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PDBsum entry 1aaq
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Hydrolase/hydrolase inhibitor
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PDB id
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1aaq
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Contents |
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* Residue conservation analysis
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References listed in PDB file
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Key reference
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Title
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Hydroxyethylene isostere inhibitors of human immunodeficiency virus-1 protease: structure-Activity analysis using enzyme kinetics, X-Ray crystallography, And infected t-Cell assays.
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Authors
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G.B.Dreyer,
D.M.Lambert,
T.D.Meek,
T.J.Carr,
T.A.Tomaszek,
A.V.Fernandez,
H.Bartus,
E.Cacciavillani,
A.M.Hassell,
M.Minnich.
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Ref.
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Biochemistry, 1992,
31,
6646-6659.
[DOI no: ]
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PubMed id
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Abstract
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Analogues of peptides ranging in size from three to six amino acids and
containing the hydroxyethylene dipeptide isosteres Phe psi Gly, Phe psi Ala, Phe
psi NorVal, Phe psi Leu, and Phe psi Phe, where psi denotes replacement of CONH
by (S)-CH(OH)CH2, were synthesized and studied as HIV-1 protease inhibitors.
Inhibition constants (Ki) with purified HIV-1 protease depend strongly on the
isostere in the order Phe psi Gly greater than Phe psi Ala greater than Phe psi
NorVal greater than Phe psi Leu greater than Phe psi Phe and decrease with
increasing length of the peptide analogue, converging to a value of 0.4 nM. Ki
values are progressively less dependent on inhibitor length as the size of the
P1' side chain within the isostere increases. The structures of HIV-1 protease
complexed with the inhibitors Ala-Ala-X-Val-Val-OMe, where X is Phe psi Gly, Phe
psi Ala, Phe psi NorVal, and Phe psi Phe, have been determined by X-ray
crystallography (resolution 2.3-3.2 A). The crystals exhibit symmetry consistent
with space group P6(1) with strong noncrystallographic 2-fold symmetry, and the
inhibitors all exhibit 2-fold disorder. The inhibitors bind in similar
conformations, forming conserved hydrogen bonds with the enzyme. The Phe psi Gly
inhibitor adopts an altered conformation that places its P3' valine side chain
partially in the hydrophobic S1' pocket, thus suggesting an explanation for the
greater dependence of the Ki value on inhibitor length in the Phe psi Gly
series. From the kinetic and crystallographic data, a minimal inhibitor model
for tight-binding inhibition is derived in which the enzyme subsites S2-S2' are
optimally occupied. The Ki values for several compounds are compared with their
potencies as inhibitors of proteolytic processing in T-cell cultures chronically
infected with HIV-1 (MIC values) and as inhibitors of acute infectivity (IC50
values). There is a rank-order correspondence, but a 20-1000-fold difference,
between the values of Ki and those of MIC or IC50. IC50 values can approach
those of Ki but are highly dependent on the conditions of the acute infectivity
assay and are influenced by physiochemical properties of the inhibitors such as
solubility.
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