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SNX8 能够促进溶酶体重构,逆转溶酶体贮积症。

SNX8 enables lysosome reformation and reverses lysosomal storage disorder.

机构信息

The MOE Key Laboratory of Biosystems Homeostasis & Protection and Zhejiang Provincial Key Laboratory of Cancer Molecular Cell Biology, Life Sciences Institute, Zhejiang University, 310058, Hangzhou, Zhejiang, China.

Center for Life Sciences, Shaoxing Institute, Zhejiang University, 321000, Shaoxing, Zhejiang, China.

出版信息

Nat Commun. 2024 Mar 22;15(1):2553. doi: 10.1038/s41467-024-46705-x.

Abstract

Lysosomal Storage Disorders (LSDs), which share common phenotypes, including enlarged lysosomes and defective lysosomal storage, are caused by mutations in lysosome-related genes. Although gene therapies and enzyme replacement therapies have been explored, there are currently no effective routine therapies against LSDs. During lysosome reformation, which occurs when the functional lysosome pool is reduced, lysosomal lipids and proteins are recycled to restore lysosome functions. Here we report that the sorting nexin protein SNX8 promotes lysosome tubulation, a process that is required for lysosome reformation, and that loss of SNX8 leads to phenotypes characteristic of LSDs in human cells. SNX8 overexpression rescued features of LSDs in cells, and AAV-based delivery of SNX8 to the brain rescued LSD phenotypes in mice. Importantly, by screening a natural compound library, we identified three small molecules that enhanced SNX8-lysosome binding and reversed LSD phenotypes in human cells and in mice. Altogether, our results provide a potential solution for the treatment of LSDs.

摘要

溶酶体贮积症(LSDs)具有共同的表型,包括溶酶体增大和溶酶体储存缺陷,是由溶酶体相关基因的突变引起的。虽然已经探索了基因治疗和酶替代疗法,但目前针对 LSDs 还没有有效的常规治疗方法。在功能性溶酶体池减少时发生溶酶体再形成,溶酶体脂质和蛋白质被回收以恢复溶酶体功能。在这里,我们报告分选连接蛋白 SNX8 促进溶酶体小管化,这是溶酶体再形成所必需的过程,而 SNX8 的缺失导致人类细胞中 LSDs 的特征性表型。SNX8 的过表达挽救了细胞中 LSDs 的特征,并且基于 AAV 的 SNX8 递送至大脑挽救了 LSD 表型在小鼠中。重要的是,通过筛选天然化合物文库,我们鉴定出三种小分子,它们增强了 SNX8-溶酶体结合并逆转了人类细胞和小鼠中 LSDs 的表型。总之,我们的研究结果为 LSDs 的治疗提供了一种潜在的解决方案。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/747a/10959956/1732aa67a727/41467_2024_46705_Fig1_HTML.jpg

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