Simultaneous Mutation Detection in 90 Retinal Disease Genes in Multiple Patients Using a Custom-designed 300-kb Retinal Resequencing Chip

Booij, Judith C.; Bakker, Arne; Kulumbetova, Jamilia; Moutaoukil, Youssef; Smeets, Bert; Verheij, Joke; Kroes, Hester Y.; Klaver, Caroline C.W.; van Schooneveld, Mary; Bergen, Arthur A.B.; Florijn, Ralph J.

doi:10.1016/j.ophtha.2010.04.022

« Previous Next »Ophthalmology
Volume 118, Issue 1 , Pages 160-167.e3, January 2011

Simultaneous Mutation Detection in 90 Retinal Disease Genes in Multiple Patients Using a Custom-designed 300-kb Retinal Resequencing Chip

Judith C. Booij, MD, PhD
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
Arne Bakker, BSc
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
Jamilia Kulumbetova, MD, PhD
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
Youssef Moutaoukil, BSc
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
Bert Smeets, PhD
- Clinical Genetics University Maastricht, The Netherlands
Joke Verheij, MD, PhD
- Genetics, University Medical Center, Groningen, The Netherlands
Hester Y. Kroes, MD, PhD
- Medical Genetics, University Medical Center Utrecht, The Netherlands
Caroline C.W. Klaver, MD, PhD
- Ophthalmology, Erasmus Medical Centre Rotterdam, The Netherlands
Mary van Schooneveld, MD, PhD
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
Arthur A.B. Bergen, PhD
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands
- Clinical Genetics, Academic Medical Centre Amsterdam, The Netherlands
- Ophthalmology, Academic Medical Centre Amsterdam, The Netherlands
- Correspondence: Arthur A. B. Bergen, NIN, Department of Clinical and Molecular Ophthalmogenetics, Meibergdreef 47, 1105 BA Amsterdam, The Netherlands
Ralph J. Florijn, PhD
- Departments of Clinical and Molecular Ophthalmogenetics, Netherlands Institute for Neuroscience, an institute of the Royal Netherlands Academy of Arts and Sciences, Amsterdam, The Netherlands

Received 19 October 2009; received in revised form 14 April 2010; accepted 14 April 2010. published online 31 August 2010.

Available online: August 30, 2010.

Purpose

To develop a high-throughput, cost-effective diagnostic strategy for the identification of known and new mutations in 90 retinal disease genes.

Design

Evidence-based study.

Participants

Sixty patients with a variety of retinal disorders, including Leber's congenital amaurosis, ocular albinism, pseudoxanthoma elasticum, retinitis pigmentosa, and Stargardt's disease.

Methods

We designed a custom 300-kb resequencing chip. Polymerase chain reaction (PCR) amplification, DNA fragmentation, and chip hybridization were performed according to Affymetrix recommendations. Hybridization signals were analyzed using Sequence pilot module seq-C mutation detection software (2009). This resequencing approach was validated by Sanger sequence technology.

Main Outcome Measures

Disease-causing sequence changes.

Results

We developed a retinal resequencing chip that covers all exons of 90 retinal disease genes. We developed and tested multiplex primer sets for 1445 amplicons representing the genes included on the chip. We validated our approach by screening 87 exons from 25 retinal disease genes containing 87 known sequence changes previously identified in our patient group using Sanger sequencing. Call rates for successfully hybridized amplicons were 98% to 100%. Of the known single nucleotide changes, 99% could be detected on the chip. As expected, deletions could not be detected reliably.

Conclusions

We designed a custom resequencing chip that can detect known and new sequence changes in 90 retinal disease genes using a new high-throughput strategy with a high sensitivity and specificity for one tenth of the cost of conventional direct sequencing. The developed amplification strategy allows for the pooling of multiple patients with non-overlapping phenotypes, enabling many patients to be analyzed simultaneously in a fast and cost-effective manner.

Financial Disclosure(s)

The author(s) have no proprietary or commercial interest in any materials discussed in this article.

To access this article, please choose from the options below

Manuscript no. 2009-1455.

Financial Disclosure(s): The author(s) have no proprietary or commercial interest in any materials discussed in this article.

Funded by the Algemene Nederlandse Vereniging ter Voorkoming van Blindheid, Landelijke Stichting voor Blinden en Slechtzienden, Rotterdamse Vereniging Blindenbelangen, Stichting Blindenpenning, Stichting Oogfonds Nederland, and Gelderse Blindenstichting.

PII: S0161-6420(10)00450-1

doi:10.1016/j.ophtha.2010.04.022

« Previous Next »Ophthalmology
Volume 118, Issue 1 , Pages 160-167.e3, January 2011

Access this article on SciVerse ScienceDirect