Pharmacokinetics-Pharmacodynamics of a Novel β-Lactamase Inhibitor, CB-618, in Combination with Meropenem in an In Vitro Infection Model

Brian D VanScoy; Michael Trang; Jennifer McCauley; Haley Conde; Sujata M Bhavnani; Lawrence V Friedrich; Dylan C Alexander; Paul G Ambrose

doi:10.1128/AAC.02943-15

Pharmacokinetics-Pharmacodynamics of a Novel β-Lactamase Inhibitor, CB-618, in Combination with Meropenem in an In Vitro Infection Model

Antimicrob Agents Chemother. 2016 Jun 20;60(7):3891-6. doi: 10.1128/AAC.02943-15. Print 2016 Jul.

Authors

Brian D VanScoy¹, Michael Trang¹, Jennifer McCauley¹, Haley Conde¹, Sujata M Bhavnani¹, Lawrence V Friedrich², Dylan C Alexander², Paul G Ambrose³

Affiliations

¹ Institute for Clinical Pharmacodynamics, Latham, New York, USA.
² Merck and Co., Kenilworth, New Jersey, USA.
³ Institute for Clinical Pharmacodynamics, Latham, New York, USA University of Oxford, Oxford, United Kingdom PAmbrose@ICPD.com.

Abstract

The usefulness of β-lactam antimicrobial agents is threatened as never before by β-lactamase-producing bacteria. For this reason, there has been renewed interest in the development of broad-spectrum β-lactamase inhibitors. Herein we describe the results of dose fractionation and dose-ranging studies carried out using a one-compartment in vitro infection model to determine the exposure measure for CB-618, a novel β-lactamase inhibitor, most predictive of the efficacy when given in combination with meropenem. The challenge panel included Enterobacteriaceae clinical isolates, which collectively produced a wide range of β-lactamase enzymes (KPC-2, KPC-3, FOX-5, OXA-48, SHV-11, SHV-27, and TEM-1). Human concentration-time profiles were simulated for each drug, and samples were collected for drug concentration and bacterial density determinations. Using data from dose fractionation studies and a challenge Klebsiella pneumoniae isolate (CB-618-potentiated meropenem MIC = 1 mg/liter), relationships between change from baseline in log10 CFU/ml at 24 h and each of CB-618 area under the concentration-time curve over 24 h (AUC0-24), maximum concentration (Cmax), and percentage of the dosing interval that CB-618 concentrations remained above a given threshold were evaluated in combination with meropenem at 2 g every 8 h (q8h). The exposure measures most closely associated with CB-618 efficacy in combination with meropenem were the CB-618 AUC0-24 (r(2) = 0.835) and Cmax (r(2) = 0.826). Using the CB-618 AUC0-24 indexed to the CB-618-potentiated meropenem MIC value, the relationship between change from baseline in log10 CFU/ml at 24 h and CB-618 AUC0-24/MIC ratio in combination with meropenem was evaluated using the pooled data from five challenge isolates; the CB-618 AUC0-24/MIC ratio associated with net bacterial stasis and the 1- and 2-log10 CFU/ml reductions from baseline at 24 h were 27.3, 86.1, and 444.8, respectively. These data provide a pharmacokinetics-pharmacodynamics (PK-PD) basis for evaluating potential CB-618 dosing regimens in combination with meropenem in future studies.

MeSH terms

Anti-Bacterial Agents / pharmacokinetics
Anti-Bacterial Agents / pharmacology*
Klebsiella pneumoniae / drug effects*
Klebsiella pneumoniae / metabolism
Meropenem
Microbial Sensitivity Tests
Thienamycins / pharmacokinetics
Thienamycins / pharmacology*
beta-Lactamase Inhibitors / pharmacokinetics
beta-Lactamase Inhibitors / pharmacology*

Substances

Anti-Bacterial Agents
Thienamycins
beta-Lactamase Inhibitors
Meropenem