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通过融合脂质体将DNA导入大鼠和灵长类动物的小梁网。

Introduction of DNA into the rat and primate trabecular meshwork by fusogenic liposomes.

作者信息

Hangai M, Tanihara H, Honda Y, Kaneda Y

机构信息

Department of Ophthalmology and Visual Science, Graduate School of Medicine, Kyoto University, Japan.

出版信息

Invest Ophthalmol Vis Sci. 1998 Mar;39(3):509-16.

PMID:9501860
Abstract

PURPOSE

To evaluate the feasibility of introducing exogenous genes and phosphorothioate oligonucleotides into the anterior chamber tissues of rats and monkeys using the authors' fusogenic liposomes.

METHODS

Hemagglutinating virus of Japan liposomes containing LacZ DNA-high-mobility group 1 complexes or fluorescein isothiocyanate (FITC)-labeled phosphorothioate oligonucleotides were prepared and injected into the anterior chambers of rats (3 microliters) and rhesus monkeys (30 microliters). The expression of LacZ DNA was visualized histochemically by beta-Galactosidase assay and was followed for as long as 60 days in rats and 30 days in monkeys. FITC-labeled phosphorothioate oligonucleotides were observed by fluorescence microscopy for as long as 14 days in rats and 7 days in monkeys.

RESULTS

Injection of LacZ DNA-high-mobility group 1 complexes encapsulated in hemagglutinating virus of Japan liposomes resulted in blue staining in the trabecular meshwork and iris-ciliary body of rats and selectively in the trabecular meshwork of monkeys at the concentrations used. This LacZ expression lasted for as long as 14 days after injection in both animals. Phosphorothioate oligonucleotides (3 microM) also were introduced into the rat trabecular meshwork and iris-ciliary body and into the primate trabecular meshwork when encapsulated in hemagglutinating virus of Japan liposomes, although the injection of naked FITC-labeled phosphorothioate oligonucleotides at the same concentration resulted in little fluorescence in any anterior chamber tissue.

CONCLUSIONS

This study shows that the use of hemagglutinating virus of Japan liposomes can transfer LacZ DNA and phosphorothioate oligonucleotides to adult rat and primate trabecular meshwork. This system may enable progress in glaucoma research and in the development of nonviral somatic gene therapy of the trabecular meshwork to treat glaucoma.

摘要

目的

评估使用作者的融合脂质体将外源基因和硫代磷酸酯寡核苷酸导入大鼠和猴前房组织的可行性。

方法

制备含有LacZ DNA-高迁移率族蛋白1复合物的日本血凝病毒脂质体或异硫氰酸荧光素(FITC)标记的硫代磷酸酯寡核苷酸,并注入大鼠(3微升)和恒河猴(30微升)的前房。通过β-半乳糖苷酶测定对LacZ DNA的表达进行组织化学可视化,并在大鼠中持续观察60天,在猴中持续观察30天。通过荧光显微镜观察FITC标记的硫代磷酸酯寡核苷酸,在大鼠中持续观察14天,在猴中持续观察7天。

结果

注射包裹在日本血凝病毒脂质体中的LacZ DNA-高迁移率族蛋白1复合物,在所用浓度下,大鼠的小梁网和虹膜睫状体出现蓝色染色,猴则选择性地在小梁网出现蓝色染色。在两种动物中,这种LacZ表达在注射后可持续长达14天。当硫代磷酸酯寡核苷酸(3 microM)包裹在日本血凝病毒脂质体中时,也可导入大鼠小梁网和虹膜睫状体以及灵长类动物的小梁网,尽管注射相同浓度的裸FITC标记硫代磷酸酯寡核苷酸在任何前房组织中几乎没有荧光。

结论

本研究表明,使用日本血凝病毒脂质体可将LacZ DNA和硫代磷酸酯寡核苷酸转移至成年大鼠和灵长类动物的小梁网。该系统可能推动青光眼研究以及小梁网非病毒体细胞基因治疗青光眼的发展。

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