Protein Binding of Antimicrobials: Methods for Quantification and for Investigation of its Impact on Bacterial Killing

Beer, Jürgen; Wagner, Cláudia; Zeitlinger, Markus

doi:10.1208/s12248-008-9072-1

Cited by 56 publications

(65 citation statements)

References 70 publications

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“…Available techniques for measurement of protein binding include equilibrium dialysis, ultrafiltration, ultracentrifugation, microdialysis, chromatographic methods, capillary electrophoresis, fluorescence spectroscopy, and ultrafast immunoextraction. These methods have been compared extensively in published review articles, and only an overview is provided here (16,48,49). With the exception of microdialysis, which may be applied in vivo to measure unbound drug concentrations, these methods are used in vitro for protein binding determination.…”

Section: Protein Binding Determinationmentioning

confidence: 99%

“…The impact of protein binding on drug efficacy will depend on the extent of the binding, PK properties, and intrinsic activity of the drug (11)(12)(13)(14)(15). In vitro, the impact of protein binding on antimicrobial activity is often investigated through determination of the MIC, time-kill curves, and cell culture assays (13,16). Numerous in vitro studies have been published, which evaluated the impact of protein binding on antimicrobials (17)(18)(19)(20)(21)(22)(23)(24)(25)(26)(27)(28), antivirals (29,30), and antifungals (31,32) by using protein supplements and/or serum to mimic in vivo conditions.…”

Section: Introductionmentioning

confidence: 99%

“…In the majority of studies, free drug concentrations are not measured directly in the experimental setting, and the extent of protein binding is accounted for by the using binding values reported in the literature. This approach can be misleading if the protein binding reported in the literature differs from the actual protein binding in the experimental setting (16,33).…”

Section: Introductionmentioning

confidence: 99%

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Importance of Relating Efficacy Measures to Unbound Drug Concentrations for Anti-Infective Agents

2013

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SUMMARY For the optimization of dosing regimens of anti-infective agents, it is imperative to have a good understanding of pharmacokinetics (PK) and pharmacodynamics (PD). Whenever possible, drug efficacy needs to be related to unbound concentrations at the site of action. For anti-infective drugs, the infection site is typically located outside plasma, and a drug must diffuse through capillary membranes to reach its target. Disease- and drug-related factors can contribute to differential tissue distribution. As a result, the assumption that the plasma concentration of drugs represents a suitable surrogate of tissue concentrations may lead to erroneous conclusions. Quantifying drug exposure in tissues represents an opportunity to relate the pharmacologically active concentrations to an observed pharmacodynamic parameter, such as the MIC. Selection of an appropriate specimen to sample and the advantages and limitations of the available sampling techniques require careful consideration. Ultimately, the goal will be to assess the appropriateness of a drug and dosing regimen for a specific pathogen and infection.

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Section: Protein Binding Determinationmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Importance of Relating Efficacy Measures to Unbound Drug Concentrations for Anti-Infective Agents

2013

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“…Such differences really matter, as the free fraction used as basis for PK/PD calculations could be assumed to be as low as 30% and 48% or as high as 60% and 75%, respectively. These differences are very likely due to methodological differences as reviewed previously [3,59], but the question is which of the published data should be selected for PK/PD calculations and based on which criteria?…”

Section: Discussionmentioning

confidence: 99%

“…It would therefore have been desirable to quantitate protein binding as well as free drug concentrations not only in the different serum preparations studied but also in the course of PK-simulations because of continuously fluctuating drug concentrations. However, quantitation of free drug concentrations is laborious and time consuming depending on the methods applied [3,59], so that total drug concentrations in the 7,224 samples withdrawn in this study were assayed instead and unspecific adsorption was avoided by siliconization of the glass-and plastic ware used. Although total drug concentrations varied by <5% from the theoretical concentrations suggesting that methodological errors can be excluded, this finding does not indicate that free drug levels were identical under the various conditions studied.…”

Section: Limitationsmentioning

confidence: 99%

The Impact of Protein Binding on Antibacterial Activities of Antibiotics is more than Predicted by Considering its Numerical Value Alone: Impact of Preparative and Incubation Methods on Different Pharmacodynamic Endpoints of ß-Lactams, Macrolides, or Fluoroquinolones Against Gram-positive and Gram-negative Bacteria-Part I

Dalhoff¹,

Schubert²

2016

J Clin Infect Dis Pract

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Objectives: Protein binding decreases antibacterial activities as the free fraction only crosses membranes thus reaching intracellular targets. However, serum components may also increase antibacterial activities. Therefore, the effect of serum proteins on activities of ß-lactams, macrolides, and fluoroquinolones was examined. Several preparation-and cultivation-conditions were examined as some preparative methods like freeze-thawing of sera may cause artifacts. Furthermore, previous studies have indicated that data may vary depending on the endpoints studied. Therefore, the aim of this study was to avoid an impact of methodological factors on the data generated and to analyse the activities of the study drugs by examining different static-or dynamic endpoints.Methods: Bacteria were grown in Brain Heart Infusion Broth (BHI), plus 50% of either fresh inactivated, pH 7.2, or fresh inactivated-, pH 7.2 or 8.2, frozen inactivated-serum, pH 8.2 as compared to BHI without any supplementations, pH 7.2 or 8.2, and BHI plus 45 g/L albumin. MICs of faropenem, amoxicillin, clarithromycin, azithromycin, moxifloxacin, and levofloxacin were determined and kill-kinetics were recorded following exposure to constant or fluctuating drug concentrations simulating serum pharmacokinetics of the agents. Kill-rates and areas under the bacterial kill curves were calculated.Results: Albumin and inactive serum increased MICs and reduced kill-rates of the agents studied in conformity with their protein binding, whereas active serum increased the activities of the agents. MICs and kill-rates did not change in parallel. The impact of protein binding in decreasing order was: MICs>kill-rates in time-kill experiments>kill-rates in kinetic-simulations. Macrolides and fluoroquinolones but not ß-lactams were more active at an alkaline-than neutral pH. Use of frozen sera caused alkalinization of media, thus generating artifacts. Conclusions:The impact of serum proteins on antibacterial activities is strongly dependent from three factors: the methods applied to prepare the serum pool, the incubation conditions, and the enpoints studied.

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Buur¹

2011

Comparative Pharmacokinetics

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Protein Binding of Antimicrobials: Methods for Quantification and for Investigation of its Impact on Bacterial Killing

Cited by 56 publications

References 70 publications

Importance of Relating Efficacy Measures to Unbound Drug Concentrations for Anti-Infective Agents

Importance of Relating Efficacy Measures to Unbound Drug Concentrations for Anti-Infective Agents

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