Complete separation of critical pain management drug analytes from hydrophilic matrix components and isobaric interferences was achieved using the new Raptor™ SPP Biphenyl LC column in less than 5 min
Pain management LC analyses can be difficult to optimize due to the limited selectivity of C18 and phenyl-hexyl phases. In contrast, the selectivity of Raptor™ Biphenyl superficially porous particle (SPP) LC columns provides complete resolution of isobaric pain medications with a total cycle time of 5 min.
Accurate, reliable analysis of pain medications is a key component in monitoring appropriate medical use and preventing drug diversion and abuse. As the demand for fast, multicomponent methods grows, LC–MS-MS methods are increasingly desired for pain management and therapeutic drug monitoring due to the low detection limits that can be achieved with this highly sensitive and selective technique. However, despite the selectivity offered by mass spectrometry, hydrophilic matrix components can still interfere with early-eluting drug compounds resulting in ion suppression. In addition, isobaric pairs must be chromatographically separated for positive identification. The need for highly selective and accurate methods makes LC column selection critical.
While C18 and phenyl-hexyl phases are frequently used for bioanalytical LC–MS-MS applications, Restek's Biphenyl phase offers better aromatic retention and selectivity for pharmaceutical and drug-like compounds, giving it a significant advantage over other phases for the analysis of pain management medications or other drugs of abuse. The Biphenyl phase, originally developed a decade ago by Restek, has recently been combined with Raptor™ SPP ("core-shell") silica particles to allow for faster separations without the need for expensive UHPLC instrumentation. Here, we demonstrate the fast, selective separation of commonly tested pain drugs that can be achieved using the new Raptor™ SPP Biphenyl LC column.
Table I: Mobile phase gradient
A standard containing multiple pain management drugs was prepared in blank human urine and diluted with mobile phase as follows, urine:mobile phase A:mobile phase B (17:76:7). The final concentration for all analytes was 10 ng/mL except for lorazepam, which was 100 ng/mL. Samples were then analyzed by LC–MS-MS using an AB SCIEX API 4000™ MS-MS in ESI+ mode. Chromatographic conditions, retention times, and mass transitions are presented here and in Tables I and II:
Column: Raptor™ Biphenyl, 50 mm × 3.0 mm i.d. × 2.7 µm
Sample: Fortified urine
Inj. vol.: 10 µL
Inj. temp.: 30 °C
Mobile phase A: Water + 0.1% formic acid
Mobile phase B: Methanol + 0.1% formic acid
Table II: Analyte retention times and transitions
As shown in Figure 1, 18 commonly tested pain management drugs were analyzed with the last compound eluting in less than 3.5 min, giving a total cycle time of 5 min on Restek's Raptor™ SPP Biphenyl LC column. Analyte retention times are presented in Table II. Important isobaric pairs (morphine/hydromorphone and codeine/hydrocodone) were completely resolved and eluted as symmetrical peaks, allowing accurate identification and integration. In addition, early-eluting compounds such as morphine, oxymorphone, and hydromorphone are separated from hydrophilic matrix interferences, resulting in decreased ion-suppression and increased sensitivity. Similar analyses on C18 and phenyl-hexyl columns often exhibit poor peak shape and resolution (for example, peak tailing between closely eluting isobars), which makes identification and accurate quantification more difficult.
Figure 1: Baseline resolution of isobaric pain management drugs in sub-5-min runs on the Raptor™ Biphenyl column.
Complete separation of critical pain management drug analytes from hydrophilic matrix components and isobaric interferences was achieved using the new Raptor™ SPP Biphenyl LC column in less than 5 min. The fast, complete separations produced in this method allow accurate quantification of pain management drugs and support increased sample throughput and improved lab productivity.
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