Identification of a novel p.R1443W mutation in RP1 gene associated with retinitis pigmentosa sine pigmento

AIM:To screen mutations in the retinitis pigmentosa 1(RP1) gene and the rhodopsin(RHO) gene in Chinese patients with retinitis pigmentosa sine pigmento(RPSP)and describe the genotype-phenotype relationship of the mutations.·METHODS:Twenty affected,unrelated Chinese individuals with RPSP(4 autosomal dominant RPSP,12autosomal recessive RPSP and 4 unknown inheritance pattern) were recruited between 2009 and 2012.The clinical features were determined by complete ophthalmologic examinations.Polymerase chain reaction(PCR) and direct DNA sequencing were used to screen the entire coding region and splice junctions of the RP1gene and the RHO gene.The cosegregation analysis and population frequency studies were performed for patients with identified mutations.·RESULTS:Five variants in the RP1 gene and one in the RHO gene were detected in 20 probands.Four missense changes(rs444772,rs446227,rs414352,rs441800) and one non-coding variant(rs56340615) were common SNPs and none of them showed a significant relationship with RPSP.A missense mutation p.R1443W was identified in the RP1 gene in three affected individuals from a family with autosomal dominant RPSP and was found to cosegregate with the phenotype in this family,suggestive of pathogenic.In addition,population frequency analysis showed the p.R1443W mutation was absent in 300 healthy controls.·CONCLUSION:The identification of p.R1443W mutationcosegregating in a family with autosomal dominant RPSP highlights an atypical phenotype of the RP1 gene mutation,while RHO gene is not associated with the pathogenesis of RPSP in this study.To our knowledge,this is the fist mutation identified to associate with RPSP.

骨髓间充质干细胞(MSCs)对N-甲基-N-亚硝脲(MNU)诱导的C57BL小鼠视网膜变性的治疗作用

目的观察骨髓间充质干细胞(mesenchymal stem cells,MSCs)对N-甲基-N-亚硝脲(N-methyl-N-nitrosourea,MNU)诱导的C57BL小鼠视网膜色素变性(retinitis pigmentosa,RP)的治疗作用。方法应用不同剂量(30 mg·kg^(-1)、45 mg·kg^(-1)、60 mg·kg^(-1)、75 mg·kg^(-1)、90 mg·kg^(-1))的MNU腹腔注射给予C57BL小鼠和MNU作用不同时间(1 d、3 d、7 d)后,通过视网膜电图(electroretinogram,ERG)和HE染色检测小鼠视网膜的电生理功能和组织形态变化,优化建立稳定的RP动物模型的最佳条件;在此动物模型的基础上,经玻璃体内注射和尾静脉注射给予MSCs移植,并应用ERG和HE染色评估MSCs对MNU诱导的RP的治疗作用。结果与对照组相比,30 mg·kg^(-1)、45mg·kg^(-1)剂量的MNU可引起视网膜形态和功能的轻微损伤,而60 mg·kg^(-1)及其以上剂量的MNU可使视网膜ERG波幅明显降低(均为P<0.001),视网膜外核层(outer nuclear layer,ONL)厚度明显变薄(P<0.001),损伤严重;与对照组相比,60 mg·kg^(-1)的MNU作用后1 d和3 d,视网膜ERG波形开始降低,形态结构开始出现ONL厚度变薄的损伤,作用7 d时,ERG波形呈现熄灭型(均为P<0.001),ONL厚度明显变薄(P<0.001),内外核层融合,损伤严重。与MNU单独作用组相比,60 mg·kg^(-1)MNU作用1 d后给予MSCs移植,7 d后MSCs组内ONL厚度增加(P<0.001),视网膜ERG波形趋于恢复(均为P<0.001)。结论MSCs移植对MNU诱导的视网膜退行性变有一定的治疗作用。

5例儿童色素性玫瑰糠疹的临床与病理分析

目的了解儿童色素性玫瑰糠疹的临床表现及组织病理特点。方法回顾性分析5例儿童色素性玫瑰糠疹患儿临床表现、组织病理及治疗效果等。结果5例患儿中,男1例,女4例,男女比例1∶4;发病年龄为5~16岁,平均9.4岁;病程1个月~6年,平均23.2个月。皮损表现为躯干及四肢散在分布淡褐色或黑褐色斑疹,皮疹长轴大致与皮纹方向一致。组织病理主要表现为表皮角化过度,基底层黑素细胞不同程度增多。采用维生素C、维生素E和抗组胺药物等以及外用润肤剂治疗后,所有患儿皮疹1~3个月后消退。结论该病根据临床表现及组织病理变化可诊断,目前尚无特效疗法,临床以对症治疗为主。

无色素性视网膜色素变性1例

报告1例2019年1月因无色素性视网膜色素变性而就诊的病例。患者因发现视力差,常规眼科检查及全身的检查未发现异常,给予眼底荧光造影后确诊。给予眼底荧光造影后最终确诊为罕见的无色素性视网膜色素变性,防止了疾病的漏诊和误诊。对于缺乏视网膜色素变性典型的三联征的无色素性视网膜色素变性患者,临床要谨防漏诊,眼底荧光血管造影(fundus fluorescein angiography,FFA)可明确诊断。

PCDH15基因复合杂合新突变致无色素性视网膜色素变性表型的1F型Usher综合征一家系

目的确定1个具有无色素性视网膜色素变性(RPSP)表型的Usher综合征(USH)家系的致病基因及其与眼部表现相关性。方法回顾性临床研究。2019年11月于河南省人民医院眼科门诊检查确诊的具有RPSP表现的1F型USH患儿1例和其父母纳入研究。患儿女,9岁。双眼夜盲4年余;听力下降7年,目前双耳感音神经性耳聋。双眼最佳矫正视力0.5+。眼底未见明显色素沉着。外围视野视敏度下降。光相干断层扫描检查,周边视网膜外层变薄,椭圆体带消失。视网膜电图检查,视杆、视锥系统反应重度下降。患儿父母临床表型正常。抽取患儿及其父母外周静脉血,提取全基因组DNA,采用自主研发的靶向捕获试剂盒(PS400),使用二代基因测序技术检测基因变异,对可疑致病突变位点通过Sanger测序进行验证,并在家系成员中进行共分离。依据序列变异解读标准和指南对变异进行致病性评估;利用生物信息学技术评估变异对编码蛋白的影响。结果基因检测结果显示,先证者检测到PCDH15基因c.4109dupA(p.K1370fs)(M1)、c.17dupA(p.Y6_L7delinsX)(M2)复合杂合突变位点,经Sanger测序验证,变异在该家系中呈共分离状态。经序列变异解读标准和指南评估,M1、M2均为PCDH15基因致病性变异,M1导致编码蛋白跨膜结构完全改变,M2导致基因仅能翻译出6个氨基酸,预测不能合成PCDH15蛋白。根据临床表型、基因变异致病性以及蛋白结构预测,最终临床诊断为PCDH15相关1F型USH。结论PCDH15基因c.4109dupA、c.17dupA为该家系患儿USH的致病突变位点,该复合杂合新突变导致PCDH15蛋白无法正常合成,从而引起眼部及耳部表现。