Department of Human Genetics, National Health Institute Doutor Ricardo Jorge, Lisbon, Portugal.
Department of Biological Sciences, University of Delaware, Newark, DE 19716, USA.
Exp Eye Res. 2018 Mar;168:161-170. doi: 10.1016/j.exer.2017.12.012. Epub 2018 Jan 2.
Keratolenticular dysgenesis (KLD) and ectopia lentis are congenital eye defects. The aim of this study is the identification of molecular genetic alterations responsible for those ocular anomalies with neurologic impairment in an individual with a de novo balanced chromosome translocation t(11;18)(q23.3;q11.2)dn. Disruption of OAF, the human orthologue of the Drosophila oaf, by the 11q23.3 breakpoint results in reduced expression of this transcriptional regulator. Furthermore, four most likely nonfunctional chimeric transcripts comprising up to OAF exon 3, derived from the der(11) allele, have also been identified. This locus has been implicated by publicly available genome-wide association data in corneal disease and corneal topography. The expression of the poliovirus receptor-related 1(PVRL1) or nectin cell adhesion molecule 1 (NECTIN1), a paralogue of nectin cell adhesion molecule 3 (PVRL3) associated with congenital ocular defects, situated 500 kb upstream from 11q23.3 breakpoint, is increased. The 18q11.2 breakpoint is localized between cutaneous T-cell lymphoma-associated antigen 1(CTAGE1) and retinoblastoma binding protein 8 (RBBP8) genes. Genomic imbalance that could contribute to the observed phenotype was excluded. Analysis of gene expression datasets throughout normal murine ocular lens embryogenesis suggests that OAF expression is significantly enriched in the lens from early stages of development through adulthood, whereas PVRL1 is lens-enriched until E12.5 and then down-regulated. This contrasts with the observation that the proposita's lymphoblastoid cell lines exhibit low OAF and high PVRL1 expression as compared to control, which offers further support that the alterations described above are most likely responsible for the clinical phenotype. Finally, gene interaction topology data for PVRL1 also agree with our proposal that disruption of OAF by the translocation breakpoint and misregulation of PVRL1 due to a position effect contribute to the observed ocular and neurological phenotype.
角膜晶状体发育不良(KLD)和晶状体异位是先天性眼部缺陷。本研究的目的是鉴定导致个体中与神经损伤相关的眼部异常的分子遗传改变,该个体存在从头获得的平衡染色体易位 t(11;18)(q23.3; q11.2)dn。11q23.3 断裂点处的果蝇 oaf 人同源物 OAF 的破坏导致该转录调节剂的表达减少。此外,还鉴定了源自 der(11)等位基因的多达 OAF 外显子 3 的四个最可能无功能的嵌合转录本。该基因座已通过公开的全基因组关联数据被牵连到角膜疾病和角膜地形图中。位于 11q23.3 断裂点上游 500kb 的脊髓灰质炎病毒受体相关 1(PVRL1)或连接蛋白细胞粘附分子 1(NECTIN1)的表达增加,该基因是连接蛋白细胞粘附分子 3(PVRL3)的旁系同源物,与先天性眼部缺陷有关,位于 11q23.3 断裂点上游 500kb。18q11.2 断裂点位于皮肤 T 细胞淋巴瘤相关抗原 1(CTAGE1)和视网膜母细胞瘤结合蛋白 8(RBBP8)基因之间。排除了可能导致观察到的表型的基因组不平衡。对正常鼠眼晶状体胚胎发生过程中的基因表达数据集的分析表明,OAF 表达在晶状体发育的早期阶段直至成年期显著富集,而 PVRL1 则在 E12.5 之前富集,然后下调。这与观察到的提议者的淋巴母细胞系与对照相比表现出低 OAF 和高 PVRL1 表达形成对比,这进一步支持了上述改变最有可能导致临床表型的观点。最后,PVRL1 的基因相互作用拓扑数据也与我们的假设一致,即易位断裂点处的 OAF 破坏和位置效应导致的 PVRL1 失调导致了观察到的眼部和神经表型。
