Marta G. Williams scite author profile

Recently, cyclooctylpyranone derivatives with m-carboxamide substituents (e.g. 2c) were identified as potent, nonpeptidic HIV protease inhibitors, but these compounds lacked significant antiviral activity in cell culture. Substitution of a sulfonamide group at the meta position, however, produces compounds with excellent HIV protease binding affinity and antiviral activity. Guided by an iterative structure-based drug design process, we have prepared and evaluated a number of these derivatives, which are readily available via a seven-step synthesis. A few of the most potent compounds were further evaluated for such characteristics as pharmacokinetics and toxicity in rats and dogs. From this work, the p-cyanophenyl sulfonamide derivative 35k emerged as a promising inhibitor, was selected for further development, and entered phase I clinical trials.

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Synthesis and DNA crosslinking by a rigid CPI dimer

Mitchell¹,

Kelly²,

Wicnienski³

et al. 1991

J. Am. Chem. Soc.

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Simultaneous quantitation of pioglitazone and its metabolites in human serum by liquid chromatography and solid phase extraction

Zhong

Williams

1996

Journal of Pharmaceutical and Biomedical Analysis

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Interstrand DNA cross-linking with dimers of the spirocyclopropyl alkylating moiety of CC-1065

Mitchell¹,

Johnson²,

Williams³

et al. 1989

J. Am. Chem. Soc.

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Rapid determination of rat plasma uridine levels by HPLC‐ESI‐MS utilizing the Captiva™ filter plates for sample preparation

Williams¹,

Palandra²,

Shobe³

2003

Biomedical Chromatography

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A rapid, accurate and precise HPLC-ESI-MS method for the determination of rat plasma uridine concentrations was developed and is described here. Sample preparation involves methanol precipitation of plasma proteins in a 96-well Captiva protein precipitation filter plate. A clear extract is drawn through the filter plate with vacuum, followed by evaporation of the extract and subsequent reconstitution prior to chromatography on a reversed-phase column with an aqueous mobile phase [0.1% (v/v) glacial acetic acid]. Detection was accomplished by positive-ion electrospray ionization mass spectrometry. A calibration curve ranging in concentration from 0.78 to 25 microM was constructed by best-fit, 1/x weighting linear regression analysis of the calibration standard concentrations vs peak height ratios of analyte with internal standard. The correlation coefficient was >0.995. The overall assay accuracy as shown by the back-calculated concentrations of the calibration curve ranged from 96.6 to 103% with RSD ranging from 4.5 to 20%. While this assay method was developed for the determination of uridine in rat plasma, it could be readily adapted for determination of uridine in plasma from other species, such as human.

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Marta G. Williams

Structure-Based Design of Nonpeptidic HIV Protease Inhibitors: The Sulfonamide-Substituted Cyclooctylpyranones

Synthesis and DNA crosslinking by a rigid CPI dimer

Simultaneous quantitation of pioglitazone and its metabolites in human serum by liquid chromatography and solid phase extraction

Interstrand DNA cross-linking with dimers of the spirocyclopropyl alkylating moiety of CC-1065

Rapid determination of rat plasma uridine levels by HPLC‐ESI‐MS utilizing the Captiva™ filter plates for sample preparation

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