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Protein Science | 2008

Design of an engineered N-terminal HIV-1 gp41 trimer with enhanced stability and potency

John J. Dwyer; Karen L. Wilson; Kimberly Martin; Jennifer E. Seedorff; Aisha Hasan; Robyn J. Medinas; Donna K. Davison; Michael D. Feese; Hans-Thomas Richter; Hidong Kim; Thomas J. Matthews; Mary K. Delmedico

HIV fusion is mediated by a conformational transition in which the C‐terminal region (HR2) of gp41 interacts with the N‐terminal region (HR1) to form a six‐helix bundle. Peptides derived from the HR1 form a well‐characterized, trimeric coiled‐coil bundle in the presence of HR2 peptides, but there is little structural information on the isolated HR1 trimer. Using protein design, we have designed synthetic HR1 peptides that form soluble, thermostable HR1 trimers. In vitro binding of HR2 peptides to the engineered trimer suggests that the design strategy has not significantly impacted the ability to form the six‐helix bundle. The peptides have enhanced antiviral activity compared to wild type, with up to 30‐fold greater potency against certain viral isolates. In vitro passaging was used to generate HR1‐resistant virus and the observed resistance mutations map to the HR2 region of gp41, demonstrating that the peptides block the fusion process by binding to the viral HR2 domain. Interestingly, the activity of the HR2 fusion inhibitor, enfuvirtide (ENF), against these resistant viruses is maintained or improved up to fivefold. The 1.5 Å crystal structure of one of these designs has been determined, and we show that the isolated HR1 is very similar to the conformation of the HR1 in the six‐helix bundle. These results provide an initial model of the pre‐fusogenic state, are attractive starting points for identifying novel fusion inhibitors, and offer new opportunities for developing HIV therapeutics based on HR1 peptides.


Biochemistry | 1990

Crystal structure of the complex of carboxypeptidase A with a strongly bound phosphonate in a new crystalline form: comparison with structures of other complexes.

Hidong Kim; William N. Lipscomb


Biochemistry | 1995

Crystal structure of glycosomal glyceraldehyde-3-phosphate dehydrogenase from Leishmania mexicana: implications for structure-based drug design and a new position for the inorganic phosphate binding site.

Hidong Kim; Ingeborg K. Feil; Christophe L. M. J. Verlinde; Philip H. Petra; Wim G. J. Hol


Biochemistry | 1991

Comparison of the structures of three carboxypeptidase A-phosphonate complexes determined by X-ray crystallography.

Hidong Kim; William N. Lipscomb


Biochemistry | 1993

X-ray crystallographic determination of the structure of bovine lens leucine aminopeptidase complexed with amastatin : formulation of a catalytic mechanism featuring a gem-diolate transition state

Hidong Kim; William N. Lipscomb


Biochemistry | 1998

Crystal structure of fructose-1,6-bisphosphate aldolase from the human malaria parasite Plasmodium falciparum.

Hidong Kim; Ulrich Certa; Heinz Döbeli; Peter Jakob; Wim G. J. Hol


Protein Science | 1994

Protein crystallography and infectious diseases.

Christophe L. M. J. Verlinde; Ethan A. Merritt; F. Van Den Akker; Hidong Kim; I. K. Feil; L. F. Delboni; Shekhar C. Mande; Steve Sarfaty; Philip H. Petra; Wim G. J. Hol


Protein Science | 2008

The importance of dynamic light scattering in obtaining multiple crystal forms of trypanosoma brucei PGK

Bradley E. Bernstein; Paul A. M. Michels; Hidong Kim; Philip H. Petra; Wim G. J. Hol


Pharmaceutical Sciences Encyclopedia | 2010

Protein X-Ray Crystallography in Drug Discovery

Peter Nollert; Michael D. Feese; Bart L. Staker; Hidong Kim


Archive | 2001

Crystal compositions comprising topoisomerase i

Craig Behnke; Alex Burgin; Michael D. Feese; Kathryn Hjerrild; Hidong Kim; Bart L. Staker; Lance J. Stewart

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Wim G. J. Hol

University of Washington

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