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桥粒斑蛋白(一种粘着斑蛋白)在晶状体中大量表达,且其表达会因细胞骨架信号受损而下调。

Abundant expression of ponsin, a focal adhesion protein, in lens and downregulation of its expression by impaired cytoskeletal signaling.

作者信息

Rao P Vasantha, Maddala Rupalatha

机构信息

Departments of Ophthalmology, Duke University School of Medicine, Durham, North Carolina 27710, USA.

出版信息

Invest Ophthalmol Vis Sci. 2009 Apr;50(4):1769-77. doi: 10.1167/iovs.08-2909. Epub 2008 Nov 21.

Abstract

PURPOSE

This study was undertaken to improve understanding of the defective lens developmental changes induced by the transgenic overexpression of the Rho GDP dissociation inhibitor RhoGDIalpha. The study was focused on a single differentially expressed gene encoding ponsin, a cell adhesion interacting signaling adaptor protein.

METHODS

Total RNA extracted from the P7 lenses of Rho GDIalpha transgenic mice was subjected to cDNA microarray analysis. Ponsin distribution in the mouse lenses was determined by immunofluorescence and immunoblot analyses. Interactions among ponsin, actin, and Rho GTPase signaling pathways were explored in lens epithelial cells.

RESULTS

The RhoGDIalpha transgenic mouse lenses revealed a marked downregulation of expression of multiple splice variants of ponsin. Expression of one of the ponsins (U58883) was found to be abundant in normal mouse lenses. Although ponsin was localized predominantly to the focal adhesions in lens epithelial cells, it was distributed to both the epithelium and fibers, with some isoforms being enriched primarily in the Triton X-100-insoluble fraction in lens tissue. Further, whereas constitutively active RhoA induced ponsin clustering at the leading edges, inhibition of Rho kinase and latrunculin treatment were noted to lead to decreases in ponsin protein levels in lens epithelial cells.

CONCLUSIONS

Abundant expression of ponsin, a focal adhesion protein in the lens tissue indicates a potential role for this protein in lens fiber cell migration and adhesion. Ponsin expression appears to be closely dependent on Rho GTPase-regulated integrity of actin cytoskeletal organization.

摘要

目的

本研究旨在增进对由Rho GDP解离抑制剂RhoGDIα转基因过表达诱导的晶状体发育缺陷变化的理解。该研究聚焦于一个编码ponsin的差异表达基因,ponsin是一种细胞黏附相互作用信号衔接蛋白。

方法

从Rho GDIα转基因小鼠的P7晶状体中提取总RNA,进行cDNA微阵列分析。通过免疫荧光和免疫印迹分析确定ponsin在小鼠晶状体中的分布。在晶状体上皮细胞中探索ponsin、肌动蛋白和Rho GTPase信号通路之间的相互作用。

结果

RhoGDIα转基因小鼠晶状体显示ponsin多个剪接变体的表达明显下调。发现其中一种ponsin(U58883)在正常小鼠晶状体中表达丰富。尽管ponsin主要定位于晶状体上皮细胞的粘着斑,但它分布于上皮和纤维中,一些异构体主要富集在晶状体组织的Triton X-100不溶性部分。此外,组成型活性RhoA诱导ponsin在前缘聚集,而Rho激酶抑制和拉春库林处理导致晶状体上皮细胞中ponsin蛋白水平降低。

结论

ponsin作为晶状体组织中的一种粘着斑蛋白的丰富表达表明该蛋白在晶状体纤维细胞迁移和粘附中具有潜在作用。ponsin表达似乎紧密依赖于Rho GTPase调节的肌动蛋白细胞骨架组织的完整性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c21e/2716002/63c8d3db7c7a/nihms109420f1.jpg

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