In vitro resistance studies of hepatitis C virus serine protease inhibitors, VX-950 and BILN 2061 - Structural analysis indicates different resistance mechanisms
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Lin, C
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Lin, C
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Lin, K
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Lin, K
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Luong, YP
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Luong, YP
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Rao, BG
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Rao, BG
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Wei, YY
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Wei, YY
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Brennan, DL
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Brennan, DL
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Fulghum, JR
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Fulghum, JR
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Hsiao, HM
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Hsiao, HM
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Ma, S
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Ma, S
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Maxwell, JP
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Maxwell, JP
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Cottrell, KM
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Cottrell, KM
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Perni, RB
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Vertex Pharmaceut Inc, Cambridge, MA 02139 USAVertex Pharmaceut Inc, Cambridge, MA 02139 USA
Perni, RB
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Gates, CA
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Gates, CA
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Kwong, AD
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Kwong, AD
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[1] Vertex Pharmaceut Inc, Cambridge, MA 02139 USA
We have used a structure-based drug design approach to identify small molecule inhibitors of the hepatitis C virus (HCV) NS3.4A protease as potential candidates for new anti-HCV therapies. VX-950 is a potent NS3.4A protease inhibitor that was recently selected as a clinical development candidate for hepatitis C treatment. In this report, we describe in vitro resistance studies using a subgenomic replicon system to compare VX-950 with another HCV NS3.4A protease inhibitor, BILN 2061, for which the Phase I clinical trial results were reported recently. Distinct drug-resistant substitutions of a single amino acid were identified in the HCV NS3 serine protease domain for both inhibitors. The resistance conferred by these mutations was confirmed by characterization of the mutant enzymes and replicon cells that contain the single amino acid substitutions. The major BILN 2061-resistant mutations at Asp(168) are fully susceptible to VX-950, and the dominant resistant mutation against VX-950 at Ala(156) remains sensitive to BILN 2061. Modeling analysis suggests that there are different mechanisms of resistance to VX-950 and BILN 2061.