A novel mutation of LIM2 causes autosomal dominant membranous cataract in a Chinese family

AIM:To identify mutations in the genes of a fourgeneration Chinese family with congenital membranous cataracts and investigate the morphologic changes and possible functional damage underlying the role of the mutant gene.METHODS:Whole exome analysis of thirteen members of a four-generation pedigree affected with congenital membranous cataracts was performed;co-segregation analysis of identified variants was validated by Sanger sequencing.All members underwent detailed physical and complete eye examinations.The physical changes caused by the mutation were analyzed in silico through homology modeling.The lens fiber block from a patient was observed under a scanning electron microscope(SEM).Cell membrane proteins and cytoplasmic proteins from the human lenses donated by one patient with cataract in this family and from the dislocated lens resulted from the penetrating ocular trauma of a patient unrelated with this family were extracted,and the expression and localization of MP20 and Cx46 were detected by Western blot(WB)assay in these proteins.RESULTS:A novel LIM2 heterozygous mutation(c.388 C>T,p.R130 C)was identified with congenital membranous cataracts inherited by an autosomal dominant(AD)pattern.Nystagmus and amblyopia were observed in all patients of this family,and exotropia and long axial length were observed in most patients.A/B ultrasound scan and ultrasound biomicroscopy revealed obvious thin crystalline lenses from 1.7 to 2.7 mm in central thickness in all cataract eyes.The bioinformatic analysis showed that the mutation was deleterious to the physiological function of LIM2-encoded MP20.Furthermore,by SEM,ultrastructure of the cataract nucleus showed that lens fiber cells(LFCs)remained morphologic characteristics of immature fiber cells,including flap cell surface with straight edges and lacking normal ball-and-socket joint boundaries,which implied that the differentiation of LFCs might be inhibited.Accumulation of MP20 and Cx46 in the cytoplasm was observed in the cytoplasm of the LFCs in human cataract lens.CONCLUSION:We identify a novel heterozygous LIM2(c.388 C>T,p.R130 C)mutation inherited by an AD pattern.This LIM2 mutation causes the abnormal sub-localization of MP20 and Cx46 in LFCs resulting in membranous cataracts.

自噬调节高浓度葡萄糖诱导的人晶状体上皮细胞上皮间质转化

目的:探究自噬水平变化对高糖诱导人晶状体上皮细胞上皮间质转化(EMT)的影响及其机制。方法:人晶状体上皮细胞(HLE-B3)分为正常对照组(NC组)和高糖处理组(HG组),分别用含5.5mmol/L葡萄糖的DMEM和添加了30mmol/L葡萄糖的上述DMEM培养12、24、48h,用Western blot检测上皮间质转化标志蛋白(E-cadherin、α-SMA)和自噬标志蛋白(LC3、Beclin 1和SQSTM1/p62)的表达变化,用划痕实验观察细胞的移行能力以明确高糖对晶状体上皮细胞自噬和EMT的影响。利用雷帕霉素调节自噬水平,将细胞分为正常对照组(NC组)、高糖处理组(HG组),高糖处理细胞的同时添加DMSO溶剂组(DMSO组)和添加200nmol/L雷帕霉素的雷帕霉素组(RAPA组),处理细胞24h,用Transwell实验观察细胞的移行能力,用Western blot检测EMT、自噬标志蛋白和TGF-β信号通路蛋白(TGF-β2、Smad2/3、p-Smad2/3、Snail)的表达。用细胞免疫荧光染色观察SQSTM1/p62与Smad2/3在细胞内的表达,免疫共沉淀方法检测细胞中SQSTM1/p62与Smad2/3之间的相互结合。结果:在高糖刺激后12、24、48h,HG组细胞E-cadherin、LC3Ⅱ/Ⅰ和Beclin 1蛋白表达逐渐降低(F=67.52、163、206,均P<0.0001),而α-SMA、SQSTM1/p62蛋白表达增加(F=53.37、302.1,均P<0.0001),细胞移行也较NC组增加(均P<0.001),提示高糖刺激后细胞发生EMT,而自噬水平降低;雷帕霉素处理后,与HG组和DMSO组相比,RAPA组LC3Ⅱ/Ⅰ和E-cadherin蛋白表达水平增加,α-SMA、p-Smad2/Smad2、p-Smad3/Smad3及Snail蛋白表达降低(均P<0.05),TGF-β2表达无明显改变(均P>0.05),细胞移行被抑制(均P<0.001),提示雷帕霉素在提高自噬水平的同时下调了TGF-β信号通路分子的表达进而抑制了EMT。细胞免疫荧光染色结果显示SQSTM1/p62与Smad2/3在胞浆内存在共定位,免疫共沉淀实验证实了SQSTM1/p62与Smad2/3蛋白相互结合。结论:高糖可刺激HLE-B3细胞发生EMT,下调细胞的自噬水平;自噬通过SQSTM1/p62与Smad2/3相互作用,改变了TGF-β信号通路中Smad2/3的表达,实现对EMT的调节。