Blepharoptosis (ptosis) is defined as the abnormal drooping of the upper eyelid and is a feature of many conditions. It can be in isolated or syndromic form, bilateral or unilateral and congenital or acquired. Previously we have carried out linkage analysis on a family with dominantly inherited congenital bilateral isolated ptosis and found the condition to be linked to a region of approximately 20 megabases of chromosome Xq24-Xq27.1 with a cumulative LOD score of 5.89. We now describe further analysis using array comparative genomic hybridisation (array CGH), fluorescence in situ hybridisation (FISH), long range PCR and sequencing. This has enabled us to identify and characterise at the level of DNA sequence an insertional duplication and rearrangement involving chromosomes 1p21.3 and a small quasipalindromic sequence in Xq27.1, disruption of which has been associated with other phenotypes but which is cosegregating with X-linked congenital bilateral isolated ptosis in this family. This work highlights the significance of the small quasipalindromic sequence in genomic rearrangements involving Xq27.1 and the importance of comprehensive molecular and molecular cytogenetic investigations to fully characterise genomic structural complexity.
Blepharoptosis, usually abbreviated to the term ptosis, is defined as the abnormal drooping of the upper eyelid. It can be bilateral or unilateral, congenital or acquired, in isolated or syndromic form and is a feature of many conditions. When present from birth it can impair the development of full visual acuity and is usually corrected by surgery. Congenital ptosis is caused by underdevelopment of the levator palpebrae superioris muscle which raises the eyelid. The underlying defect is unknown and may be myogenic or neurogenic. The condition can be familial and we have previously carried out linkage analysis on a UK pedigree with dominantly inherited congenital bilateral isolated ptosis which indicated that the causative locus lay within a critical region of approximately 20 Mb of Xq24-27.1 which has since been refined to a region of 18 Mb [
Because of the limitations of linkage analysis and the number of family members available we were unable to further refine the critical region in our family using this methodology. We now describe a different approach enabling detailed characterisation of a chromosomal rearrangement cosegregating with X-linked ptosis in this pedigree. Array competitive genome hybridisation (aCGH) identified the duplication of a fragment of chromosome 1p21.3 and fluorescence in situ hybridization (FISH) analysis showed the fragment to be inserted into Xq27.1. Likely areas for the insertion breakpoints were then identified by conducting an in silico search for 1) repetitive sequences common to both the critical region of the X chromosome as identified by FISH and the ends of the inserted fragment as identified by aCGH and 2) potential fragile sites. Long-range PCR across candidate loci was then performed, failure of amplification in patient DNA compared with controls indicating that the insertion lay between specific primers. Subsequent PCR was then carried out using the same X chromosome primers paired with primers homologous to the ends of the inserted chromosome 1 sequence to generate a PCR product spanning the breakpoint. DNA sequencing was then performed to identify the exact location of the insertion in Xq27.1, involving a palindromic sequence previously identified as a site of interchromosomal insertions associated with other phenotypes [
In order to exclude the presence of another causative mutation within the 18 Mb critical region of the X chromosome derived from linkage data, exome sequencing was also performed.
Affected family members exhibit dominantly inherited congenital isolated bilateral ptosis. There is no evidence of epicanthus inversus, blepharophimosis or prevailing ocular motility disorder. Ptosis is symmetrical and equal in both males and females and results in an abnormally low upper eyelid position that impinges upon the visual axis in the primary position of gaze. There is minimal levator function bilaterally, absence of the upper lid skin crease, pronounced frontalis overaction, a characteristic chin-up head posture and no evidence of progression or variability of ptosis. The family pedigree is shown in
Array CGH analysis was performed initially using a 244 k Agilent array (reference 014693, Agilent Technologies, Santa Clara, CA) followed by an 8 × 60 k custom array (Agilent reference 024453) built on an Agilent
4 × 44 k backbone with coverage of approximately 1 probe per 100 base pairs of the approximately 120 kb area of chromosome 1p21.3 shown to be duplicated by the 244 k array.
FISH was performed using fluorescence labelled bacterial artificial chromosome clones (BACs) and a plasmid artificial chromosome clone (PAC) from the 30 k human tiling path clone set (ensembl.org/homo_sapiens/index) and standard protocols. A duplication of part of the chromosome 1 DPYD gene (dihydropyrimidine dehydrogenase, MIM 612779), identified by array CGH was verified using the 1p21.3 specific BAC clone RP11-359C24. Further analysis using RP11-359D24 together with Xq27 specific probes BAC RP11-197K18 and PAC RP1- 177G6 refined the location of the duplicated fragment.
Dosage analysis was carried out using MLPA [
Likely sites of insertion of the DPYD fragment in the X chromosome were identified by an in silico search for homologous sequences common to the critical region of chromosome Xq (as defined by FISH) and the duplicated fragment of the DPYD gene near the breakpoint areas as defined by array CGH. 1 kb of sequence at either end of the duplicated fragment was analysed using the BLAT sequence alignment program (genome. ucsc.edu/cgi-bin/hgBlat) to search for homologous sequences in the X chromosome critical region. A second in silico analysis involved a search for AT dinucleotide rich regions (commonly associated with fragile sites) within the X chromosome critical region. The X chromosome sequence was downloaded from Ensembl (ensembl.org) as a text file and a Microsoft Word search function was used to identify AT dinucleotide rich regions within the critical region.
Long range PCR was carried out using the “Expand long template system” and buffer 2 (Roche) according to the manufacturer’s protocol. Primers were designed within the X chromosome critical region to give a product of approximately 7.5 kb in a normal control individual (primer sequences available upon request). PCR was then performed using normal male controls and males with the partial DPYD gene insertion with the premise that the insertion would render the PCR fragment too large to amplify in affected males but not in normal controls. The long range PCR was focused on areas of the critical region of the X chromosome highlighted by in silico analysis.
Following the identification by long range PCR of the approximate site of insertion of the DPYD gene fragment within a 7.5 kb fragment of the X chromosome, PCR amplification of genomic DNA was performed using combinations of primers from the ends of the inserted DPYD fragment and the relevant long range PCR primers on the X chromosome (primer sequences available on request) to generate a fragment spanning the insertion breakpoint. Reactions were in a 25 μl volume containing 50 ng DNA, 1mM forward primer, 1 mM reverse primer, 2.5 μl 10× reaction buffer (Perkin Elmer), 0.16 mM dNTPs, 1.5 mM MgCl2, 0.5 u Taq polymerase (Taq Gold, Perkin Elmer). Cycling parameters were 94˚C for 12 minutes followed by 35 cycles of 94˚C for 30 seconds, 60˚C for 30 seconds and 72˚C for 30 seconds. PCR products were sequenced bi-directionally using the Big Dye™ Terminator v1.1 cycle sequencing kit (Applied Biosystems, Warrington, UK) using the same primers as for PCR amplification. Results were analysed with Mutation Surveyor version 3.2 (Soft Genetics, State College, PA).
Exome sequencing was carried out on two affected second-cousins from generation VI of the pedigree. Exome capture and sequencing were conducted at the Wellcome Trust Centre for Human Genetics at Oxford University. Data analysis was performed by using an in-house software pipeline, consisting of Novoalign (Novocraft Technologies, Selangor, Malaysia) for read alignment, Samtools [
Array CGH analysis of an affected female member of the pedigree with the Agilent 244 k array detected a duplication of 13 probes on chromosome 1p21.3. Further array CGH analysis on six affected and two unaffected family members using the 8 × 60 k custom array, which included dense coverage of the duplicated area of chromosome 1, showed 1163 probes to be duplicated and indicated the duplication to be a maximum of bases 1: 97,886,245-98,006,232 and a minimum of bases 1: 97,886,322-98,006,161. The duplication was present in all six affected individuals tested and absent in two unaffected individuals (
FISH analysis using chromosome 1 BAC probe RP11-359C24, which contains the duplicated fragment, showed the duplicated segment of chromosome 1 to be inserted into chromosome Xq27.1 (
MLPA analysis confirmed the presence of the duplication in five affected family members and its absence in five unaffected family members (data not shown). It was also shown to be present in two unaffected carrier females previously shown by linkage analysis to have the “at risk” Xq haplotype (see Section 4).
BLAT analysis (genome.ucsc.edu/cgi-bin/hgBlat) to look for homologous DPYD gene fragment sequences failed to find any significant matches within the X chromosome critical region. However the search for an
AT-rich region identified an area of the X chromosome spanning approximately 2 kb of sequence (X: 139,493,405-139,495,484) within the 1 Mb critical region defined by FISH.
PCR amplification was performed with a series of X chromosome specific primer pairs in the region of the X chromosome containing the AT-rich region identified above. One primer pair (covering fragment X: 139,498,501-139,506,034) gave a PCR product of the expected size with control DNA but no product with DNA from affected males (
Subsequent PCR analysis to identify the second X: 1 junction point was unable to generate a product using a primer located close to the distal end of the inserted chromosome 1 sequence paired with an X primer immediately distal to the X breakpoint at base 139,505,833. This suggested a more complex rearrangement than a simple insertion. PCR amplification with the insert specific primer paired with a range of X chromosome primers more distal to the breakpoint region was performed and the second chromosome X breakpoint was identified at base 139,502,960 which was within a 180 bp quasipalindromic sequence (
Further sequence analysis revealed additional complexity of the X chromosome rearrangement. A 427 base pair fragment (X: 139,505,833-139,506,259) has been duplicated, one copy of which is situated immediately distal to the inserted chromosome 1 segment. Also a 7 base pair sequence (X: 139,502,954-139,502,960) has been duplicated, one copy being situated immediately proximal to the inserted chromosome 1 segment (
PCR amplification across the distal junction was carried out on DNA from all available family members. The chromosome 1 primer (bases 98,006,082-98,006,100) paired with the X chromosome primer (bases 139,506,014-139,506,034) gave an amplification product with all 19 available affected family members and two unaffected females with the at risk haplotype. No product was generated from 16 unaffected family members without the at risk haplotype (data not shown).
No disease-causing mutations were identified within the 18 Mb critical region of the X chromosome (or elsewhere in the genome). All detected changes were known variants or single nucleotide polymorphisms.
We have identified an unbalanced insertional duplication of approximately 120 kb of the DPYD gene on chromosome 1p21.3 into Xq27.1, der (X) dir ins (X;1) (q27.1;p21.3), in a family with X linked dominant congenital bilateral isolated ptosis. The insertion is associated with a rearrangement of X chromosome sequences close to the site of insertion which includes a 427 base duplication and a 7 base duplication. The rearrangement segregates with the previously described familial at risk haplotype [
Our strategy to use aCGH and FISH, followed by in silico analysis to identify likely regions on the X chromosome for the insertion, has been successful. The search for an AT-rich region identified such a locus close to the X chromosome breakpoint. This directed the targeting of PCR analysis and subsequent characterisation of the DNA base sequence of the breakpoints.
There is no direct evidence that this rearrangement causes X-linked bilateral congenital ptosis. The rearrangement segregates with 18 Mb of chromosome Xq in all affected family members, so it is possible that a mutation elsewhere in this Xq fragment is causing the phenotype, although no evidence of a causative mutation was detected by exome sequencing. Such an insertion in this region of Xq is a rare event—we have only identified this one case in over 6000 samples analysed by array CGH in our laboratory, and we can only find three cases in the literature [
There are a number of possible mechanisms whereby the rearrangement may cause the ptosis phenotype. It could be caused by 1) disruption of a gene on the X chromosome 2) trisomy for the inserted DPYD fragment 2) position effect, i.e. the disruption of regulatory sequences of a nearby gene by the DYPD insertion or X sequence rearrangement or 3) the generation of a hybrid transcript involving the translocated DPYD exons and the exons of a nearby gene.
The insertion does not disrupt a known gene on the X chromosome, the closest genes on either side being SOX3 (MIM 313430), a transcription factor which is ~80 kb distal to the insertion and CXorf66, a predicted type 1 membrane protein, which is 458 kb proximal to the insertion.
Trisomy for the inserted DPYD fragment seems an unlikely cause for the ptosis phenotype. There is a possibility that the translocated exons 13 and 14 of DPYD could be expressed from the X chromosome and compromise the function of the normal DPYD gene, resulting in dihydropyrimidine dehydrogenase deficiency (MIM 274270), but ptosis is not a feature of this condition. We can find no other cases of a duplication of part of DPYD in the literature.
Position effect is a possibility as the site of insertion of the DPYD fragment is only 80 kb downstream of the 3’ end of SOX3, and there are numerous examples of position effect acting over this and much longer sequences of DNA [
Although there is evidence that position effect can influence SOX3 expression, there is no direct evidence that this may cause ptosis. Other phenotypes associated with SOX3 mutation or altered expression include mental retardation with panhypopituitarism (OMIM 300123), 46,XX male sex reversal [
The generation of a hybrid gene involving SOX3 and exons 13 and 14 of DPYD is a possibility. The two inserted DPYD exons are in the same orientation as the SOX3 gene and DPYD exon 13 is only ~100 kb from the 3’ end of SOX3. Such a hybrid would be likely to completely abrogate the functions of SOX3 and give a much more severe phenotype than ptosis, but if the hybrid transcript was present at a low level compared to the normal transcript it could have a lesser effect. SOX3 is a single exon gene and the generation of such a hybrid transcript would require the use of a cryptic splice donor site within the gene, in frame with the inserted exons of the DPYD gene. Analysis using five splice site prediction programs (interactive-biosoftware.com/alamut) has identified a putative cryptic donor site within SOX3 with a relatively high score for all 5 programs (core dinucleotide, SOX3 bases c.442 - 443, data not shown) which would remain in frame with the inserted DPYD exons, so this possibility is not excluded.
The nature of the rearrangement, as with many translocations [
Two cases with X-linked congenital hypertrichosis and insertional duplications into Xq27.1 described by Zhu et al. [
We have identified an insertion and duplication mutation in Xq27.1 cosegregating with X-linked congenital bilateral ptosis. The mutation is ~80 kb from the 3’ end of the SOX3 gene but we have no conclusive evidence to implicate SOX3 with the ptosis phenotype. A comparison with other cases with almost the same X chromosome breakpoint suggests that the position of the breakpoint alone does not define the resultant phenotype, which must therefore be defined by the nature of the inserted sequence and/or the duplication or deletion of X chromosome material.
This case adds to the evidence that a 180 bp quasipalindromic sequence in Xq27.1 is a hot spot for genomic recombination in an area where complex rearrangements are associated with a number of different abnormal phenotypes, dependent upon the nature of the genetic material that is inserted at this point.
We thank the family members for participating in this study. The work was supported by the TFC Frost charitable trust, The Salisbury Medical Society, Salisbury Hospitals Foundation, The British Council for Prevention of Blindness, The Wessex Medical Trust and the Mason Medical Research Foundation.