Literature DB >> 21333792

Using tryptophan fluorescence to measure the stability of membrane proteins folded in liposomes.

C Preston Moon1, Karen G Fleming.   

Abstract

Accurate measurements of the thermodynamic stability of folded membrane proteins require methods for monitoring their conformation that are free of experimental artifacts. For tryptophan fluorescence emission experiments with membrane proteins folded into liposomes, there are two significant sources of artifacts: the first is light scattering by the liposomes; the second is the nonlinear relationship of some tryptophan spectral parameters with changes in protein conformation. Both of these sources of error can interfere with the method of determining the reversible equilibrium thermodynamic stability of proteins using titrations of chemical denaturants. Here, we present methods to manage light scattering by liposomes for tryptophan emission experiments and to properly monitor tryptophan spectra as a function of protein conformation. Our methods are tailored to the titrations of membrane proteins using common chemical denaturants. One of our recommendations is to collect and analyze the right-angle light scattering peak that occurs around the excitation wavelength in a fluorescence experiment. Another recommendation is to use only those tryptophan spectral parameters that are linearly proportional to the protein conformational population. We show that other commonly used spectral parameters lead to errors in protein stability measurements.
Copyright © 2011 Elsevier Inc. All rights reserved.

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Year:  2011        PMID: 21333792      PMCID: PMC3799943          DOI: 10.1016/B978-0-12-381268-1.00018-5

Source DB:  PubMed          Journal:  Methods Enzymol        ISSN: 0076-6879            Impact factor:   1.600


  15 in total

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5.  Light scattering and turbidity measurements on lipid vesicles.

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7.  The transition state for folding of an outer membrane protein.

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8.  Fluorescence and the location of tryptophan residues in protein molecules.

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  32 in total

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Journal:  J Mol Biol       Date:  2011-08-24       Impact factor: 5.469

4.  Side-chain hydrophobicity scale derived from transmembrane protein folding into lipid bilayers.

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5.  Assessing and Improving Protein Sample Quality.

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8.  Negative Charge Neutralization in the Loops and Turns of Outer Membrane Phospholipase A Impacts Folding Hysteresis at Neutral pH.

Authors:  Sarah K McDonald; Karen G Fleming
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9.  Slow Interconversion in a Heterogeneous Unfolded-State Ensemble of Outer-Membrane Phospholipase A.

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10.  Influence of circular permutations on the structure and stability of a six-fold circular symmetric designer protein.

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