A missense founder mutation in VLDLR is associated with Dysequilibrium Syndrome without quadrupedal locomotion

For Family 1, a 5 K whole genome linkage SNP scan was performed using the Illumina Linkage IVb mapping panel [18] and analyzed with easyLinkage-Plus software [19]. The VLDLR candidate gene was sequenced using primers designed to amplify each of the coding exons and splice sites using the ExonPrimer software (http://​ihg.​gsf.​de/​ihg/​ExonPrimer.​html) as described [8]. For Family 2, exome sequence was generated from individual IV-8, by exome capture with the Agilent SureSelect Human All Exome 50 Mb kit, sequenced on an Illumina HiSeq2000 instrument, resulting in ~95% recovery at >10x coverage. GATK software [20] was used for variant identification. These variants were used to identify identity-by-descent blocks with the online software HomozygosityMapper [21], set to analysis of blocks containing 200 markers and only flag blocks > 100 markers in a row. Variants were annotated using SeattleSeq (http://​snp.​gs.​washington.​edu/​SeattleSeqAnnota​tion/​) to identify homozygous potentially deleterious variants. For SNP genotyping, informative markers from Family 1 were selected based upon the previous 5 K SNP genotyping results surrounding the VLDLR gene at 100,000-1,000,000 bp intervals on chromosome 9 and amplified in one affected individual from each Family and from a healthy control individual. PCR amplification was carried out using a standard touchdown PCR protocol. After successful amplification, PCR products were sequenced on an ABI 3730 sequencer (Applied Biosystems, Foster City, CA, USA) and analyzed using Sequencher software (Genecode, Inc).

In order to identify the genetic cause of disease in Family 1, we performed linkage analysis using a 5 K SNP linkage panel on each of the members of generation III and IV, and identified one linkage peak on chromosome 9 (Figure 3A) that overlapped the VLDLR gene locus, known to cause DES [8]. An additional linkage peak on chromosome 1 did not contain genes known to cause neurological disturbances. Direct sequence of each of the 17 exons including canonical splice sites from individual IV-4 revealed a single probable pathogenic mutation (Figure 3B) in exon 15 of the VLDLR gene at base position chr9:2650382 G > T according to the hg19 build of the human genome. For Family 2, because we had no reason to suspect VLDLR gene mutations over the other DES genes or potentially novel causes, exome sequencing of the affected child from generation IV (IV-8) was performed and revealed the same chr9:2650382 G > T mutation (Figure 3B). This alteration resulted in a c.2117 G > T nucleotide change and a p.C706F amino acid substitution in the transcript NP_003374.3. This change resulted in altering a cysteine residue that is conserved across all of vertebrate evolution (Figure 3C). The variant produced a Grantham score of 205 and a PhastCon score of 1.0 [22, 23]. In addition, the mutation was predicted by PolyPhen-2 [24] to be probably damaging with a score of 1.0, which is the highest score possible. Furthermore, the mutation was not identified in dbGaP nor was it encountered in over 1000 exome sequence analyses from Middle Eastern patients with other diseases in our in-house database.

The finding that the two families shared a common genetic mutation in the VLDLR gene suggested the possibility of a common founder mutation. In order to test for a shared affected haplotype, we designed PCR primers at spaced intervals surrounding the VLDLR mutation, which were selected to be informative in Family 1 from the previous 5 K SNP analysis. Amplification from Family 1 IV-4 and Family 2 IV-8 showed PCR products of the predicted sizes for all amplicons, and sequence analysis of each SNP was in full agreement with Family 1 previous SNP analysis. Family 2 genotyping showed identical homozygous calls for SNPs rs1535842, rs1331829, rs729367, rs1455175, from base position 2,212,796-3,796,061 on chromosome 9, or a distance of approximately 1,500,000 base pairs (Table 2). This haplotype was not encountered in any of ~100 UAE individuals on whom whole genome SNP results were reviewed in our lab, suggesting that the mutation occurred on a uniquely shared haplotype and segregated in the two families.