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Variable Expressivity of Neurodevelopmental Disturbances Due to Loss-of-Function of AP1S2
Objectives: To investigate genetic variants that would explain the ASD and ID segregating in 4 generations in a family with an X-linked inheritance pattern.
Methods: We selected two distant related cousins (individuals IV-2 and IV-4 in Figure 1), which belong to a family (Family F8293) with a total of 3 autistic individuals (individuals III-7, IV-2 and IV-4 in Figure 1) and 4 ID affected individuals (individuals II-4, II-5, III-6 and III-8 in Figure 1), to perform whole-exome sequencing (WES) using the Nextera Rapid Capture Exome kit (Illumina) for library preparation and sequencing on a HighSeq 2500 (Illumina). The alignment, processing, variant calling and annotation were carried out on BWA, GATK and ANNOVAR. To filter possible pathogenic variants we used a MAF<0.01, adopting as references 1000g, 6500 exomes and Brazilian control 60+ databases. Sanger sequencing was used to investigate if the selected candidate variants were shared among the other members of the family.
Results: We first search for shared variants between both cousins, but we did not detect any X-linked or autosomal variant that could explain the phenotype. Next, we searched for loss of function variants (LoFs) in brain expressed genes located in the chromosome X that were exclusive of each affected individual. In individual IV-4 we identified a stop codon variant in AP1S2. We verified that the same variant was shared among all other affected individuals, except for individual IV-2. AP1S2 is already associated with syndromic mental retardation, but it had not been linked to ASD yet. No relevant LoF variant in the X-chromosome or in autosomes of IV-2 was identified.
Conclusions: Our findings show the complexity of the analysis of each ASD family and highlight the relevance of another ID-associated gene to ASD.