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dc.contributor.authorIzes, Aaron M.en_AU
dc.contributor.authorKimble, Benjaminen_AU
dc.contributor.authorNorris, Jacqueline M.en_AU
dc.contributor.authorGovendir, Merranen_AU
dc.date.accessioned2020-09-24
dc.date.available2020-09-24
dc.date.issued2020en_AU
dc.identifier.urihttps://hdl.handle.net/2123/23460
dc.description.abstractThe antimalarial agent mefloquine is currently being investigated for its potential to inhibit feline coronavirus and feline calicivirus infections. A simple, high pressure liquid chromatography assay was developed to detect mefloquine plasma concentrations in feline plasma. The assay's lower limit of quantification was 250 ng/mL. The mean ± standard deviation intra- and inter-day precision expressed as coefficients of variation were 6.83 ± 1.75 and 5.33 ± 1.37%, respectively, whereas intra- and inter-day accuracy expressed as a percentage of the bias were 11.40 ± 3.73 and 10.59 ± 3.88%, respectively. Accordingly, this validated assay should prove valuable for future in vivo clinical trials of mefloquine as an antiviral agent against feline coronavirus and feline calicivirus. However, the proportion of mefloquine binding to feline plasma proteins has not been reported. The proportion of drug bound to plasma protein binding is an important concept when developing drug dosing regimens. As cats with feline infectious peritonitis (FIP) demonstrate altered concentrations of plasma proteins, the proportion of mefloquine binding to plasma proteins in both clinically normal cats and FIP-affected cats was also investigated. An in vitro method using rapid equilibrium dialysis demonstrated that mefloquine was highly plasma protein bound in both populations (on average > 99%).en_AU
dc.language.isoenen_AU
dc.subjectCOVID-19en_AU
dc.subjectCoronavirusen_AU
dc.titleAssay validation and determination of in vitro binding of mefloquine to plasma proteins from clinically normal and FIP-affected catsen_AU
dc.typeArticleen_AU
dc.identifier.doi10.1371/journal.pone.0236754


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