Mutation Screening of EXT1 and EXT2 by Denaturing High-Performance Liquid Chromatography, Direct Sequencing Analysis, Fluorescence in Situ Hybridization, and a New Multiplex Ligation-Dependent Probe Amplification Probe Set in Patients with Multiple Osteochondromas

Jennes, Ivy; Entius, Mark M.; Hul, Els Van; Parra, Alessandro; Sangiorgi, Luca; Wuyts, Wim

doi:10.2353/jmoldx.2008.070086

Cited by 48 publications

(68 citation statements)

References 33 publications

(42 reference statements)

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“…The positive rate of 9.3% for CREBBP intragenic deletions in 75 patients with Rubinstein-Taybi syndrome and of 7.3% for EXT1 or EXT2 deletions in 55 patients with multiple exostoses falls in the range reported by others. 10 Finally, consistent with previous reports, 1 out of 13 patients …”

Section: Autosomal Dominant Disorderssupporting

confidence: 80%

Exon-level array CGH in a large clinical cohort demonstrates increased sensitivity of diagnostic testing for Mendelian disorders

Aradhya¹,

Lewis²,

Bonaga³

et al. 2012

Genetics in Medicine

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Purpose: Mendelian disorders are most commonly caused by mutations identifiable by DNA sequencing. Exonic deletions and duplications can go undetected by sequencing, and their frequency in most Mendelian disorders is unknown. methods:We designed an array comparative genomic hybridization (CGH) test with probes in exonic regions of 589 genes. Targeted testing was performed for 219 genes in 3,018 patients. We demonstrate for the first time the utility of exon-level array CGH in a large clinical cohort by testing for 136 autosomal dominant, 53 autosomal recessive, and 30 X-linked disorders.Results: Overall, 98 deletions and two duplications were identified in 53 genes, corresponding to a detection rate of 3.3%. Approximately 40% of positive findings were deletions of only one or two exons. A high frequency of deletions was observed for several autosomal dominant disorders, with a detection rate of 2.9%. For autosomal recessive disorders, array CGH was usually performed after a single mutation was identified by sequencing. Among 138 individuals tested for recessive disorders, 10.1% had intragenic deletions. For X-linked disorders, 3.5% of 313 patients carried a deletion or duplication.conclusion: Our results demonstrate that exon-level array CGH provides a robust option for intragenic copy number analysis and should routinely supplement sequence analysis for Mendelian disorders. 2012:14(6):594-603 Genet Med

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Section: Autosomal Dominant Disorderssupporting

confidence: 80%

Exon-level array CGH in a large clinical cohort demonstrates increased sensitivity of diagnostic testing for Mendelian disorders

Aradhya¹,

Lewis²,

Bonaga³

et al. 2012

Genetics in Medicine

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“…In our patients with EXT1 and EXT2 mutations the tibia, femur and humerus were the most frequently affected bones, which explains the common complications and deformations seen in these bones by Jennes et al 2008. Our patients with EXT2 mutations showed a smaller number of affected bones.…”

Section: Discussionmentioning

confidence: 80%

“…The exon numbering is according to Clines et al 1997. MLPA analysis was performed with Salsa® MLPA® kit P215 (Jennes et al 2008). FISH analysis was performed with EXT1 cosmid probes 46F10 and 90D8 (Ahn et al 1995) to confirm large deletions.…”

Section: Patients and Clinical Studymentioning

confidence: 99%

Clinical and molecular studies of EXT1/EXT2 in Bulgaria

Stancheva-Ivanova

Wuyts

Hul

et al. 2011

J of Inher Metab Disea

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EXT1/EXT2-CDG (Multiple cartilagineous exostoses, hereditary multiple osteochondroma (MO); OMIM 133700/133701) are common defects of O-xylosylglycan glycosylation. The diagnostic criteria are at least two osteochondromas of the juxta-epiphyseal region of long bones with in the majority of cases a positive family history and/or mutation in one of the EXT genes. The authors report data on clinical symptoms and complications of 23 patients (from 16 families), discussing the family history, age of diagnosis, new clinical and molecular data. Fifteen mutations and large deletions, of which nine are new, were detected in the EXT1 and EXT2 gene by sequence analysis, FISH and MLPA analysis.

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“…Mutation screening of the EXT1 or EXT2 genes using standard sequencing for all exons including exon-intron junction points and MLPA testing using exon dedicated probe set for each exon coding regions were normal as reported earlier (Jennes et al, 2008;Wuyts et al, 2005). These mutation-negative patient samples were tested using the custom made EXT-tiling-array.…”

Section: Samplesmentioning

confidence: 99%

“…The complexity of osteochondroma formation, however, is not yet completely clarified by the bi-allelic inactivation as mosaic distribution of cells with retained chromosome 8 regions (presumably normal cells) was observed in the cartilage cap of both human osteochondromas and animal model systems (de Andrea et al, 2010;Jones et al, 2010;Bovee et al, 2010) The majority of the hereditary cases (70-75%) are caused by point mutations resulting in truncated proteins (Wuyts and Van Hul, 2000;Signori et al, 2007;Lonie et al, 2006;Pedrini et al, 2005;Jennes et al, 2009). Deletions involving single or multiple exons were found in about 10 % of all hereditary cases using Multiplex Ligation-dependent Probe Amplification (MLPA) (Jennes et al, 2008;Fredman et al, 2004;Vink et al, 2005). However, in about 10-15 % of the MO cases, genomic alterations can not be detected implying the potential role of other alterations such as inversions, translocations or somatic mosaicism (Vink et al, 2005).…”

Section: Introductionmentioning

confidence: 99%

Tiling resolution array-CGH shows that somatic mosaic deletion of the EXT gene is causative in EXT gene mutation negative multiple osteochondromas patients

et al. 2010

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Multiple osteochondromas (MO) is a hereditary skeletal disorder characterized by the presence of cartilage capped bony outgrowths at bone surface. Causative mutations in EXT1 or EXT2 genes have been described in 85-90 % of MO cases. However, in about 10-15 % of the MO cases, genomic alterations can not be detected, implying the potential role of other alterations. We have designed a custom-made Agilent oligonucleotide-based microarray, containing 44,000 probes, with tiling coverage of EXT1/2 genes and addition of 68 genes involved in heparan sulfate biosynthesis and other related pathways. Out of the 17 patient samples with previously undetected mutations, a low level of deletion of the EXT1 gene in about 10-15% of the blood cells was detected in two patients and mosaic deletion of the EXT2 was detected in one patient. Here we show that for the first time somatic mosaicism with large genomic deletions as the underlying mechanism in MO formation was identified. We propose that the existence of mosaic mutations and not alterations of other heparan sulfate biosynthesis related genes play a significant role in the development of MO in patients who are tested negative for mutations in Exostosins.

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Mutation Screening of EXT1 and EXT2 by Denaturing High-Performance Liquid Chromatography, Direct Sequencing Analysis, Fluorescence in Situ Hybridization, and a New Multiplex Ligation-Dependent Probe Amplification Probe Set in Patients with Multiple Osteochondromas

Cited by 48 publications

References 33 publications

Exon-level array CGH in a large clinical cohort demonstrates increased sensitivity of diagnostic testing for Mendelian disorders

Exon-level array CGH in a large clinical cohort demonstrates increased sensitivity of diagnostic testing for Mendelian disorders

Clinical and molecular studies of EXT1/EXT2 in Bulgaria

Tiling resolution array-CGH shows that somatic mosaic deletion of the EXT gene is causative in EXT gene mutation negative multiple osteochondromas patients

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