Assay for the quantification of abemaciclib, its metabolites, and olaparib in human plasma by liquid chromatography-tandem mass spectrometry

被引:0
|
作者
Hill, Kasey L. [1 ]
Abbott, Nicole L. [1 ]
Na, Joo Young [1 ]
Rudek, Michelle [2 ]
Moore, Kathleen [3 ]
Lee, Eudocia Q. [4 ]
Phelps, Mitch A. [1 ,5 ]
机构
[1] Ohio State Univ, Comprehens Canc Ctr, Pharmacoanalyt Shared Resource, 460 W 12th Ave, Columbus, OH 43210 USA
[2] SKCCC Johns Hopkins, Analyt Pharmacol Shared Resource, 1650 Orleans St, Baltimore, MD 21287 USA
[3] Univ Oklahoma, Hlth Sci Ctr, Stephenson Canc Ctr, 800 NE 10th St, Oklahoma City, OK 73104 USA
[4] Dana Farber Brigham & Womens Canc Ctr, Ctr Neurooncol, 450 Brookline Ave, Boston, MA 02215 USA
[5] Ohio State Univ, Coll Pharm, Div Pharmaceut & Pharmacol, 496 W 12th Ave, Columbus, OH 43210 USA
关键词
Abemaciclib; N-desethylabemaciclib (M2); Hydroxyabemaciclib (M20); Hydroxy-N-desethylabemaciclib (M18); Olaparib; Pharmacokinetic studies; BREAST-CANCER; ANTITUMOR-ACTIVITY; JAPANESE PATIENTS; SINGLE-AGENT; INHIBITOR; COMBINATION; CDK4; VALIDATION; LY2835219; SAFETY;
D O I
10.1016/j.jpba.2024.116531
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
An isotope-dilution bioanalytical assay for abemaciclib and its metabolites in combination with olaparib was developed and validated in human plasma K2 EDTA. For the quantitative assay, human plasma samples (or human plasma QC samples) were spiked with internal standard solution before a simple protein precipitation with methanol. The extract was injected onto a liquid chromatography-tandem mass spectrometry (LC-MS/MS) instrument where it was chromatographically separated by a polar end-capped reversed phase column and guard using gradient elution with water and methanol both modified with 0.2 % formic acid (v/v) as the mobile phases. The analytes and internal standards were measured by heated electrospray ionization (HESI) in positive polarity using selected reaction monitoring (SRM) on a triple quadrupole mass spectrometer. The assay was validated for linear ranges as follows: 0.4 - 1000 nM abemaciclib, 0.35 - 1000 nM M2 and M18, 0.5 - 1000 nM M20, and 0.75 - 1000 nM olaparib. The inter-day or between day precision for the quality controls (n = 18) was < 13% and the accuracy was +/- 12 %, for all analytes, including the lower limit of quantification (LLOQ). The intra-day or within day precision for the quality controls (n = 6) was <= 11 % and the accuracy was +/- 12% for low, mid, and high and < 19% at LLOQ. The recovery in human plasma was determined to be between 92% and 102% for all analytes spanning the linear range. The validated, bioanalytical quantitative assay was designed to measure abemaciclib, its metabolites, and olaparib for pharmacokinetic evaluation of patients in clinical trials for breast, brain, and ovarian cancers.
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页数:8
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