Influence of Liposomes and Niosomes on the In Vitro Permeation and Skin Retention of Finasteride

Authors

  • Mahmoud Reza Jaafari Faculty of Pharmacy & Biotechnology Research Center, Mashad University of Medical Sciences, Mashad, Iran
  • Majid Tabbakhian Faculty of Pharmacy & Pharmaceutical Research Center, Isfahan University of Medical Sciences, Isfahan, Iran
  • Naser Tavakoli Faculty of Pharmacy & Pharmaceutical Research Center, Isfahan University of Medical Sciences, Isfahan, Iran
  • Saeid Daneshamouz Faculty of Pharmacy & Pharmaceutical Research Center, Shiraz University of Medical Sciences, Shiraz, Iran Faculty of Pharmacy & Pharmaceutical Research Center, Isfahan University of Medical Sciences, Isfahan, Iran
Abstract:

      In this work we sought to determine whether vesicles (liposomes/niosomes) were able to enhance finasteride concentration in the dermis layer, including the pilosebaceous units (PSU). Such enhancement could be beneficial in the treatment of some androgen-related skin disorders. Hamster flank skin was used to study  3Hfinasteride permeation via vesicles and a hydroalcoholic solution (HA). The drug-containing vesicles were composed of dimyristoyl phosphatidylcholine (DMPC) or egg lecithin: cholesterol: dicetyl phosphate (liposomes) and polyoxyethylene  alkyl ethers (Brij ® series) or sorbitan monopalmitate (Span 40): cholesterol: dicetyl phosphate (niosomes) and were prepared by the film hydration technique. Determination of finasteride content by HPLC showed 80-97% drug entrapment efficiency in the vesicles. The amount of 3H-finasteride penetrated into and permeated through hamster skin 24 h after topical application of vesicles ranged from 5.5 to 13% of the initial dose, compared to 24%, observed with HA  ( pSpan 40 and lecithin vesicles was lower, when compared with liquid-state Brij97, Brij 76: Brij 97 and DMPC vesicles. The fraction of finasteride found in the dermis  layer was greatest where DMPC liposomes were used (7.8%). The vesicles significantly reduced drug permeation as indicated by the flux of finasteride from vesicles (0.025-0.058 µg/cm 2.h), where compared with the HA (0.13 µg/cm2.h),  (pthe percutaneous absorption of finasteride and increasing its concentration and retention in the dermis layer.

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Journal title

volume 1  issue 3

pages  119- 130

publication date 2005-03-01

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