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Original Research Article | OPEN ACCESS

Simultaneous quantitative determination of zidovudine and nevirapine in human plasma using isocratic, reverse phase high performance liquid chromatography

Vibhuti Kabra1 , Vivek Agrahari1, Chandrabose Karthikeyan2, Piyush Trivedi2

1Department of Pharmacy, Shri G. S. Institute of Technology & Science (SGSITS), Indore 452001; 2School of Pharmaceutical Sciences, Rajiv Gandhi Technical University (RGTU), Bhopal 462036, Madhya Pradesh, India.

For correspondence:-  Vibhuti Kabra   Email: vibhuti.kabra@rediffmail.com   Tel:+919827500875

Received: 30 July 2008        Accepted: 24 October 2008        Published: 23 February 2009

Citation: Kabra V, Agrahari V, Karthikeyan C, Trivedi P. Simultaneous quantitative determination of zidovudine and nevirapine in human plasma using isocratic, reverse phase high performance liquid chromatography. Trop J Pharm Res 2009; 8(1):79-86 doi: 10.4314/tjpr.v8i1.11

© 2009 The authors.
This is an Open Access article that uses a funding model which does not charge readers or their institutions for access and distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0) and the Budapest Open Access Initiative (http://www.budapestopenaccessinitiative.org/read), which permit unrestricted use, distribution, and reproduction in any medium, provided the original work is properly credited..

Abstract

Purpose: To develop a sensitive and rapid reverse phase high performance liquid chromatography (HPLC) method for the measurement of the levels of zidovudine (ZVD) and nevirapine (NVP) in human plasma.
Methods: Standard stock solutions for HPLC analysis were prepared by dissolving ZVD and NVP in methanol. In the HPLC measurement, sample detection was carried out at 246 nm using an ultraviolet (UV)-photo diode array (PDA) detector. Plasma sample pretreatment consisted of protein precipitation extraction with methanol. The compounds were separated using a mobile phase consisting of a pH 3.0 solution (obtained by adjusting the pH of water with orthophosphoric acid): acetonitrile (73:27 v/v) on a Phenomenex LUNA C18, column (250×4.6 mm i.d., 5μm) at a flow rate of 0.9 mL min-1. The total run time for the assay was 10.2 min. The method was validated over the range of 300-9600 ng mL-1 and 200-6400 ng mL-1 for ZVD and NVP, respectively.  
Results: The lowest limits of quantification (LLOQ) and of detection (LOD) were 300 and 63 ng mL-1 for ZVD and 200 and 17 ng mL-1 for NVP, respectively. The method was found to be accurate, with accuracy ranging from -10.92 to +9.57 % and precise, with intra-day, inter-day as well as analyst to analyst precision of 0.68 to 9.38 %. Extraction recoveries of the drugs from plasma were 91.39, 95.01, 89.51 % for ZVD and 90.93, 93.26, 92.13 % for NVP, for LQC (low quality control), MQC (medium quality control) and HQC (high quality control) samples, respectively. Stability data revealed that the drugs were stable in plasma under various test conditions.
Conclusion: This assay can be suitably used for the determination of zidovudine (ZVD) and nevirapine (NVP) in human plasma and should be useful in HIV clinical trials and clinical therapeutic drug monitoring (TDM) programs. It would also be potentially useful in the determination of pharmacokinetic profiles and in bioequivalence studies in HIV research.

Keywords: Assay, Zidovudine, Nevirapine, Human plasma, Reverse phase high-performance liquid chromatography

Impact Factor
Thompson Reuters (ISI): 0.6 (2023)
H-5 index (Google Scholar): 49 (2023)

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