Liu Fei, Qin Yayun, Yu Shanshan, Soares Dinesh C, Yang Lifang, Weng Jun, Li Chang, Gao Meng, Lu Zhaojing, Hu Xuebin, Liu Xiliang, Jiang Tao, Liu Jing Yu, Shu Xinhua, Tang Zhaohui, Liu Mugen
From the Key Laboratory of Molecular Biophysics of Ministry of Education, Department of Genetics and Developmental Biology, College of Life Science and Technology, Huazhong University of Science and Technology, Wuhan, Hubei 430074, China.
MRC Human Genetics Unit/Centre for Genomic and Experimental Medicine, MRC Institute of Genetics and Molecular Medicine, University of Edinburgh, Edinburgh EH4 2XU, United Kingdom, and.
J Biol Chem. 2017 Apr 14;292(15):6225-6239. doi: 10.1074/jbc.M116.760314. Epub 2017 Feb 16.
Mutations in retinitis pigmentosa 2 () account for 10-20% of X-linked retinitis pigmentosa (RP) cases. The encoded RP2 protein is implicated in ciliary trafficking of myristoylated and prenylated proteins in photoreceptor cells. To date >70 mutations in have been identified. How these mutations disrupt the function of RP2 is not fully understood. Here we report a novel in-frame 12-bp deletion (c.357_368del, p.Pro120_Gly123del) in zebrafish The mutant zebrafish shows reduced rod phototransduction proteins and progressive retinal degeneration. Interestingly, the protein level of mutant Rp2 is almost undetectable, whereas its mRNA level is near normal, indicating a possible post-translational effect of the mutation. Consistent with this hypothesis, the equivalent 12-bp deletion in human markedly impairs RP2 protein stability and reduces its protein level. Furthermore, we found that a majority of the pathogenic mutations (including missense, single-residue deletion, and C-terminal truncation mutations) severely destabilize the RP2 protein. The destabilized RP2 mutant proteins are degraded via the proteasome pathway, resulting in dramatically decreased protein levels. The remaining non-destabilizing mutations T87I, R118H/R118G/R118L/R118C, E138G, and R211H/R211L are suggested to impair the interaction between RP2 and its protein partners (such as ARL3) or with as yet unknown partners. By utilizing a combination of , , and approaches, our work comprehensively indicates that loss of RP2 protein structural stability is the predominating pathogenic consequence for most mutations. Our study also reveals a role of the C-terminal domain of RP2 in maintaining the overall protein stability.
视网膜色素变性2(RP2)基因的突变占X连锁视网膜色素变性(RP)病例的10%-20%。编码的RP2蛋白参与光感受器细胞中肉豆蔻酰化和异戊二烯化蛋白的纤毛运输。迄今为止,已在RP2中鉴定出>70种突变。这些突变如何破坏RP2的功能尚不完全清楚。在这里,我们报告了斑马鱼RP2基因中一个新的框内12碱基缺失(c.357_368del,p.Pro120_Gly123del)。突变的斑马鱼显示视杆光转导蛋白减少和进行性视网膜变性。有趣的是,突变型Rp2的蛋白水平几乎检测不到,而其mRNA水平接近正常,表明该突变可能存在翻译后效应。与此假设一致,人类RP2基因中的等效12碱基缺失显著损害RP2蛋白稳定性并降低其蛋白水平。此外,我们发现大多数RP2致病突变(包括错义突变、单残基缺失和C端截短突变)严重破坏RP2蛋白的稳定性。不稳定的RP2突变蛋白通过蛋白酶体途径降解,导致蛋白水平显著降低。其余不破坏稳定性的突变T87I、R118H/R118G/R118L/R118C、E138G和R211H/R211L被认为损害了RP2与其蛋白伴侣(如ARL3)之间或与尚未明确的伴侣之间的相互作用。通过综合运用多种方法,我们的研究全面表明,RP2蛋白结构稳定性的丧失是大多数RP2突变的主要致病后果。我们的研究还揭示了RP2 C端结构域在维持整体蛋白稳定性中的作用。
