A naphthyridine carboxamide provides evidence for discordant resistance between mechanistically identical inhibitors of HIV-1 integrase

Hazuda, Daria J.; Anthony, Neville J.; Gomez, Robert; Jolly, Samson M.; Wai, John S.; Zhuang, Liujing; Fisher, Thorsten E.; Embrey, Mark W.; Guare, James P.; Egbertson, Melissa S.; Vacca, Joseph P.; Huff, Joel R.; Felock, Peter J.; Witmer, Marc; Stillmock, Kara A.; Danovich, Robert M.; Grobler, Jay A.; Miller, Michael D.; Espeseth, Amy S.; Jin, Lixia; Chen, I-Wu; Lin, Jiunn H.; Kassahun, Kelem; Ellis, Joan D.; Wong, Bradley K.; Xu, Wujie; Pearson, Paul G.; Schleif, William A.; Cortese, Riccardo; Emini, Emilio A.; Summa, Vincenzo; Holloway, M. Katharine; Young, Steven D.

doi:10.1073/pnas.0402357101

Cited by 319 publications

(308 citation statements)

References 30 publications

Supporting

Mentioning

292

Contrasting

Unclassified

Order By: Relevance

“…The N155H, Q148R, and E92Q enzymes were all between 4 and 15% as efficient as WT, with N155H being the weakest single variant (4%). The N155S virus has been reported to be less fit than WT (42,43), and the N155E, N155K, and N155L variants were reported to have 6% of WT strand transfer activity (44), similar to the N155H results reported here. T66I had a relative efficiency of 36%, indicating that this enzyme is not much altered catalytically, as compared with WT, similar to what has been reported previously (38).…”

Section: Discussionsupporting

confidence: 78%

Biochemical Analysis of HIV-1 Integrase Variants Resistant to Strand Transfer Inhibitors

Dicker

Terry

Lin

et al. 2008

Journal of Biological Chemistry

View full text Add to dashboard Cite

In this study, eight different HIV-1 integrase proteins containing mutations observed in strand transfer inhibitor-resistant viruses were expressed, purified, and used for detailed enzymatic analyses. All the variants examined were impaired for strand transfer activity compared with the wild type enzyme, with relative catalytic efficiencies (k p /K m ) ranging from 0.6 to 50% of wild type. The origin of the reduced strand transfer efficiencies of the variant enzymes was predominantly because of poorer catalytic turnover (k p ) values. However, smaller secondorder effects were caused by up to 4-fold increases in K m values for target DNA utilization in some of the variants. All the variants were less efficient than the wild type enzyme in assembling on the viral long terminal repeat, as each variant required more protein than wild type to attain maximal activity. In addition, the variant integrases displayed up to 8-fold reductions in their catalytic efficiencies for 3-processing. The Q148R variant was the most defective enzyme. The molecular basis for resistance of these enzymes was shown to be due to lower affinity binding of the strand transfer inhibitor to the integrase complex, a consequence of faster dissociation rates. In the case of the Q148R variant, the origin of reduced compound affinity lies in alterations to the active site that reduce the binding of a catalytically essential magnesium ion. Finally, except for T66I, variant viruses harboring the resistance-inducing substitutions were defective for viral integration.

show abstract

Section: Discussionsupporting

confidence: 78%

Biochemical Analysis of HIV-1 Integrase Variants Resistant to Strand Transfer Inhibitors

Dicker

Terry

Lin

et al. 2008

Journal of Biological Chemistry

View full text Add to dashboard Cite

show abstract

“…Published models of HIV IN (19,22) suggest that these specific STIs bind to the IN active site in a pocket flanked by the end of the LTR such that the diketoacid moiety, or its mimic, is positioned to coordinate with both of the catalytic magnesium atoms (23)(24)(25) (14,19,22,(26)(27)(28)(29). Amino acid substitutions which confer resistance to STIs cluster around the IN active site (30)(31)(32)(33)(34)(35)(36)(37), and changes to the 5′ end of the LTR reduce the affinity of a specific STI for its binding site (16). Published models do not address the issue of the precise placement of the 3′ terminus of the viral LTR in the inhibitor-bound state.…”

mentioning

confidence: 99%

The Terminal (Catalytic) Adenosine of the HIV LTR Controls the Kinetics of Binding and Dissociation of HIV Integrase Strand Transfer Inhibitors

et al. 2008

View full text Add to dashboard Cite

Specific HIV integrase strand transfer inhibitors are thought to bind to the integrase active site, positioned to coordinate with two catalytic magnesium atoms in a pocket flanked by the end of the viral LTR. A structural role for the 3′ terminus of the viral LTR in the inhibitor-bound state has not previously been examined. This study describes the kinetics of binding of a specific strand transfer inhibitor to integrase variants assembled with systematic changes to the terminal 3′ adenosine. Kinetic experiments are consistent with a two-step binding model in which there are different functions for the terminal adenine base and the terminal deoxyribose sugar. Adenine seems to act as a "shield" which retards the rate of inhibitor association with the integrase active site, possibly by acting as an internal competitive inhibitor. The terminal deoxyribose is responsible for retarding the rate of inhibitor dissociation, either by sterically blocking inhibitor egress or by a direct interaction with the bound inhibitor. These findings further our understanding of the details of the inhibitor binding site of specific strand transfer inhibitors.

show abstract

“…The activity of AZT and Raltegravir are consistent with previous reports in FIV/HIV. 51,52 Overall, these results indicate that the nucleocapsid protein of FIV can be targeted effectively with symmetrical dual functionality compounds with high efficacy. The relative simplicity and tractability of the synthetic approach makes these compounds attractive for further development and optimization.…”

Section: A R T Ic Le In F Omentioning

confidence: 75%

Novel fused tetrathiocines as antivirals that target the nucleocapsid zinc finger containing protein of the feline immunodeficiency virus (FIV) as a model of HIV infection

Asquith

Meli

Konstantinova

et al. 2015

Bioorganic & Medicinal Chemistry Letters

View full text Add to dashboard Cite

show abstract

A naphthyridine carboxamide provides evidence for discordant resistance between mechanistically identical inhibitors of HIV-1 integrase

Cited by 319 publications

References 30 publications

Biochemical Analysis of HIV-1 Integrase Variants Resistant to Strand Transfer Inhibitors

Biochemical Analysis of HIV-1 Integrase Variants Resistant to Strand Transfer Inhibitors

The Terminal (Catalytic) Adenosine of the HIV LTR Controls the Kinetics of Binding and Dissociation of HIV Integrase Strand Transfer Inhibitors

Novel fused tetrathiocines as antivirals that target the nucleocapsid zinc finger containing protein of the feline immunodeficiency virus (FIV) as a model of HIV infection

Contact Info

Product

Resources

About