Abstract

AbstractA HJPLC method for the determination of acyclovir in plasma is described. The method is simple and sensitive enough for bioequiva‐lence studies, where a large number of plasma samples with low acyclovir concertration are involved. The procedure is based on the deproteinization of plasma with perchloric acid and separation of acyclovir on a Hypersil ODS Column at pH 5.6 with UV detection. The calibration standards are linear up to at least 4000 ng/mL and the limit of quantification is 10 ng/mL.

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