4.5 Article

The role of glutathione in the permeation enhancing effect of thiolated polymers

Journal

PHARMACEUTICAL RESEARCH
Volume 19, Issue 5, Pages 602-608

Publisher

KLUWER ACADEMIC/PLENUM PUBL
DOI: 10.1023/A:1015345827091

Keywords

ussing-type chamber; glutathione; small intestine; permeation enhancement

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Purpose. To verify or refute the mechanism of permeation enhancement with thiolated polymers via GSH by the use of NaFlu as marker for the paracellular permeation. Methods. The capability of 0.5% polycarbophil cysteine conjugate (PCP-Cys) to reduce 0.02% oxidized glutathione (GSSG) was evaluated via iodometric titration in aqueous solution. Glutathione in its reduced form (GSH; 0.1%-0.4%) and in combination with 0.5% PCP-Cys were tested for their permeation enhancement of sodium fluorescein (NaFlu) and fluorescence labeled bacitracin (bac-FITC) used as paracellular markers. Permeation studies across guinea pig duodenum were carried out in Ussing-type chambers. Opening of the tight junctions was additionally monitored by transepithelial electrical resistance (TEER) measurements. Results. PCP-Cys (0.5%) was shown to reduce 22.0% +/- 8.2% of GSSG (0.02%) to GSH in aqueous solution at pH 7.0 and 37degreesC within 3 h. Permeation of NaFlu was shown to depend on the concentration of GSH. The apparent permeability coefficient (P(a)pp) of NaFlu in buffer only was 4.98 +/- 0.5*10(-)6, while in the presence of 0.4% GSH a P(a)pp of 9.31 +/- 0.92*10(-)6 was achieved, representing an enhancement ratio (R = P(a)pp enhancer system/P(a)pp control) of 1.86. The combination of GSH (0.4%) with PCP-Cys (0.5%) led to a significant (p < 0.001) improvement of R for NaFlu up to 2.93 accompanied by a decrease in TEER of 20.3% +/- 1.4%. Incubation of bac-FITC with the same GSH / PCP-Cys combination led to an enhancement ratio of 2.06 within 3 h. Conclusion. GSH plays an important role in the opening of tight junctions of intestinal epithelia. It would appear that PCP-Cys is able to reduce GSSG, prolonging the concentration of GSH at the apical membrane, resulting in significantly enhanced paracellular transport.

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