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Trp42 rotamers report reduced flexibility when the inhibitor acetyl-pepstatin is bound to HIV-1 protease

Published online by Cambridge University Press:  15 December 2000

BEÁTA ULLRICH
Affiliation:
Institute of Biophysics and Radiation Biology, Semmelweis University, P.O.B. 263 H-1444 Budapest, Hungary
MONIQUE LABERGE
Affiliation:
Institute of Biophysics and Radiation Biology, Semmelweis University, P.O.B. 263 H-1444 Budapest, Hungary
FERENC TÖLGYESI
Affiliation:
Institute of Biophysics and Radiation Biology, Semmelweis University, P.O.B. 263 H-1444 Budapest, Hungary
ZOLTÁN SZELTNER
Affiliation:
Institute of Enzymology, Biological Research Centre, Hungarian Academy of Sciences, P.O.B. 7, H-1518 Budapest, Hungary
LÁSZLÓ POLGÁR
Affiliation:
Institute of Enzymology, Biological Research Centre, Hungarian Academy of Sciences, P.O.B. 7, H-1518 Budapest, Hungary
JUDIT FIDY
Affiliation:
Institute of Biophysics and Radiation Biology, Semmelweis University, P.O.B. 263 H-1444 Budapest, Hungary
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Abstract

The Q7K/L33I/L63I HIV-1 protease mutant was expressed in Escherichia coli and the effect of binding a substrate-analog inhibitor, acetyl-pepstatin, was investigated by fluorescence spectroscopy and molecular dynamics. The dimeric enzyme has four intrinsic tryptophans, located at positions 6 and 42 in each monomer. Fluorescence spectra and acrylamide quenching experiments show two differently accessible Trp populations in the apoenzyme with kq1 = 6.85 × 109 M−1 s−1 and kq2 = 1.88 × 109 M−1 s−1, that merge into one in the complex with kq = 1.78 × 109 M−1 s−1.

500 ps trajectory analysis of Trp χ12 rotameric interconversions suggest a model to account for the observed Trp fluorescence. In the simulations, Trp6/Trp6B rotameric interconversions do not occur on this timescale for both HIV forms. In the apoenzyme simulations, however, both Trp42s and Trp42Bs are flipping between χ12 states; in the complexed form, no such interconverions occur. A detailed investigation of the local Trp environments sampled during the molecular dynamics simulation suggests that one of the apoenzyme Trp42B rotameric interconversions would allow indole-quencher contact, such as with nearby Tyr59. This could account for the short lifetime component. The model thus interprets the experimental data on the basis of the conformational fluctuations of Trp42s alone. It suggests that the rotameric interconversions of these Trps, located relatively far from the active site and at the very start of the flap region, becomes restrained when the apoenzyme binds the inhibitor. The model is thus consistent with associating components of the fluorescence decay in HIV-1 protease to ground state conformational heterogeneity.

Type
Research Article
Copyright
2000 The Protein Society

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