Volume 12 Issue 2
May  2022
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Vijay Kumar Shankar, Mei Wang, Srinivas Ajjarapu, Praveen Kolimi, Bharathi Avula, Reena Murthy, Ikhlas Khan, Sathyanarayana Narasimha Murthy. Analysis of docosanol using GC/MS: Method development, validation, and application to ex vivo human skin permeation studies[J]. Journal of Pharmaceutical Analysis, 2022, 12(2): 287-292. doi: 10.1016/j.jpha.2021.08.004
Citation: Vijay Kumar Shankar, Mei Wang, Srinivas Ajjarapu, Praveen Kolimi, Bharathi Avula, Reena Murthy, Ikhlas Khan, Sathyanarayana Narasimha Murthy. Analysis of docosanol using GC/MS: Method development, validation, and application to ex vivo human skin permeation studies[J]. Journal of Pharmaceutical Analysis, 2022, 12(2): 287-292. doi: 10.1016/j.jpha.2021.08.004

Analysis of docosanol using GC/MS: Method development, validation, and application to ex vivo human skin permeation studies

doi: 10.1016/j.jpha.2021.08.004
  • Received Date: Mar. 09, 2021
  • Accepted Date: Aug. 27, 2021
  • Rev Recd Date: Aug. 09, 2021
  • Publish Date: Aug. 29, 2021
  • Docosanol is the only US Food and Drug Administration (FDA) approved over-the-counter topical product for treating recurrent oral-facial herpes simplex labialis. Validated analytical methods for docosanol are required to demonstrate the bioequivalence of docosanol topical products. A gas chromatography/selected ion monitoring mode mass spectrometry (GC/SIM-MS) method was developed and validated for docosanol determination in biological samples. Docosanol and isopropyl palmitate (internal standard) were separated on a high-polarity GC capillary column with (88% cyanopropy)aryl-polysiloxane employed as the stationary phase. The ions of m/z 83 and 256 were selected to monitor docosanol and isopropyl palmitate, respectively; the total run time was 20 min. The GC/SIM-MS method was validated in accordance with US FDA guidelines, and the results met the US FDA acceptance criteria. The docosanol calibration standards were linear in the 100–10000 ng/mL concentration range (R2>0.994). The recoveries for docosanol from the receptor fluid and skin homogenates were >93.2% and >95.8%, respectively. The validated method was successfully applied to analyze ex vivo human cadaver skin permeation samples. On applying Abreva® cream tube and Abreva® cream pump, the amount of docosanol that penetrated human cadaver skin at 48 h was 21.5 ±7.01 and 24.0 ±6.95 ng/mg, respectively. Accordingly, we concluded that the validated GC/SIM-MS was sensitive, specific, and suitable for quantifying docosanol as a quality control tool. This method can be used for routine analysis as a cost-effective alternative to other techniques.
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