Literature DB >> 23307900

Dissecting protein function: an efficient protocol for identifying separation-of-function mutations that encode structurally stable proteins.

Johnathan W Lubin1, Timsi Rao, Edward K Mandell, Deborah S Wuttke, Victoria Lundblad.   

Abstract

Mutations that confer the loss of a single biochemical property (separation-of-function mutations) can often uncover a previously unknown role for a protein in a particular biological process. However, most mutations are identified based on loss-of-function phenotypes, which cannot differentiate between separation-of-function alleles vs. mutations that encode unstable/unfolded proteins. An alternative approach is to use overexpression dominant-negative (ODN) phenotypes to identify mutant proteins that disrupt function in an otherwise wild-type strain when overexpressed. This is based on the assumption that such mutant proteins retain an overall structure that is comparable to that of the wild-type protein and are able to compete with the endogenous protein (Herskowitz 1987). To test this, the in vivo phenotypes of mutations in the Est3 telomerase subunit from Saccharomyces cerevisiae were compared with the in vitro secondary structure of these mutant proteins as analyzed by circular-dichroism spectroscopy, which demonstrates that ODN is a more sensitive assessment of protein stability than the commonly used method of monitoring protein levels from extracts. Reverse mutagenesis of EST3, which targeted different categories of amino acids, also showed that mutating highly conserved charged residues to the oppositely charged amino acid had an increased likelihood of generating a severely defective est3(-) mutation, which nevertheless encoded a structurally stable protein. These results suggest that charge-swap mutagenesis directed at a limited subset of highly conserved charged residues, combined with ODN screening to eliminate partially unfolded proteins, may provide a widely applicable and efficient strategy for generating separation-of-function mutations.

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Year:  2013        PMID: 23307900      PMCID: PMC3583993          DOI: 10.1534/genetics.112.147801

Source DB:  PubMed          Journal:  Genetics        ISSN: 0016-6731            Impact factor:   4.562


  34 in total

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3.  The Est3 protein is a subunit of yeast telomerase.

Authors:  T R Hughes; S K Evans; R G Weilbaecher; V Lundblad
Journal:  Curr Biol       Date:  2000-06-29       Impact factor: 10.834

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Authors:  S A Rudge; T R Pettitt; C Zhou; M J Wakelam; J A Engebrecht
Journal:  Genetics       Date:  2001-08       Impact factor: 4.562

5.  Senescence mutants of Saccharomyces cerevisiae with a defect in telomere replication identify three additional EST genes.

Authors:  T S Lendvay; D K Morris; J Sah; B Balasubramanian; V Lundblad
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Journal:  Genetics       Date:  1992-08       Impact factor: 4.562

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  8 in total

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Journal:  J Pediatr Genet       Date:  2020-10-05

2.  Structure of Est3 reveals a bimodal surface with differential roles in telomere replication.

Authors:  Timsi Rao; Johnathan W Lubin; Geoffrey S Armstrong; Timothy M Tucey; Victoria Lundblad; Deborah S Wuttke
Journal:  Proc Natl Acad Sci U S A       Date:  2013-12-16       Impact factor: 12.779

3.  Regulated assembly and disassembly of the yeast telomerase quaternary complex.

Authors:  Timothy M Tucey; Victoria Lundblad
Journal:  Genes Dev       Date:  2014-09-19       Impact factor: 11.361

4.  Ontogeny of Unstable Chromosomes Generated by Telomere Error in Budding Yeast.

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5.  Using Separation-of-Function Mutagenesis To Define the Full Spectrum of Activities Performed by the Est1 Telomerase Subunit in Vivo.

Authors:  Johnathan W Lubin; Timothy M Tucey; Victoria Lundblad
Journal:  Genetics       Date:  2017-11-29       Impact factor: 4.562

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8.  The N Terminus of the OB Domain of Telomere Protein TPP1 Is Critical for Telomerase Action.

Authors:  Sherilyn Grill; Valerie M Tesmer; Jayakrishnan Nandakumar
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  8 in total

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