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阿昔洛韦酯前药通过兔角膜和SIRC-兔角膜上皮细胞系的转运

Transport of acyclovir ester prodrugs through rabbit cornea and SIRC-rabbit corneal epithelial cell line.

作者信息

Tak R V, Pal D, Gao H, Dey S, Mitra A K

机构信息

Division of Pharmaceutical Sciences, School of Pharmacy, University of Missouri-Kansas City, 5005 Rockhill Road, Kansas City, Missouri 64110, USA.

出版信息

J Pharm Sci. 2001 Oct;90(10):1505-15. doi: 10.1002/jps.1101.

Abstract

The purpose of this study is to assess the permeability of acyclovir (ACV) prodrugs through the rabbit corneal cell line (SIRC) as well as the cornea, and characterize the SIRC cell line for transport and metabolism studies of ester prodrugs. Prodrug derivatization of an acycloguanosine antiviral agent, acyclovir, was employed to improve its permeability across the cornea. New Zealand albino rabbits were used as an animal model for corneal studies. The SIRC cell line grown on polyester membranes was used for transport of these prodrugs. SIRC cells grown on the membrane support for 10 days developed four to six layers of epithelial cells, and this is comparable to the normal rabbit corneal epithelial layer. Transport experiments were conducted across the rabbit cornea and confluent SIRC cells using side-by-side diffusion-cell apparatus. Enzymatic hydrolysis of these compounds was evaluated in SIRC cell lysates. Appropriate reversed phase HPLC method(s) were employed for quantitation of both the prodrug and ACV simultaneously. Corneal permeabilities of some of these prodrugs (Malonyl ACV and Acetyl ACV) were higher relative to ACV. The SIRC cell line permeability values of all the prodrugs were higher compared to that of the intact cornea. The total amount of ACV-prodrugs transported, i.e., unhydrolyzed prodrugs and regenerated ACV, across the SIRC cell line was more relative to ACV. Hydrolytic studies in the SIRC cell line homogenate demonstrated the bioreversion potential of the prodrugs and the presence of enzymes, particularly the cholinesterase in the SIRC cell line. It may be concluded that the SIRC cell line is leakier compared to the cornea. Keeping in mind the limitations, the SIRC cell line after further characterization may be used for transport and metabolism studies of ester prodrugs.

摘要

本研究的目的是评估阿昔洛韦(ACV)前药通过兔角膜细胞系(SIRC)以及角膜的渗透性,并对SIRC细胞系进行表征,以用于酯前药的转运和代谢研究。采用阿昔洛韦(一种无环鸟苷抗病毒剂)的前药衍生化方法来提高其角膜通透性。新西兰白化兔被用作角膜研究的动物模型。在聚酯膜上生长的SIRC细胞系用于这些前药的转运。在膜载体上生长10天的SIRC细胞形成了四到六层上皮细胞,这与正常兔角膜上皮层相当。使用并排扩散池装置在兔角膜和汇合的SIRC细胞上进行转运实验。在SIRC细胞裂解物中评估这些化合物的酶促水解。采用适当的反相高效液相色谱法同时定量前药和ACV。相对于ACV,其中一些前药(丙二酰ACV和乙酰ACV)的角膜通透性更高。与完整角膜相比,所有前药的SIRC细胞系通透性值更高。跨SIRC细胞系转运的ACV前药总量,即未水解的前药和再生的ACV,相对于ACV更多。在SIRC细胞系匀浆中的水解研究表明了前药的生物逆转潜力以及酶的存在,特别是SIRC细胞系中的胆碱酯酶。可以得出结论,与角膜相比,SIRC细胞系的通透性更高。考虑到局限性,进一步表征后的SIRC细胞系可用于酯前药的转运和代谢研究。

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