A simple dual selection for functionally active mutants of Plasmodium falciparum dihydrofolate reductase with improved solubility

doi:10.1093/protein/gzi044

PEDS Advance Access published online on August 24, 2005
Protein Engineering Design and Selection, doi:10.1093/protein/gzi044

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© The Author 2005. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oupjournals.org
Received March 10, 2005
Revised June 16, 2005
Accepted June 17, 2005

Article

A simple dual selection for functionally active mutants of Plasmodium falciparum dihydrofolate reductase with improved solubility

D. Japrung ¹, S. Chusacultanachai ², J. Yuvaniyama ³, P. Wilairat ⁴, and Y. Yuthavong ²^*

¹ National Center for Genetic Engineering and Biotechnology, National Science and Technology Development Agency, Science Park, Pathumthani 12120, Thailand; Department of Biochemistry, Faculty of Science, Mahidol University, Rama 6 Road, Bangkok 10400, Thailand
² National Center for Genetic Engineering and Biotechnology, National Science and Technology Development Agency, Science Park, Pathumthani 12120, Thailand
³ Center for Excellence in Protein Structure and Function, Mahidol University, Rama 6 Road, Bangkok 10400, Thailand; Department of Biochemistry, Faculty of Science, Mahidol University, Rama 6 Road, Bangkok 10400, Thailand
⁴ Department of Biochemistry, Faculty of Science, Mahidol University, Rama 6 Road, Bangkok 10400, Thailand

^* To whom correspondence should be addressed.
Y. Yuthavong, E-mail: yongyuth{at}nstda.or.th

Abstract

Sufficient solubility of the active protein in aqueous solutionis a prerequisite for crystallization and other structural studiesof proteins. In this study, we have developed a simple and effectivein vivo screening system to select for functionally active proteinswith increased solubility by using Plasmodium falciparum dihydrofolatereductase (pfDHFR), a well-known malarial drug target, as amodel. Prior to the dual selection process, pfDHFR was fusedto green fluorescent protein (GFP), which served as a reporterfor solubility. The fusion gene was used as a template for constructionof mutated DNA libraries of pfDHFR. Two amino acids with largehydrophobic side chains (Y35 and F37) located on the surfaceof pfDHFR were selected for site-specific mutagenesis. Additionally,the entire pfDHFR gene was randomly mutated using error-pronePCR. During the first step of the dual selection, mutants withfunctionally active pfDHFR were selected from two librariesby using bacterial complementation assay. Fluorescence signalsof active mutants were subsequently measured and five mutantswith increased GFP signal, namely Y35Q + F37R, Y35L + F37T,Y35G + F37L and Y35L + F37R from the site-specific mutant libraryand K27E from the random mutant library, were recovered. Themutants were expressed, purified and characterized as monofunctionalpfDHFR following excision of GFP. Our studies indicated thatall mutant pfDHFRs exhibited kinetic properties similar to thatof the wild-type protein. For comparison of protein solubility,the maximum concentrations of mutant enzymes prior to aggregationwere determined. All mutants selected in this study exhibited3- to 6-fold increases in protein solubility compared with thewild-type protein, which readily aggregated at 2 mg/ml. Thedual selection system we have developed should be useful forengineering functionally active protein mutants with sufficientsolubility for functional/structural studies and other applications.

Keywords: dihydrofolate reductase; error-prone PCR; green fluorescent protein; Plasmodium falciparum; protein solubility.

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