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Transscleral diffusion of ethacrynic acid and sodium fluorescein

PURPOSE: One of the current limitations in developing novel glaucoma drugs that target the trabecular meshwork (TM) is the induced corneal toxicity from eyedrop formulations. To avoid the corneal toxicity, an alternative approach would be to deliver TM drugs through the sclera. To this end, we quant...

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Autores principales: Lin, Cheng-Wen, Wang, Yong, Challa, Pratap, Epstein, David L., Yuan, Fan
Formato: Texto
Lenguaje:English
Publicado: Molecular Vision 2007
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2633483/
https://www.ncbi.nlm.nih.gov/pubmed/17356511
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author Lin, Cheng-Wen
Wang, Yong
Challa, Pratap
Epstein, David L.
Yuan, Fan
author_facet Lin, Cheng-Wen
Wang, Yong
Challa, Pratap
Epstein, David L.
Yuan, Fan
author_sort Lin, Cheng-Wen
collection PubMed
description PURPOSE: One of the current limitations in developing novel glaucoma drugs that target the trabecular meshwork (TM) is the induced corneal toxicity from eyedrop formulations. To avoid the corneal toxicity, an alternative approach would be to deliver TM drugs through the sclera. To this end, we quantified ex vivo diffusion coefficient of a potential TM drug, ethacrynic acid (ECA), and investigated mechanisms of ECA transport in the sclera. METHODS: An Ussing-type diffusion apparatus was built to measure the apparent diffusion coefficient of ECA in fresh porcine sclera at 4 °C. To understand mechanisms of ECA transport, we quantified the transscleral transport of a fluorescent tracer, sodium fluorescein (NaF), that has a similar molecular weight but is more hydrophilic compared to ECA. Furthermore, we developed a mathematical model to simulate the transport processes and used it to analyze the experimental data. The model was also used to investigate the dependence of diffusion coefficients on volume fraction of viable cells and the binding of NaF and ECA to scleral tissues. RESULTS: The diffusion coefficients of ECA and NaF in the sclera were 48.5±15.1x10(-7) cm(2)/s (n=9) and 5.23±1.93x10(-7) cm(2)/s (n=8), respectively. Both diffusion coefficients were insensitive to cell shrinkage caused by ECA during the diffusion experiments and cell damage caused by the storage of tissues ex vivo before the experiments. Binding of ECA to scleral tissues could not be detected. The apparent maximum binding capacity and the apparent equilibrium dissociation constant for NaF were 80±5 mM and 2.5±0.5 mM (n=3), respectively. CONCLUSIONS: These data demonstrated that ECA diffusion was minimally hindered by structures in the sclera, presumably due to the lack of cells and binding sites for ECA in the sclera.
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spelling pubmed-26334832009-02-02 Transscleral diffusion of ethacrynic acid and sodium fluorescein Lin, Cheng-Wen Wang, Yong Challa, Pratap Epstein, David L. Yuan, Fan Mol Vis Research Article PURPOSE: One of the current limitations in developing novel glaucoma drugs that target the trabecular meshwork (TM) is the induced corneal toxicity from eyedrop formulations. To avoid the corneal toxicity, an alternative approach would be to deliver TM drugs through the sclera. To this end, we quantified ex vivo diffusion coefficient of a potential TM drug, ethacrynic acid (ECA), and investigated mechanisms of ECA transport in the sclera. METHODS: An Ussing-type diffusion apparatus was built to measure the apparent diffusion coefficient of ECA in fresh porcine sclera at 4 °C. To understand mechanisms of ECA transport, we quantified the transscleral transport of a fluorescent tracer, sodium fluorescein (NaF), that has a similar molecular weight but is more hydrophilic compared to ECA. Furthermore, we developed a mathematical model to simulate the transport processes and used it to analyze the experimental data. The model was also used to investigate the dependence of diffusion coefficients on volume fraction of viable cells and the binding of NaF and ECA to scleral tissues. RESULTS: The diffusion coefficients of ECA and NaF in the sclera were 48.5±15.1x10(-7) cm(2)/s (n=9) and 5.23±1.93x10(-7) cm(2)/s (n=8), respectively. Both diffusion coefficients were insensitive to cell shrinkage caused by ECA during the diffusion experiments and cell damage caused by the storage of tissues ex vivo before the experiments. Binding of ECA to scleral tissues could not be detected. The apparent maximum binding capacity and the apparent equilibrium dissociation constant for NaF were 80±5 mM and 2.5±0.5 mM (n=3), respectively. CONCLUSIONS: These data demonstrated that ECA diffusion was minimally hindered by structures in the sclera, presumably due to the lack of cells and binding sites for ECA in the sclera. Molecular Vision 2007-02-22 /pmc/articles/PMC2633483/ /pubmed/17356511 Text en http://creativecommons.org/licenses/by/3.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Lin, Cheng-Wen
Wang, Yong
Challa, Pratap
Epstein, David L.
Yuan, Fan
Transscleral diffusion of ethacrynic acid and sodium fluorescein
title Transscleral diffusion of ethacrynic acid and sodium fluorescein
title_full Transscleral diffusion of ethacrynic acid and sodium fluorescein
title_fullStr Transscleral diffusion of ethacrynic acid and sodium fluorescein
title_full_unstemmed Transscleral diffusion of ethacrynic acid and sodium fluorescein
title_short Transscleral diffusion of ethacrynic acid and sodium fluorescein
title_sort transscleral diffusion of ethacrynic acid and sodium fluorescein
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2633483/
https://www.ncbi.nlm.nih.gov/pubmed/17356511
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