Vincent Ajoy, Ng Judith, Gerth-Kahlert Christina, Tavares Erika, Maynes Jason T, Wright Thomas, Tiwari Amit, Tumber Anupreet, Li Shuning, Hanson James V M, Bahr Angela, MacDonald Heather, Bähr Luzy, Westall Carol, Berger Wolfgang, Cremers Frans P M, den Hollander Anneke I, Héon Elise
Program of Genetics and Genome Biology The Hospital for Sick Children, Toronto, Canada 2Department of Ophthalmology and Vision Sciences, The Hospital for Sick Children, University of Toronto, Toronto, Canada 3Department of Ophthalmology and Vision Science.
Program of Genetics and Genome Biology The Hospital for Sick Children, Toronto, Canada.
Invest Ophthalmol Vis Sci. 2016 May 1;57(6):2637-46. doi: 10.1167/iovs.15-18281.
To identify the genetic cause of autosomal recessive familial foveal retinoschisis (FFR).
A female sibship with FFR was identified (Family-A; 17 and 16 years, respectively); panel based genetic sequencing (132 genes) and comparative genome hybridization (142 genes) were performed. Whole-exome sequencing (WES) was performed on both siblings using the Illumina-HiSeq-2500 platform. A sporadic male (Family-B; 35 years) with FFR underwent WES using Illumina NextSeq500. All three affected subjects underwent detailed ophthalmologic evaluation including fundus photography, autofluorescence imaging, spectral-domain optical coherence tomography (SD-OCT), and full-field electroretinogram (ERG).
Panel-based genetic testing identified two presumed disease causing variants in CRB1 (p.Gly123Cys and p.Cys948Tyr) in Family-A sibship; no deletion or duplication was detected. WES analysis in the sibship identified nine genes with two or more shared nonsynonymous rare coding sequence variants; CRB1 remained a strong candidate gene, and CRB1 variants segregated with the disease. WES in Family-B identified two presumed disease causing variants in CRB1 (p.Ile167_Gly169del and p.Arg764Cys) that segregated with the disease phenotype. Distance visual acuity was 20/40 or better in all three affected except for the left eye of the older subject (Family-B), which showed macular atrophy. Fundus evaluation showed spoke-wheel appearance at the macula in five eyes. The SD-OCT showed macular schitic changes in inner and outer nuclear layers in all cases. The ERG responses were normal in all subjects.
This is the first report to implicate CRB1 as the underlying cause of FFR. This phenotype forms the mildest end of the spectrum of CRB1-related diseases.
确定常染色体隐性遗传性黄斑视网膜劈裂症(FFR)的遗传病因。
确定了一个患有FFR的女性同胞关系家族(A家族;分别为17岁和16岁);进行了基于基因panel的测序(132个基因)和比较基因组杂交(142个基因)。使用Illumina-HiSeq-2500平台对两个同胞进行了全外显子组测序(WES)。一名患有FFR的散发男性(B家族;35岁)使用Illumina NextSeq500进行了WES。所有三名受影响的受试者均接受了详细的眼科评估,包括眼底照相、自发荧光成像、光谱域光学相干断层扫描(SD-OCT)和全视野视网膜电图(ERG)。
基于基因panel的基因检测在A家族同胞中鉴定出CRB1基因中的两个推测致病变异(p.Gly123Cys和p.Cys948Tyr);未检测到缺失或重复。该同胞关系家族的WES分析鉴定出九个具有两个或更多共享非同义罕见编码序列变异的基因;CRB1仍然是一个强有力的候选基因,且CRB1变异与疾病相关。B家族的WES鉴定出CRB1基因中的两个推测致病变异(p.Ile167_Gly169del和p.Arg764Cys),它们与疾病表型相关。除了年龄较大的受试者(B家族)的左眼出现黄斑萎缩外,所有三名受影响者的远视力均为20/40或更好。眼底评估显示五只眼睛的黄斑区呈辐轮状外观。所有病例的SD-OCT均显示内、外核层的黄斑劈裂改变。所有受试者的ERG反应均正常。
这是首次报道CRB1是FFR的潜在病因。这种表型构成了CRB1相关疾病谱系中最轻微的一端。
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