1 / 25

Eleanor Reavey West of Scotland Regional Genetics Laboratory Yorkhill Hospital Glasgow

Development of a molecular genetic diagnostic service for X-linked ichthyosis, with emphasis on carrier detection. Eleanor Reavey West of Scotland Regional Genetics Laboratory Yorkhill Hospital Glasgow. Introduction.

errin
Download Presentation

Eleanor Reavey West of Scotland Regional Genetics Laboratory Yorkhill Hospital Glasgow

An Image/Link below is provided (as is) to download presentation Download Policy: Content on the Website is provided to you AS IS for your information and personal use and may not be sold / licensed / shared on other websites without getting consent from its author. Content is provided to you AS IS for your information and personal use only. Download presentation by click this link. While downloading, if for some reason you are not able to download a presentation, the publisher may have deleted the file from their server. During download, if you can't get a presentation, the file might be deleted by the publisher.

E N D

Presentation Transcript

  1. Development of a molecular genetic diagnostic service for X-linked ichthyosis, with emphasis on carrier detection Eleanor Reavey West of Scotland Regional Genetics Laboratory Yorkhill Hospital Glasgow

  2. Introduction • Associated with STS deficiency in fibroblasts and ↑ plasma cholesterol sulphate • X-linked recessive inheritance • 1 in 2000-6000 males • STS gene - Xp22.3 • 10 exons

  3. STS enzyme Responsible for hydrolysis of cholesterol sulfate (CS) to cholesterol in epidermis XLI – accumulation of CS in epidermis leads to barrier instability and inhibits desmosomal degradation Phenotype Scaly skin on scalp, trunk and limbs Corneal opacities

  4. Placental sulphatase deficiency • Placenta – STS-rich tissue • STS is involved in steroid conversion pathway: cholesterol  estriol • Deficiency associated with: • longer gestation and poor cervical dilatation • Results in slowing of delivery + indicates need for C-section or instrumental delivery • ↑ perinatal morbidity + mortality

  5. Associated Conditions • Approx. 90% of XLI individuals – complete deletion of the STS gene • More extensive deletions - contiguous gene deletion syndromes • Kallmann syndrome • Short stature • X-linked chondrodysplasia punctata • X-linked ocular albinism • ADHD

  6. Biochemical Analysis • STS activity is measured on white cells or cultured fibroblasts • Radiolabelled assay with 3H Dehydroepiandrosterone sulphate as a substrate • Affected males are tested for presence or absence of STS gene by PCR • No info on any intragenic deletions or point mutations

  7. Mutations • Several point mutations in STS gene identified • No evidence of genotype-phenotype correlation, regardless of the location or type of the STS mutation • production of a catalytically inactive STS enzyme • both the N-terminal region and the C-terminal region of the STS protein are important for enzyme activity

  8. Initial referral • Patient NH clinically affected with XLI • No enzyme activity detected • But, normal result for gene deletion analysis • Request from Dundee for full seq screen of STS coding exons (1-10), including intron/exon boundaries • Primers designed for sequencing

  9. Y chr Pseudogene • Transcriptionally inactive at the promoter • Several exons deleted • Significant sequence homology between X-STS and Y-STS genes

  10. Results from Temperature Gradient PCR • 55°C - 65°C • Example gel for exons 1-8 Exon 1 2 3 4 5 6 7 8 55C 58C 60C 62C 65C

  11. NHc.583delGp.Val195SerfsX19

  12. Further Testing • Screening of NH’s mother confirmed her as a carrier. • Second referral – Edinburgh • Patient JM clinically affected, no STS activity and normal result on gene deletion analysis

  13. JMc.387_391dupAGCACp.Leu131GlnfsX3

  14. Extended Testing • A further 10 samples were received from Dr Graham • Dosage analysis carried out to confirm presence of STS gene • Full sequencing screen carried out on all 10 exons • Four additional mutations detected = high pickup rate

  15. STS dosage analysis DMD 53 STS 5’ DMD 17 STS 3’ DMD 51

  16. MDc.1046_1048delAGGp.Glu349del

  17. TTc.1649G>Ap.Trp550X

  18. AEc.1360C>Tp.Arg454Cys

  19. JAc.494C>Tp.Thr165Ile

  20. MLPA kit P160 • Probes for each of 10 exons • Other probes include KAL1 and NLGN4X • In female heterozygotes, 35-50% reduced relative peak area of amplified product expected • Deletion of one exon – needs to be confirmed by sequencing to rule out mutation/ polymorphism close to probe ligation site

  21. Carrier testing in females

  22. Current testing strategy for XLI in Glasgow • Enzyme activity measured and gene deletion PCR carried out in Biochemical Genetics • Dosage assay available in Molecular Genetics Lab to identify female carriers • MLPA better suited for carrier testing – detects single (or multiple) exon deletions/ duplications as well as deletions of entire gene

  23. Sample is received by Biochemical Genetics at Yorkhill Hospital for XLI diagnostic analysis Steroid sulphatase enzyme analysis carried out on white cells -ve +ve Report patient as negative for XLI Dosage analysis to identify partial/ full STS gene deletions +ve Report patient is affected with XLI due to a STS gene deletion -ve Full screen sequencing of 10 coding exons of STS gene to identify point mutations Offer mother, and other family members, MLPA testing for carrier status -ve Confirm XLI diagnosed biochemically however, genetic basis is unknown Offer mother, and other family members, STS sequence testing for identified point mutation

  24. Summary • Service offered for males affected with XLI – dosage analysis + full screen sequencing for point mutations • Carrier testing for mothers • Important for genetic counselling for future pregnancies and for predicting risk of difficult labour

  25. Acknowledgements • Molecular Genetics Lab, Yorkhill, Glasgow • Su Stenhouse, Sandy Cooke • Biochemical Genetics Lab, Yorkhill, Glasgow • Gordon Graham

More Related