Validation of an UPLC-MS/MS Method for Quantitative Analysis of Raltegravir in Human Plasma Samples

Fortuna, Serena; Ragazzoni, Enzo; Lisi, Lucia; Giambenedetto, Simona Di; Fabbiani, Massimiliano; Navarra, Pierluigi

doi:10.1097/ftd.0b013e318280110d

Cited by 9 publications

(8 citation statements)

References 32 publications

(30 reference statements)

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“…The method has been previously described in detail [21]. Briefly, plasma samples were extracted by liquid-liquid extraction followed by evaporation to dryness and reconstitution in mobile phase solution.…”

Section: Methodsmentioning

confidence: 99%

Variability of Raltegravir Plasma Levels in the Clinical Setting

Fortuna¹,

Fabbiani²,

Digiambenedetto³

et al. 2013

Pharmacology

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Therapeutic drug monitoring of raltegravir C_trough levels was carried out in the setting of the Raltegravir Switch for Toxicity or Adverse events (RASTA) trial, a randomized pilot study exploring a 48-week safety and efficacy of treatment switch to raltegravir associated with tenofovir/emtricitabine or abacavir/lamivudine in patients with regimens with optimal virologic control. Blood sampling for measurement of raltegravir plasma levels was carried out at weeks 4, 12, 24, 36 and 48. Plasma samples were analysed by a recently developed and validated UPLC-MS method. A total of 164 samples from 39 patients were assayed. Analysis for intra- and inter-subject variability was restricted to those patients with 4 or more determinations, including 30 patients and 142 determinations. The intra- and inter-subject variability measures were 85.9 and 124.6%, respectively, with an intra-/inter-subject variability ratio of 69%. We also analysed data from a subset of patients with well-documented adherence to protocol, defined as protocol compliant population, including 21 patients and 93 determinations. In this subpopulation, we estimated intra- and inter-subject variability of 79.87% and 110%, respectively, with an intra-/inter-subject variability ratio of 72.6%. This study confirms the notion that raltegravir is a highly variable drug according to the European Medicines Agency criteria. While this condition does not favour the adoption of therapeutic drug monitoring in the clinical practice, the latter is deemed useful in patients with drug plasma concentrations below or near the threshold level of efficacy (since intracellular raltegravir levels might be as low as 5% of the corresponding plasma levels), or to identify drug-drug interactions of potential clinical relevance.

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Section: Methodsmentioning

confidence: 99%

Variability of Raltegravir Plasma Levels in the Clinical Setting

Fortuna¹,

Fabbiani²,

Digiambenedetto³

et al. 2013

Pharmacology

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“…All the reported methods employed positive ionization mode for LC–MS/MS analysis of RAL in different biological matrices [8] , [9] , [12] , [14] , [15] , [16] , [19] , [20] , [21] , [24] , [25] , [26] . Contrary to this approach, negative ionization mode was selected in the present work as it showed better selectivity without compromising the sensitivity.…”

Section: Resultsmentioning

confidence: 99%

“…The proposed method is more sensitive compared to several methods developed for determination of raltegravir in human plasma [8] , [9] , [10] , [11] , [13] , [14] , [15] , [18] , [20] , [24] , [25] , [26] . Further, it is more rapid than all other methods except one report [20] . The present method employs small plasma volume (100 µL) for processing, which is much less compared to many reported procedures.…”

Section: Resultsmentioning

confidence: 99%

“… Extraction technique Sample volume (µL) Linear range (ng/mL) Retention time (min); run time (min) Application Refs. LLE with hexane–DCM 200 2.0–1000 1.56; 3.5 To support 18 clinical studies during Phase I through Phase III [8] LLE with hexane–DCM 200 1.0–3000 3.80; 7.0 Determination of raltegravir in a single HIV-infected patient [12] LLE with hexane–DCM 500 10.0–7680 8.23; 16.0 – [13] PP with ACN–methanol 25 10–3000 1.65; 4.0 Analysis of human plasma samples [14] PP with ACN–methanol 50 50–10000 4.20; 10.0 Pharmacokinetic study in one HIV-infected patient [15] LLE 100 5.0–2560 –; 1.0 Pharmacokinetic study in human plasma samples [20] PP with ACN 50 2.0–2000 nmol/L 4.90; 9.0 Pharmacokinetic study with 400 mg raltegravir in 6 healthy subjects [21] LLE with hexane–DCM 100 2.0–6000 1.35; 2.0 Bioequivalence study with 400 mg raltegravir in 18 healthy subjects; Reanalysis of 87 incurred samples (% change within±17%) PW LLE: liquid–liquid extraction; PP: protein precipitation; SPE: solid phase extraction; DCM: dichloromethane; ACN: acetonitrile; PW: present work. …”

Section: Resultsmentioning

confidence: 99%

“…Selective and sensitive determination of anti-HIVs in plasma is essential for studying drug–drug interaction, pharmacokinetics, pharmacodynamics and therapeutic drug monitoring. Several methods are reported for the determination of RAL as a single analyte [8] , [9] , [10] , [11] , [12] , [13] , [14] , [15] , [16] , [17] , [18] , [19] , [20] or in combination with its glucuronide (Glu) metabolite [21] or other anti-HIV drugs [22] , [23] , [24] , [25] , [26] in different biological samples such as human cell extracts [15] , [19] , cerebrospinal fluid [16] , cervicovaginal fluid [17] , dried blood spots [15] , bile [9] , feces [9] and human plasma [8] , [10] , [11] , [12] , [13] , [14] , [18] , [20] , [21] , [22] , [23] , [24] , [25] , [26] . Mainly, liquid chromatography with UV [10] , [17] , [23] , photodiode array [18] , [22] , fluorescence [11] or mass spectrometry [8] , [9] , [12] , [13] , [14] , [15] , [16] , [19] , [20] , [21] , [24] , [25] , [26] detection has been used for the quantification of RAL in these matrices.…”

Section: Introductionmentioning

confidence: 99%

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Selective and rapid determination of raltegravir in human plasma by liquid chromatography–tandem mass spectrometry in the negative ionization mode

Gupta

Guttikar

Shah

et al. 2015

Journal of Pharmaceutical Analysis

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A selective and rapid high-performance liquid chromatography–tandem mass spectrometry method was developed and validated for the quantification of raltegravir using raltegravir-d3 as an internal standard (IS). The analyte and IS were extracted with methylene chloride and n-hexane solvent mixture from 100 µL human plasma. The chromatographic separation was achieved on a Chromolith RP-18e endcapped C18 (100 mm×4.6 mm) column in a run time of 2.0 min. Quantitation was performed in the negative ionization mode using the transitions of m/z 443.1→316.1 for raltegravir and m/z 446.1→319.0 for IS. The linearity of the method was established in the concentration range of 2.0–6000 ng/mL. The mean extraction recovery for raltegravir and IS was 92.6% and 91.8%, respectively, and the IS-normalized matrix factors for raltegravir ranged from 0.992 to 0.999. The application of this method was demonstrated by a bioequivalence study on 18 healthy subjects.

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Stability indicating validated UPLC technique for the simultaneous analysis of raltegravir and lamivudine in pharmaceutical dosage forms

Konari

Jacob

2016

HIV & AIDS Review

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Validation of an UPLC-MS/MS Method for Quantitative Analysis of Raltegravir in Human Plasma Samples

Abstract: This rapid and sensitive method was validated and could be applied to pharmacokinetic studies for the determination of RTG concentrations in human plasma samples.

Cited by 9 publications

References 32 publications

Variability of Raltegravir Plasma Levels in the Clinical Setting

Variability of Raltegravir Plasma Levels in the Clinical Setting

Selective and rapid determination of raltegravir in human plasma by liquid chromatography–tandem mass spectrometry in the negative ionization mode

Stability indicating validated UPLC technique for the simultaneous analysis of raltegravir and lamivudine in pharmaceutical dosage forms

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