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使用离子电渗法增强寡核苷酸向小鼠视网膜细胞的递送。

Enhanced oligonucleotide delivery to mouse retinal cells using iontophoresis.

作者信息

Andrieu-Soler Charlotte, Doat Marc, Halhal Mounia, Keller Nicole, Jonet Laurent, BenEzra David, Behar-Cohen Francine

机构信息

INSERM, U598, Paris, France.

出版信息

Mol Vis. 2006 Sep 26;12:1098-107.

Abstract

PURPOSE

To study the combination of oligodeoxynucleotides (ODNs) intravitreous injection and saline transpalpebral iontophoresis on the delivery of ODNs to photoreceptors in the newborn rd1/rd1 mice.

METHODS

Cathodal or anodal transpalpebral iontophoresis (1.43 mA/cm(2) for 5 min) was applied to eyes of postnatal day 7 (PN7) rd1/rd1 mice immediately before the intravitreous injection of ODNs. The effect of cathodal iontophoresis after ODNs injection was also evaluated. The influence of current intensity (0.5, 1.5, and 2.5 mA) was assayed with cathodal iontophoresis performed prior to ODNs injection. The duration of current-induced facilitation of ODNs delivery to photoreceptors was evaluated for 6 h following iontophoresis. One group of control eyes received cathodal iontophoresis prior to the intravitreous injection of phosphate buffered saline (PBS) or hexachlorofluorescein (Hex). The second control group received ODN or Hex intravitreous injection without iontophoresis. The penetration of fluorescent ODNs in the outer nuclear layer (ONL) was quantified by image analysis of the ONL fluorescence intensity on cryosection microphotographs. Integrity of ODN was assessed using acrylamide gel migration after its extraction from the retina of treated mice. The integrity of retinal structure, 1 and 24 h after iontophoresis, was analyzed using light and electron microscopy.

RESULTS

Transpalpebral anodal or cathodal saline iontophoresis enhanced the penetration of ODNs in all retinal layers. Cathodal iontophoresis was more efficient than anodal iontophoresis in enhancing the tissue penetration of the injected ODN. Photoreceptor delivery of ODN was significantly higher when cathodal saline transpalpebral iontophoresis was applied prior than after the injection. The extent of enhanced tissue penetration decreased in parallel to the increased interval between iontophoresis application and the intravitreous injection. Current of 1.5 mA was safe and optimal for the delivery of ODNs to the ONL. One hour after iontophoresis followed by injection, ODN extracted from the retina of treated eyes remained intact. Histology and electron microscopy observations demonstrated that iontophoresis using the optimal parameters did not induce any permanent tissue alterations or structure damage.

CONCLUSIONS

Saline transpalpebral iontophoresis facilitates the penetration of injected ODNs in photoreceptors for at least 3 h. This method may be considered for photoreceptor targeted gene therapy.

摘要

目的

研究寡脱氧核苷酸(ODNs)玻璃体内注射联合经睑离子电渗疗法(使用生理盐水)对新生rd1/rd1小鼠光感受器递送ODNs的作用。

方法

在向出生后第7天(PN7)的rd1/rd1小鼠眼内玻璃体内注射ODNs之前,立即施加阴极或阳极经睑离子电渗疗法(1.43 mA/cm²,持续5分钟)。还评估了ODNs注射后阴极离子电渗疗法的效果。在ODNs注射前进行阴极离子电渗疗法,测定电流强度(0.5、1.5和2.5 mA)的影响。在离子电渗疗法后6小时内评估电流诱导的ODNs向光感受器递送促进作用的持续时间。一组对照眼在玻璃体内注射磷酸盐缓冲盐水(PBS)或六氯荧光素(Hex)之前接受阴极离子电渗疗法。第二组对照组接受ODN或Hex玻璃体内注射但不进行离子电渗疗法。通过对冷冻切片显微照片上外核层(ONL)荧光强度的图像分析,对荧光ODNs在ONL中的渗透进行定量。从处理过的小鼠视网膜中提取ODN后,使用丙烯酰胺凝胶迁移评估ODN的完整性。使用光学显微镜和电子显微镜分析离子电渗疗法后1小时和24小时视网膜结构的完整性。

结果

经睑阳极或阴极生理盐水离子电渗疗法增强了ODNs在所有视网膜层中的渗透。在增强注射的ODN的组织渗透方面,阴极离子电渗疗法比阳极离子电渗疗法更有效。当在注射前应用阴极经睑生理盐水离子电渗疗法时,ODN向光感受器的递送显著更高。随着离子电渗疗法应用与玻璃体内注射之间间隔时间的增加,组织渗透增强的程度平行降低。1.5 mA的电流对于将ODNs递送至ONL是安全且最佳的。离子电渗疗法后紧接着注射1小时后,从处理过的眼睛视网膜中提取的ODN保持完整。组织学和电子显微镜观察表明,使用最佳参数的离子电渗疗法不会引起任何永久性组织改变或结构损伤。

结论

经睑生理盐水离子电渗疗法可促进注射的ODNs在光感受器中的渗透至少3小时。这种方法可考虑用于光感受器靶向基因治疗。

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