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Probing the structure of falcipain‐3, a cysteine protease from Plasmodium falciparum : Comparative protein modeling and docking studies
Author(s) -
Sabnis Yogesh A.,
Desai Prashant V.,
Rosenthal Philip J.,
Avery Mitchell A.
Publication year - 2003
Publication title -
protein science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 3.353
H-Index - 175
eISSN - 1469-896X
pISSN - 0961-8368
DOI - 10.1110/ps.0228103
Subject(s) - cysteine protease , proteases , docking (animal) , homology modeling , plasmodium falciparum , cysteine , protease , computational biology , biology , protein structure , enzyme , biochemistry , chemistry , stereochemistry , malaria , medicine , immunology , nursing
Increasing resistance of malaria parasites to conventional antimalarial drugs is an important factor contributing to the persistence of the disease as a major health threat. The ongoing search for novel targets has resulted in identification and expression of several enzymes including cysteine proteases that are implicated in hemoglobin degradation. Falcipain‐2 and falcipain‐3 are considered to be the two principal cysteine proteases in this degradation, and hence, are potential drug targets. A homology model of falcipain‐3 was built and validated by various structure/geometry verification tools as well as docking studies of known substrates. The correlation coefficient of 0.975 between interaction energies and K m values of these substrates provided additional support for the model. On comparison with the previously reported falcipain‐2 homology model, the currently constructed falcipain‐3 structure showed important differences between the S2 pockets that might explain the variations in the K m values of various substrates for these enzymes. Further, docking studies also provided insight into possible binding modes and interactions of ligands with falcipain‐3. Results of the current study could be employed in de novo drug design leading to development of new antimalarial agents.

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