteins/domains are quite feasible.

Item Type: Journal Article
Additional Information: Copyright for this article belongs to NATL Academic Sciences.
Department/Centre: Division of Biological Sciences > Molecular Biophysics Unit
Depositing User: B.S Priyanka
Date Deposited: 16 Dec 2005
Last Modified: 19 Sep 2010 04:22
URI: http://eprints.iisc.ac.in/id/eprint/4679

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