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Evaluation of Transdermal Drug Permeation as Modulated by Lipoderm and Pluronic Lecithin Organogel
Authors:Qian Zhang  Yunmei Song  Stephen W. Page  Sanjay Garg
Affiliation:1. Centre for Pharmaceutical Innovation and Development, School of Pharmacy and Medical Science, University of South Australia, Adelaide 5000, South Australia, Australia;2. Luoda Pharma, Caringbah 2229, New South Wales, Australia
Abstract:
The transdermal delivery of 2 fluorescent probes with similar molecular weight but different lipophilicity, into and through the skin from 2 commercially available transdermal bases, pluronic lecithin organogel, and Lipoderm® has been evaluated. First, in vitro penetration of fluorescein sodium and fluorescein (free acid) through porcine skin was evaluated. Retention and depth distribution profiles in skin were obtained by tape stripping and then followed by optical sectioning using multiphoton microscopy. The results showed that Lipoderm® led to an enhanced penetration of the hydrophilic compound, fluorescein sodium. For the lipophilic compound fluorescein (free acid), Lipoderm® performed similar to pluronic lecithin organogel base, where minimal drug was detected in either receptor phase. The skin retention and depth distribution results also showed that the hydrophilic fluorescein sodium had high skin retention with Lipoderm®, whereas fluorescein (free acid) had very low penetration and retention with increasing skin depth. Moreover, optical sectioning by multiphoton microscopy revealed an uneven distribution of probes across the skin in the x-y plane for both transdermal bases. This work showed that a hydrophilic compound has significantly increased skin penetration and retention when formulated with Lipoderm®, and the skin retention of the probe was the main determinant of its skin flux.
Keywords:transdermal drug delivery  percutaneous  permeation enhancers  solubility  imaging method  PLO  pluronic lecithin organogel  PBS  phosphate-buffered saline  BSA  bovine serum albumin  DMSO  dimethyl sulfoxide  steady-state flux  MPM  multiphoton microscopy
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