Literature DB >> 16322566

Re-engineering redox-sensitive green fluorescent protein for improved response rate.

Mark B Cannon1, S James Remington.   

Abstract

Redox-sensitive variants of the green fluorescent protein (roGFPs) had previously been developed that allow "real-time" monitoring of the redox status of cellular compartments by fluorescence excitation ratiometry. However, the response time of these probes limits the study of certain rapid oxidative events, such as H2O2 bursts in cell signaling. The substitution of up to three positively charged amino acids adjacent to the introduced disulfide in roGFP1 (variants designated roGFP1-R1 through -R14) substantially improved the response rate. The pseudo first-order rate constants for oxidation by H2O2 and reduction by DTT and redox midpoint potentials were determined. The rate constants approximately doubled with each additional positively charged substitution, to nearly an order of magnitude total. The midpoint potentials are highly correlated with the rate increases, becoming more oxidizing with increasing numbers of positive substitutions. Crystal structures of two variants with opposite disulfide oxidation states have been determined: a 2.2 A resolution structure of oxidized "R7" containing two basic substitutions, and a 1.95 A resolution structure of reduced "R8" with one basic and one acidic substitution. Nonlinear Poisson-Boltzmann (PB) calculations are shown to accurately predict the effects of the substitutions on the rate constants. The effects of the substitutions on dimer formation, relative oxidative midpoint potentials, and oxidation and reduction rates are discussed. roGFPs are demonstrated to constitute an excellent model system for quantitative analysis of factors influencing thiol transfer reactions. roGFP1-R12 is most suitable for use in live cells, due to significantly increased reaction rate and increased pI.

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Year:  2005        PMID: 16322566      PMCID: PMC2242357          DOI: 10.1110/ps.051734306

Source DB:  PubMed          Journal:  Protein Sci        ISSN: 0961-8368            Impact factor:   6.725


  47 in total

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2.  Prediction of pKa and redox properties in the thioredoxin superfamily.

Authors:  Efrosini Moutevelis; Jim Warwicker
Journal:  Protein Sci       Date:  2004-08-31       Impact factor: 6.725

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4.  The crystallographically determined structures of atypical strained disulfides engineered into subtilisin.

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5.  The molecular structure of green fluorescent protein.

Authors:  F Yang; L G Moss; G N Phillips
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6.  Why is DsbA such an oxidizing disulfide catalyst?

Authors:  U Grauschopf; J R Winther; P Korber; T Zander; P Dallinger; J C Bardwell
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7.  Microscopic pKa values of Escherichia coli thioredoxin.

Authors:  P T Chivers; K E Prehoda; B F Volkman; B M Kim; J L Markley; R T Raines
Journal:  Biochemistry       Date:  1997-12-02       Impact factor: 3.162

8.  Active site labeling of the Yersinia protein tyrosine phosphatase: the determination of the pKa of the active site cysteine and the function of the conserved histidine 402.

Authors:  Z Y Zhang; J E Dixon
Journal:  Biochemistry       Date:  1993-09-14       Impact factor: 3.162

9.  Characterization of ferredoxin:thioredoxin reductase modified by site-directed mutagenesis.

Authors:  Dominique A Glauser; Florence Bourquin; Wanda Manieri; Peter Schürmann
Journal:  J Biol Chem       Date:  2004-02-09       Impact factor: 5.157

10.  Differential reactivity of the functional sulfhydryl groups of cysteine-32 and cysteine-35 present in the reduced form of thioredoxin from Escherichia coli.

Authors:  G B Kallis; A Holmgren
Journal:  J Biol Chem       Date:  1980-11-10       Impact factor: 5.157

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  28 in total

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5.  Mitochondrial-targeted nitroxides disrupt mitochondrial architecture and inhibit expression of peroxiredoxin 3 and FOXM1 in malignant mesothelioma cells.

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6.  Targeting Mycobacterium tuberculosis Sensitivity to Thiol Stress at Acidic pH Kills the Bacterium and Potentiates Antibiotics.

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8.  Rapid cell death is preceded by amyloid plaque-mediated oxidative stress.

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9.  An integrated imaging approach to the study of oxidative stress generation by mitochondrial dysfunction in living cells.

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