Molecular characterization of CPS1 deletions by array CGH

Wang, Jing; Shchelochkov, Oleg A.; Zhan, Haifei; Li, Fangyuan; Chen, Li-Chieh; Brundage, Ellen K.; Pursley, Amber N.; Schmitt, Éric; Häberle, Johannes; Wong, Lee‐Jun C.

doi:10.1016/j.ymgme.2010.08.020

Cited by 12 publications

(10 citation statements)

References 19 publications

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“…As reported before, 11 distribution of CPS1 mutations shows predominance of the catalytic domains (116 of 172 mutations): the bicarbonate phosphorylation domain (exons [13][14][15][16][17][18][19][20] was affected by 61 mutations and the carbamate phosphorylation domain (exons 25-34) by 55 mutations ( Figure 2).…”

Section: Methodsmentioning

confidence: 53%

“…More than 230 CPS1 mutations are currently reported . Molecular genetic investigation for CPS1D can use different methods: exon per exon sequencing (direct Sanger sequencing), next generation sequencing (NGS) as part of a (often custom‐made) gene panel or whole exome or whole genome sequencing with or without the analysis of copy number variation (CNV), and RNA analysis …”

Section: Introductionmentioning

confidence: 99%

“…[7][8][9][10][11][12][13][14][15] Molecular genetic investigation for CPS1D can use different methods: exon per exon sequencing (direct Sanger sequencing), next generation sequencing (NGS) as part of a (often custom-made) gene panel or whole exome or whole genome sequencing with or without the analysis of copy number variation (CNV), and RNA analysis. [16][17][18] While automated sequencing applying NGS became more widely available in recent years and showed improved detection rates if compared to direct Sanger sequencing, 19 our laboratory performed in most cases RNA analysis for the confirmation of CPS1D. 6,16 Source of RNA can be liver tissue but also skin fibroblasts 17 or, hereby improving the turn-around time, peripheral lymphocytes that were stimulated with phytohemagglutinin hereby applying a straightforward and less invasive protocol.…”

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confidence: 99%

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Improvement of diagnostic yield in carbamoylphosphate synthetase 1 (CPS1) molecular genetic investigation by RNA sequencing

et al. 2020

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Carbamoylphosphate synthetase 1 (CPS1) deficiency is a rare inborn error of metabolism leading often to neonatal onset hyperammonemia with coma and high mortality. The biochemical features of the disease are nonspecific and cannot distinguish this condition from other defects of the urea cycle, namely N‐acetylglutamate synthase deficiency. Therefore, molecular genetic investigation is required for confirmation of the disease, and nowadays this is done with increasing frequency applying next‐generation sequencing (NGS) techniques. Our laboratory has a long‐standing interest in CPS1 molecular genetic investigation and receives samples from centers in Europe and many other countries. We perform RNA‐based CPS1 molecular genetic investigation as first line investigation and wanted in this study to evaluate our experience with this approach as compared to NGS. In the past 15 years, 297 samples were analyzed, which were referred from 37 countries. CPS1 deficiency could be confirmed in 155 patients carrying 136 different genotypes with only a single mutation recurring more than two times. About 10% of the total 172 variants comprised complex changes (eg, intronic changes possibly affecting splicing, deletions, insertions, or deletions_insertions), which would have been partly missed if only NGS was done. Likewise, RNA analysis was crucial for correct interpretation of at least half of the complex mutations. This study gives highest sensitivity to RNA‐based CPS1 molecular genetic investigation and underlines that NGS should be done together with copy number variation analysis. We propose that unclear cases should be investigated by RNA sequencing in addition, if this method is not used as the initial diagnostic procedure.

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Section: Methodsmentioning

confidence: 53%

Section: Introductionmentioning

confidence: 99%

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confidence: 99%

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Improvement of diagnostic yield in carbamoylphosphate synthetase 1 (CPS1) molecular genetic investigation by RNA sequencing

et al. 2020

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“…Of the variants, 81 (30.7%) were predicted to cause protein truncation, including 22 nonsense, 31 small deletions, 16 small insertions, 4 small indels, 6 splicing site changes, and 2 large deletions. Our reviewing data further clarified that most CPS1 variants (≥90%) were “private” with non-recurrence, and the few recurrent mutations tended to occur at CpG dinucleotides, which made the diagnosis more complicated ( Supplementary Tables S1 to S4 ) (Hoshide et al, 1993; Finckh et al, 1998; Summar et al, 1998; Ihara et al, 1999; Aoshima et al, 2001a; Aoshima et al, 2001b; Rapp et al, 2001; Wakutani et al, 2001; Häberle et al, 2003; Eeds et al, 2006; Kurokawa et al, 2007; Khayat, 2009; Ono et al, 2009; Pekkala et al, 2010; Häberle et al, 2011; Wang et al, 2011; Funghini et al, 2012; Kretz et al, 2012; Diez-Fernandez et al, 2014; Ali et al, 2016; Choi et al, 2017; Rokicki et al, 2017; Yang et al, 2017; Chen et al, 2018; Zhang et al, 2018).…”

Section: Discussionmentioning

confidence: 77%

Novel Neonatal Variants of the Carbamoyl Phosphate Synthetase 1 Deficiency: Two Case Reports and Review of Literature

et al. 2019

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Carbamoyl phosphate synthetase I (CPS1) deficiency (CPS1D), is a rare autosomal recessive disorder, characterized by life-threatening hyperammonemia. In this study, we presented the detailed clinical features and genetic analysis of two patients with neonatal-onset CPS1D carrying two compound heterozygous variants of c.1631C > T (p.T544M)/c.1981G > T (p.G661C), and c.2896G > T (p.E966X)/c622-3C > G in CPS1 gene, individually. Out of them, three variants are novel, unreported including a missense (c.1981G > T, p.G661C), a nonsense (c.2896G > T, p.E966X), and a splicing change of c.622-3C > G. We reviewed all available publications regarding CPS1 mutations, and in total 264 different variants have been reported, with majority of 157 (59.5%) missense, followed by 35 (13.2%) small deletions. This study expanded the mutational spectrum of CPS1 . Moreover, our cases and review further support the idea that most (≥90%) of the mutations were “private” and only ∼10% recurred in unrelated families.

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“…To detect copy number variations, two well established techniques are used. The method of CGH array [103,104] is able to detect copy number variations by measuring the fluorescence ratio between a reference and a sample, while the method of multiplex ligation-dependent probe amplification (MLPA) is able to detect genomic deletions and insertions of single nucleotides up to one or more entire exons.…”

Section: Future Prospectsmentioning

confidence: 99%

Mutation analysis of urea cycle disorders

Häberle

Rüfenacht

2016

J Pediatr Biochem

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Urea cycle disorders (UCDs) are a group of autosomal or X-linked, recessively inherited errors of metabolism that lead to severe neurological disease due to insufficient detoxification of excess nitrogen. The resulting hyperammonemia is the key feature of UCDs, but at the same time only a surrogate marker. In the majority of cases, a sole biochemical analysis is indicative but not diagnostic. Therefore, additional means are required and mutation analysis is the method of choice for confirmation in most cases of UCD. In addition to confirming the diagnosis, mutation analysis enables genetic counseling and prenatal testing and contributes to new research approaches. All genes involved in any of the enzymatic (namely the genes for N-acetylglutamate synthase, NAGS; carbamoylphosphate synthetase, CPS1; ornithine transcarbamylase, OTC; argininosuccinate synthetase, ASS1; argininosuccinate lyase, ASL; arginase, ARG1) or transporter steps (namely the genes for the ornithine/citrulline antiporter ORNT1, SLC25A15; glutamate/aspartate antiporter citrin, SLC25A13) of the urea cycle are known and thus accessible for genetic testing. In most situations, direct Sanger sequencing using DNA from peripheral blood cells can be done but there are exceptions to this such as in the case of the relatively large CPS1 gene which renders RNA based mutation analysis an attractive alternative. With this review, we provide an overview on the current methods used for mutation analysis of each UCD gene, we mention possible pitfalls and their solutions, and discuss alternative methods which may become standard in the future.

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Molecular characterization of CPS1 deletions by array CGH

Cited by 12 publications

References 19 publications

Improvement of diagnostic yield in carbamoylphosphate synthetase 1 (CPS1) molecular genetic investigation by RNA sequencing

Improvement of diagnostic yield in carbamoylphosphate synthetase 1 (CPS1) molecular genetic investigation by RNA sequencing

Novel Neonatal Variants of the Carbamoyl Phosphate Synthetase 1 Deficiency: Two Case Reports and Review of Literature

Mutation analysis of urea cycle disorders

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