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巩膜通透性因小鼠品系而异,并可被慢性实验性青光眼所降低。

Scleral permeability varies by mouse strain and is decreased by chronic experimental glaucoma.

机构信息

Glaucoma Center of Excellence and Center for Nanomedicine, Wilmer Ophthalmological Institute, Department of Ophthalmology, Johns Hopkins University School of Medicine, Baltimore, Maryland, United States.

出版信息

Invest Ophthalmol Vis Sci. 2014 Apr 21;55(4):2564-73. doi: 10.1167/iovs.13-13327.

Abstract

PURPOSE

To determine differences in scleral permeability, as measured by diffusion of macromolecules, by using fluorescence recovery after photobleaching (FRAP), with reference to differences by mouse strain, scleral region, and the effect of experimental glaucoma.

METHODS

In three mouse strains (B6, CD1, and B6 mice with mutation in collagen 8α2 [Aca23]), we used FRAP to measure the diffusion of fluorescein isothiocyanate-dextran, molecular weight 40 kDa, into a photobleached zone of sclera. Scleral regions near the optic nerve head (peripapillary) and two successively more anterior regions were compared. Sclera from mouse eyes subjected to chronically elevated intraocular pressure after bead injection into the anterior chamber were compared to fellow eye controls. FRAP data were compared against estimated retinal ganglion cell axon loss in glaucomatous eyes.

RESULTS

Diffusion rates of dextran molecules in the sclera were significantly greater in Aca23 and B6 mice than in CD1 mice in a multivariate model adjusted for region and axial length (P < 0.0001). Dextran diffusion significantly decreased in glaucomatous eyes, and the decline increased with greater axon loss (P = 0.0003, multivariable model). Peripapillary scleral permeability was higher in CD1 than B6 and Aca23 mice (P < 0.05, multivariable model, adjusted by Bonferroni).

CONCLUSIONS

Measurement of the diffusion rates of dextran molecules in the sclera showed that glaucoma leads to decreased scleral permeability in all three mouse strains tested. Among mouse strains tested, those that were more susceptible to glaucomatous loss of retinal ganglion cells had a lower scleral permeability at baseline.

摘要

目的

通过荧光恢复后光漂白(FRAP)测量大分子扩散,确定巩膜通透性的差异,并参考不同的小鼠品系、巩膜区域和实验性青光眼的影响。

方法

在三种小鼠品系(B6、CD1 和胶原 8α2 突变的 B6 小鼠[Aca23])中,我们使用 FRAP 测量荧光素异硫氰酸酯-葡聚糖(分子量 40 kDa)扩散到巩膜漂白区。比较视神经头附近的巩膜区域(视盘周围)和两个连续更靠前的区域。比较经前房注珠后慢性眼压升高的小鼠眼与对侧眼对照的巩膜。FRAP 数据与青光眼眼中估计的视网膜神经节细胞轴突丢失进行比较。

结果

在多变量模型中,调整区域和眼轴长度后,Aca23 和 B6 小鼠巩膜中葡聚糖分子的扩散率明显高于 CD1 小鼠(P < 0.0001)。在青光眼眼中,葡聚糖的扩散明显减少,且随着轴突丢失的增加而增加(P = 0.0003,多变量模型)。在 CD1 小鼠中,视盘周围巩膜的通透性高于 B6 和 Aca23 小鼠(P < 0.05,多变量模型,经 Bonferroni 校正)。

结论

巩膜中葡聚糖分子扩散率的测量表明,在所有三种测试的小鼠品系中,青光眼都会导致巩膜通透性降低。在测试的小鼠品系中,那些更容易发生青光眼性视网膜神经节细胞丧失的品系,其巩膜通透性在基线时较低。

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