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Biotechnology and Bioengineering
Article . 2005 . Peer-reviewed
License: Wiley Online Library User Agreement
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High‐throughput measurement of protein stability in microtiter plates

Authors: Jean P, Aucamp; Ana M, Cosme; Gary J, Lye; Paul A, Dalby;

High‐throughput measurement of protein stability in microtiter plates

Abstract

AbstractThe direct determination of protein stability at high throughput has applications in proteomics, directed evolution, and formulation. Each application places different requirements on the accuracy of stability or transition midpoint determination. The measurement of protein stability by chemical denaturation has been previously performed at medium throughput and high accuracy using autotitrating fluorometers, after removal of proteins from the 96‐well plate format in which they were expressed and purified. Herein we present a higher‐throughput method for measuring and indexing the stability of proteins maintained within the 96‐well format using a fluorescence microplate reader. Protein unfolding transitions were monitored by tryptophan fluorescence at 340 nm and assessed using bovine and equine cytochrome c (cyt c), as well as bovine serum albumin (BSA) stabilized with various amounts of palmitic acid. Two different approaches for generating unfolding curves in microtiter plates have been evaluated for their accuracy and applicability. Unfolding curves generated by the serial addition of denaturant into single wells allowed high‐throughput stability screens capable of identifying protein variants with unfolding midpoint differences of 0.15 M denaturant concentration or larger. Such a method would be suitable for screening large numbers of proteins, as typically generated for directed evolution. Unfolding curves generated using one well per denaturant concentration allowed for medium‐throughput stability screening and generated more accurate and precise stability values (C1/2 ± 0.05 M, mG, and ΔG) for cyt c that are similar to values reported in literature. This method is suitable for screening the smaller numbers of proteins generated in proteomic research programmes. By using BSA stabilized with various palmitate concentrations and simple numerical indexing, it was shown that both experimental methods can successfully rank the order of protein stability. © 2005 Wiley Periodicals, Inc.

Keywords

Protein Denaturation, Protein Folding, Dose-Response Relationship, Drug, Protein Conformation, Proteins, Cytochrome c Group, Serum Albumin, Bovine, Bioreactors, Animals, Thermodynamics, Urea, Cattle, Horses

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selected citations
These citations are derived from selected sources.
This is an alternative to the "Influence" indicator, which also reflects the overall/total impact of an article in the research community at large, based on the underlying citation network (diachronically).
BIP!Citations provided by BIP!
popularity
This indicator reflects the "current" impact/attention (the "hype") of an article in the research community at large, based on the underlying citation network.
BIP!Popularity provided by BIP!
influence
This indicator reflects the overall/total impact of an article in the research community at large, based on the underlying citation network (diachronically).
BIP!Influence provided by BIP!
impulse
This indicator reflects the initial momentum of an article directly after its publication, based on the underlying citation network.
BIP!Impulse provided by BIP!
48
Top 10%
Top 10%
Top 10%
bronze