Development of High-Throughput Clinical Testing of RPGR ORF15 Using a Large Inherited Retinal Dystrophy Cohort

John P W Chiang; Tina M Lamey; Nicholas K Wang; Jie Duan; Wei Zhou; Terri L McLaren; Jennifer A Thompson; Jonathan Ruddle; John N De Roach

doi:10.1167/iovs.18-24555

Development of High-Throughput Clinical Testing of RPGR ORF15 Using a Large Inherited Retinal Dystrophy Cohort

Invest Ophthalmol Vis Sci. 2018 Sep 4;59(11):4434-4440. doi: 10.1167/iovs.18-24555.

Authors

John P W Chiang¹, Tina M Lamey^{2

3}, Nicholas K Wang¹, Jie Duan¹, Wei Zhou⁴, Terri L McLaren², Jennifer A Thompson², Jonathan Ruddle⁵, John N De Roach^{2

3}

Affiliations

¹ Molecular Vision Laboratory, Hillsboro, Oregon, United States.
² Australian Inherited Retinal Disease Registry and DNA Bank, Department of Medical Technology and Physics, Sir Charles Gairdner Hospital, Nedlands, Western Australia, Australia.
³ Centre for Ophthalmology and Visual Science, The University of Western Australia, Crawley, Western Australia, Australia.
⁴ Centrillion Technologies, Palo Alto, California, United States.
⁵ Royal Children's Hospital, Melbourne, Victoria, Australia.

PMID: 30193314
DOI: 10.1167/iovs.18-24555

Abstract

Purpose: Mutations in the ORF15 region of RPGR account for approximately half of all X-linked retinitis pigmentosa cases. However, a robust high-throughput method for the detection of ORF15 mutations has yet to be validated. We set out to develop the first clinically validated next-generation sequencing (NGS) method for the detection of mutations in this difficult-to-sequence region, including test accuracy and coverage data.

Methods: As part of a blind-test, 145 research samples, previously tested by Sanger sequencing, and 81 clinical samples were evaluated using NGS of long-range PCR products fragmented with Illumina's Nextera library preparation kit (method 1), or with Centrillion's OneTube technology, supplemented with duplication analysis using an ORF15-specific in-silico array (method 2). DNA fragments were analyzed using Agilent's DNA 1000 assay, and sequencing was done on Illumina's MiSeq 2×150 or HiSeq2500 2×100. NextGENe by SoftGenetics was used for data analysis and variant calling.

Results: The Nextera library preparation method produced 24 cases of discordance due to (in order of decreasing occurrence) false-negatives, incorrectly called variants, and a false-positive. Subsequent use of a new, OneTube NGS library preparation method, supplemented with duplication analyses, resolved discordance between Sanger and NGS data in all cases. This improvement in variant detection accuracy was largely attributed to improvement in random fragmentation offered by the enzymatic OneTube method, resulting in more complete coverage of the highly repetitive ORF15 region. Minimum coverage was roughly 320 reads for Nextera and 6800 reads for OneTube (normalized for total read counts).

Conclusions: This paper documents the first clinically validated NGS method for reliable, high-throughput sequencing of RPGR ORF15. Sensitivity and specificity of the new method were 100%, with the caveat of unclear zygosity calling for one large duplication case. These findings demonstrate a reliable and practical implementation for NGS-based diagnosis of RPGR ORF15 mutations. They also provide the foundation for targeted, high-coverage sequencing of any other repetitive regions within the genome.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adult
Cohort Studies
DNA Mutational Analysis
Eye Proteins / genetics*
Female
Genetic Diseases, X-Linked / diagnosis*
Genetic Diseases, X-Linked / genetics
High-Throughput Nucleotide Sequencing*
Humans
Male
Mutation*
Open Reading Frames / genetics*
Pedigree
Polymerase Chain Reaction
Reproducibility of Results
Retinitis Pigmentosa / diagnosis*
Retinitis Pigmentosa / genetics
Sensitivity and Specificity

Substances

Eye Proteins
RPGR protein, human