Your search keyword '"angelman syndrome"' showing total 741 results

1. Imprinting analysis by droplet digital PCR coupled with locked nucleic acid TaqMan probes.

Author

Mitake M, Hirano S, and Kishino T

Subjects

DNA Methylation, Humans, Oligonucleotides, Polymerase Chain Reaction, Ubiquitin-Protein Ligases genetics, Angelman Syndrome genetics, Genomic Imprinting

Abstract

Imprinted genes are differentially expressed in a parent-of-origin-specific manner. Parental origin of the alleles is discriminated by intragenic DNA polymorphisms. Comparisons of parental allelic expression have been analysed by semiquantitative RT-PCR. Here, we developed a novel quantitative method for allelic expression of the imprinted gene Ube3a , which inactivation and mutations cause Angelman syndrome and predominantly expressed by the maternal allele in neuronal tissues. In this method, cDNA was amplified by droplet digital PCR (ddPCR) coupled with allele-specific locked nucleic acid (LNA) TaqMan probes, which labelled by FAM and HEX were designed to detect the SNPs in the target regions. ddPCR assay demonstrated that the sense transcript of Ube3a was equally expressed from both parental alleles in adult tissues except neuronal tissues, where Ube3a expression from the paternal allele was about 10 to 14% of total Ube3a expression in adult brain, and 20% in spinal cord. The antisense transcript of Ube3a was expressed at 60% to 70% of the sense transcript of Ube3a in adult brain. Changes in the Ube3a transcripts during postnatal brain development were also evaluated by ddPCR. The ddPCR method is far more reliable and simpler to use than semiquantitative PCR to analyse skewed or faint allelic expression of imprinted genes.

Published

2021

2. Differentiating molecular etiologies of Angelman syndrome through facial phenotyping using deep learning.

Author

Gomez DA, Bird LM, Fleischer N, and Abdul-Rahman OA

Subjects

Adolescent, Adult, Angelman Syndrome classification, Angelman Syndrome diagnosis, Angelman Syndrome pathology, Child, Child, Preschool, Face pathology, Female, Humans, Infant, Male, Maternal Inheritance genetics, Phenotype, Ubiquitin-Protein Ligases genetics, Uniparental Disomy diagnosis, Uniparental Disomy pathology, Young Adult, Angelman Syndrome genetics, Deep Learning, Genomic Imprinting genetics, Uniparental Disomy genetics

Abstract

Angelman syndrome (AS) is caused by several genetic mechanisms that impair the expression of maternally-inherited UBE3A through deletions, paternal uniparental disomy (UPD), UBE3A pathogenic variants, or imprinting defects. Current methods of differentiating the etiology require molecular testing, which is sometimes difficult to obtain. Recently, computer-based facial analysis systems have been used to assist in identifying genetic conditions based on facial phenotypes. We sought to understand if the facial-recognition system DeepGestalt could find differences in phenotype between molecular subtypes of AS. Images and molecular data on 261 individuals with AS ranging from 10 months through 32 years were analyzed by DeepGestalt in a cross-validation model with receiver operating characteristic (ROC) curves generated. The area under the curve (AUC) of the ROC for each molecular subtype was compared and ranked from least to greatest differentiable phenotype. We determined that DeepGestalt demonstrated a high degree of discrimination between the deletion subtype and UPD or imprinting defects, and a lower degree of discrimination with the UBE3A pathogenic variants subtype. Our findings suggest that DeepGestalt can recognize subclinical differences in phenotype based on etiology and may provide decision support for testing., (© 2020 Wiley Periodicals, Inc.)

Published

2020

3. Nutrition Assessment and Intervention in a Pediatric Patient with Angelman Syndrome: A Case Presentation Highlighting Clinical Challenges and Evidence-Based Solutions.

Author

Fisher K, Keng J, and Ziegler J

Subjects

Algorithms, Anthropometry, Child, Child Nutritional Physiological Phenomena, Evidence-Based Medicine, Female, Gene Deletion, Genetic Association Studies, Humans, Nutrition Surveys, Pediatrics, Angelman Syndrome diet therapy, Angelman Syndrome genetics, Genomic Imprinting, Nutrition Assessment

Abstract

Background: Angelman syndrome (AS) is a rare disorder of genetic imprinting which results in intellectual and developmental disability. It meets criteria of a disorder of neurologic impairment. A deletion in the long arm of chromosome 15 (del 15q11.2-q13) is responsible for about 70% of cases of AS (deletion genotype)., Summary: There is a paucity of evidence to allow algorithmic nutrition assessment and intervention in pediatric patients with AS. Therefore, our objective is to use a case presentation to provide an example of nutrition assessment and intervention in a pediatric patient with the deletion genotype of AS and then highlight common challenges to providing evidenced-based nutrition care. For the highlighted challenges, we suggest evidence-based solutions to provide a resource for clinicians who may encounter similar challenges in clinical practice. Key Messages: There are genotype-phenotype correlations in AS that can help guide clinicians regarding nutritionally relevant clinical characteristics and corresponding interventions that are patient specific. The deletion genotype in AS is associated with multiple characteristics that are relevant to nutrition care and may also be different and/or more severe than characteristics seen in other AS genetic mechanisms. There is also overlap in certain nutritionally relevant clinical characteristics between AS and other conditions, including Prader-Willi syndrome, autism spectrum disorders, and disorders of neurological impairment like cerebral palsy. Clinicians can utilize nutrition resources related to these conditions to expand the scope of relevant resources available., (© 2019 The Author(s) Published by S. Karger AG, Basel.)

Published

2020

4. Genetic variation of UBE3A is associated with schizotypy in a population of typical individuals.

Author

Salminen I, Read S, Hurd P, and Crespi B

Subjects

Angelman Syndrome genetics, Autistic Disorder genetics, Chromosomes, Human, Pair 15 genetics, Female, Gene Dosage, Genotype, Humans, Male, Phenotype, Polymorphism, Single Nucleotide, Prader-Willi Syndrome genetics, Genomic Imprinting, Maternal Inheritance, Psychotic Disorders genetics, Schizotypal Personality Disorder genetics, Ubiquitin-Protein Ligases genetics

Abstract

The maternally expressed imprinted gene UBE3A has been implicated in autism, schizophrenia and psychosis. The phenotype of Angelman syndrome, caused by loss of UBE3A expression, involves autism spectrum traits, while Prader-Willi syndrome, where the genotype of maternal disomy increases dosage of UBE3A, shows high penetrance for the development of psychosis. Maternal duplications of the 15q11-q13 chromosome region that overlap the imprinted region also show an association with schizophrenia, further implying a connection between increased dosage of UBE3A and the development of schizophrenia and psychosis. We phenotyped a large population of typical individuals for autism spectrum and schizotypal traits and genotyped them for a set of SNPs in UBE3A. Genetic variation of rs732739, an intronic SNP tagging a large haplotype spanning nearly the entire range of UBE3A, was significantly associated with variation in total schizotypy. Our results provide an independent line of evidence, connecting the imprinted UBE3A gene to the schizophrenia spectrum., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

5. A bipartite boundary element restricts UBE3A imprinting to mature neurons.

Author

Hsiao JS, Germain ND, Wilderman A, Stoddard C, Wojenski LA, Villafano GJ, Core L, Cotney J, and Chamberlain SJ

Subjects

Angelman Syndrome genetics, Binding Sites, Chromatin metabolism, Epistasis, Genetic, Exons, Gene Expression, Gene Expression Regulation, Induced Pluripotent Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Protein Binding, RNA, Antisense, RNA, Long Noncoding, Sequence Deletion, Chromatin genetics, Genomic Imprinting, Neurons metabolism, Ubiquitin-Protein Ligases genetics

Abstract

Angelman syndrome (AS) is a severe neurodevelopmental disorder caused by the loss of function from the maternal allele of UBE3A , a gene encoding an E3 ubiquitin ligase. UBE3A is only expressed from the maternally inherited allele in mature human neurons due to tissue-specific genomic imprinting. Imprinted expression of UBE3A is restricted to neurons by expression of UBE3A antisense transcript ( UBE3A-ATS ) from the paternally inherited allele, which silences the paternal allele of UBE3A in cis However, the mechanism restricting UBE3A-ATS expression and UBE3A imprinting to neurons is not understood. We used CRISPR/Cas9-mediated genome editing to functionally define a bipartite boundary element critical for neuron-specific expression of UBE3A-ATS in humans. Removal of this element led to up-regulation of UBE3A-ATS without repressing paternal UBE3A However, increasing expression of UBE3A-ATS in the absence of the boundary element resulted in full repression of paternal UBE3A , demonstrating that UBE3A imprinting requires both the loss of function from the boundary element as well as the up-regulation of UBE3A-ATS These results suggest that manipulation of the competition between UBE3A-ATS and UBE3A may provide a potential therapeutic approach for AS., Competing Interests: The authors declare no conflict of interest.

Published

2019

6. Comprehensive meta-analysis reveals association between multiple imprinting disorders and conception by assisted reproductive technology.

Author

Cortessis VK, Azadian M, Buxbaum J, Sanogo F, Song AY, Sriprasert I, Wei PC, Yu J, Chung K, and Siegmund KD

Subjects

Female, Humans, Risk Factors, Chromosome Disorders etiology, Fertilization, Genomic Imprinting, Reproductive Techniques, Assisted adverse effects

Abstract

Purpose: To determine whether a history of conception by assisted reproductive technology (ART) is associated with occurrence of one or more imprinting disorders of either maternal or paternal origin., Methods: We implemented a systematic review of scholarly literature followed by comprehensive meta-analysis to quantitatively synthesize data from reports relating to use of ART to occurrence of any imprinting disorder of humans, including Beckwith-Wiedemann (BWS), Angelman (AS), Prader-Willi (PWS), and Silver-Russell (SRS) syndromes, as well as transient neonatal diabetes mellitus (TNDB) and sporadic retinoblasoma (RB)., Results: The systematic review identified 13 reports presenting unique data from 23 studies that related conception following ART to occurrence of imprinting disorders. Multiple studies of four disorder were identified, for which meta-analysis yielded the following summary estimates of associations with a history of ART: AS, summary odds ratio (sOR) = 4.7 (95% confidence interval (CI) 2.6-8.5, 4 studies); BWS, sOR = 5.8 (95% CI 3.1-11.1, 8 studies); PWS, sOR = 2.2 (95% CI 1.6-3.0, 6 studies); SRS, sOR = 11.3 (95% CI 4.5-28.5, 3 studies). Only one study reported on each of TNDB and RB., Conclusion: Published data reveal positive associations between history of ART conception and each of four imprinting disorders. Reasons for these associations warrant further investigation.

Published

2018

7. Detection of a case of Angelman syndrome caused by an imprinting error in 949 pregnancies analyzed for AS following IVF.

Author

Johnson JP, Schoof J, Beischel L, Schwancke C, Goldberg J, Black L, Ross L, and Bhatt S

Subjects

Adult, Angelman Syndrome genetics, Angelman Syndrome pathology, Female, Humans, Prader-Willi Syndrome diagnosis, Prader-Willi Syndrome genetics, Prader-Willi Syndrome pathology, Pregnancy, Angelman Syndrome diagnosis, Fertilization in Vitro trends, Genomic Imprinting genetics, Prenatal Diagnosis

Published

2018

8. Genomic imprinting does not reduce the dosage of UBE3A in neurons.

Author

Hillman PR, Christian SGB, Doan R, Cohen ND, Konganti K, Douglas K, Wang X, Samollow PB, and Dindot SV

Subjects

Alleles, Animals, Female, Gene Expression Regulation, Mice, Neurogenesis genetics, Neurons metabolism, RNA, Antisense genetics, Ubiquitin-Protein Ligases biosynthesis, Gene Dosage genetics, Genomic Imprinting, Maternal Inheritance genetics, Ubiquitin-Protein Ligases genetics

Abstract

Background: The ubiquitin protein E3A ligase gene ( UBE3A ) gene is imprinted with maternal-specific expression in neurons and biallelically expressed in all other cell types. Both loss-of-function and gain-of-function mutations affecting the dosage of UBE3A are associated with several neurodevelopmental syndromes and psychological conditions, suggesting that UBE3A is dosage-sensitive in the brain. The observation that loss of imprinting increases the dosage of UBE3A in brain further suggests that inactivation of the paternal UBE3A allele evolved as a dosage-regulating mechanism. To test this hypothesis, we examined UBE3A transcript and protein levels among cells, tissues, and species with different imprinting states of UBE3A ., Results: Overall, we found no correlation between the imprinting status and dosage of UBE3A. Importantly, we found that maternal Ube3a protein levels increase in step with decreasing paternal Ube3a protein levels during neurogenesis in mouse, fully compensating for loss of expression of the paternal Ube3a allele in neurons., Conclusions: Based on our findings, we propose that imprinting of UBE3A does not function to reduce the dosage of UBE3A in neurons but rather to regulate some other, as yet unknown, aspect of gene expression or protein function.

Published

2017

9. Atypical Angelman syndrome due to a mosaic imprinting defect: Case reports and review of the literature.

Author

Le Fevre A, Beygo J, Silveira C, Kamien B, Clayton-Smith J, Colley A, Buiting K, and Dudding-Byth T

Subjects

Adolescent, Child, Chromosome Mapping, DNA Methylation, Facies, Female, Genetic Association Studies, Genetic Heterogeneity, Humans, Incidence, Male, snRNP Core Proteins genetics, Angelman Syndrome diagnosis, Angelman Syndrome genetics, Genomic Imprinting, Mosaicism, Phenotype

Abstract

Angelman syndrome (AS) is characterized by severe intellectual disability, limited, or absent speech and a generally happy demeanor. The four known etiological mechanisms; deletions, uniparental disomy, imprinting defects, and UBE3A mutation all affect expression of the UBE3A gene at 15q11-q13. An atypical phenotype is seen in individuals who are mosaic for a chromosome 15q11-q13 imprinting defect on the maternal allele. These patients present with a milder phenotype, often with hyperphagia and obesity or non-specific intellectual disability. Unlike typical AS syndrome, they can have a vocabulary up to 100 words and speak in sentences. Ataxia and seizures may not be present, and the majority of individuals do not have microcephaly. Here we review the current literature and present three individuals with atypical AS caused by a mosaic imprinting defect to demonstrate why DNA methylation analysis at the SNRPN locus needs to be considered in a broader clinical context. © 2017 Wiley Periodicals, Inc., (© 2017 Wiley Periodicals, Inc.)

Published

2017

10. Epigenetic regulation of UBE3A and roles in human neurodevelopmental disorders.

Author

LaSalle JM, Reiter LT, and Chamberlain SJ

Subjects

Angelman Syndrome metabolism, Angelman Syndrome pathology, Cell Nucleus metabolism, Chromosomes, Human, Pair 15 genetics, Chromosomes, Human, Pair 15 metabolism, Female, Humans, Male, Neurons metabolism, Neurons pathology, Proteasome Endopeptidase Complex metabolism, Protein Stability, Proteolysis, Synapses metabolism, Synapses pathology, Transcription, Genetic, Trisomy pathology, Ubiquitin genetics, Ubiquitin metabolism, Ubiquitin-Protein Ligases metabolism, Angelman Syndrome genetics, Epigenesis, Genetic, Genomic Imprinting, Trisomy genetics, Ubiquitin-Protein Ligases genetics

Abstract

The E3 ubiquitin ligase UBE3A, also known as E6-AP, has a multitude of ascribed functions and targets relevant to human health and disease. Epigenetic regulation of the UBE3A gene by parentally imprinted noncoding transcription within human chromosome 15q11.2-q13.3 is responsible for the maternal-specific effects of 15q11.2-q13.3 deletion or duplication disorders. Here, we review the evidence for diverse and emerging roles for UBE3A in the proteasome, synapse and nucleus in regulating protein stability and transcription as well as the current mechanistic understanding of UBE3A imprinting in neurons. Angelman and Dup15q syndromes as well as experimental models of these neurodevelopmental disorders are highlighted as improving understanding of UBE3A and its complex regulation for improving therapeutic strategies., Competing Interests: Financial & competing interests disclosure The authors thank the NIH NINDS (R01NS076263) and the Prader–Willi Research Foundation for ongoing support of research in this area. The authors have no other relevant affiliations or financial involvement with any organization or entity with a financial interest in or financial conflict with the subject matter or materials discussed in the manuscript apart from those disclosed. No writing assistance was utilized in the production of this manuscript.

Published

2015

11. Mild Angelman syndrome phenotype due to a mosaic methylation imprinting defect.

Author

Fairbrother LC, Cytrynbaum C, Boutis P, Buiting K, Weksberg R, and Williams C

Subjects

Child, Preschool, Electroencephalography, Female, Humans, Ubiquitin-Protein Ligases genetics, Angelman Syndrome genetics, Angelman Syndrome pathology, Chromosomes, Human, Pair 15 genetics, DNA Methylation genetics, Genomic Imprinting genetics, Phenotype, Ubiquitin-Protein Ligases metabolism

Abstract

Angelman syndrome (AS) is a neurogenetic disorder causing severe to profound intellectual disability, absent or very limited speech and a high risk for seizures. AS is caused by a loss of function of the maternally-derived UBE3A allele due to one of several mechanisms including imprinting defects (ImpDs). We present a girl with AS due to a mosaic ImpD who has relatively high developmental function (VABS-II composite score of 76) and communication skills (as demonstrated in supplemental video links). Given the patient's relatively mild developmental impairment, without clinical evidence of seizures, gait disturbance or inappropriate laughter, the diagnosis of AS was not initially suspected. Initial laboratory testing for AS was inconclusive but additional studies suggested mosaic ImpD and characteristic EEG findings provided further support for the clinical diagnosis. Our patient, along with other case reports of children with AS and relatively mild phenotypes, raises the question as to whether there exists an undiagnosed group of individuals with mild intellectual disability and expressive speech delays due to mosaic methylation defects of the chromosome 15q11.2-13 region. Population studies may be needed to determine if such an undiagnosed group exists., (© 2015 Wiley Periodicals, Inc.)

Published

2015

12. Angelman syndrome imprinting center encodes a transcriptional promoter.

Author

Lewis MW, Brant JO, Kramer JM, Moss JI, Yang TP, Hansen PJ, Williams RS, and Resnick JL

Subjects

Animals, Cattle, DNA Methylation, DNA Primers genetics, Gene Components, Humans, Oocytes metabolism, Promoter Regions, Genetic genetics, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, RNA, Species Specificity, snRNP Core Proteins genetics, snRNP Core Proteins metabolism, Angelman Syndrome genetics, Gene Expression Regulation genetics, Genomic Imprinting genetics, Models, Biological, Prader-Willi Syndrome genetics

Abstract

Clusters of imprinted genes are often controlled by an imprinting center that is necessary for allele-specific gene expression and to reprogram parent-of-origin information between generations. An imprinted domain at 15q11-q13 is responsible for both Angelman syndrome (AS) and Prader-Willi syndrome (PWS), two clinically distinct neurodevelopmental disorders. Angelman syndrome arises from the lack of maternal contribution from the locus, whereas Prader-Willi syndrome results from the absence of paternally expressed genes. In some rare cases of PWS and AS, small deletions may lead to incorrect parent-of-origin allele identity. DNA sequences common to these deletions define a bipartite imprinting center for the AS-PWS locus. The PWS-smallest region of deletion overlap (SRO) element of the imprinting center activates expression of genes from the paternal allele. The AS-SRO element generates maternal allele identity by epigenetically inactivating the PWS-SRO in oocytes so that paternal genes are silenced on the future maternal allele. Here we have investigated functional activities of the AS-SRO, the element necessary for maternal allele identity. We find that, in humans, the AS-SRO is an oocyte-specific promoter that generates transcripts that transit the PWS-SRO. Similar upstream promoters were detected in bovine oocytes. This result is consistent with a model in which imprinting centers become DNA methylated and acquire maternal allele identity in oocytes in response to transiting transcription.

Published

2015

13. Increased body mass in infancy and early toddlerhood in Angelman syndrome patients with uniparental disomy and imprinting center defects.

Author

Brennan ML, Adam MP, Seaver LH, Myers A, Schelley S, Zadeh N, Hudgins L, and Bernstein JA

Subjects

Cephalometry, Child, Female, Humans, Infant, Male, Angelman Syndrome genetics, Angelman Syndrome pathology, Body Weight, Genomic Imprinting, Uniparental Disomy genetics, Uniparental Disomy pathology

Abstract

The diagnosis of Angelman syndrome (AS) is based on clinical features and genetic testing. Developmental delay, severe speech impairment, ataxia, atypical behavior and microcephaly by two years of age are typical. Feeding difficulties in young infants and obesity in late childhood can also be seen. The NIH Angelman-Rett-Prader-Willi Consortium and others have documented genotype-phenotype associations including an increased body mass index in children with uniparental disomy (UPD) or imprinting center (IC) defects. We recently encountered four cases of infantile obesity in non-deletion AS cases, and therefore examined body mass measures in a cohort of non-deletion AS cases. We report on 16 infants and toddlers (ages 6 to 44 months; 6 female, and 10 male) with severe developmental delay. Birth weights were appropriate for gestational age in most cases, >97th% in one case and not available in four cases. The molecular subclass case distribution consisted of: UPD (n = 2), IC defect (n = 3), UPD or IC defect (n = 3), and UBE3A mutation (n = 8). Almost all (7 out of 8) UPD, IC and UPD/IC cases went on to exhibit >90th% age- and gender-appropriate weight for height or BMI within the first 44 months. In contrast, no UBE3A mutation cases exhibited obesity or pre-obesity measures (percentiles ranged from <3% to 55%). These findings demonstrate that increased body mass may be evident as early as the first year of life and highlight the utility of considering the diagnosis of AS in the obese infant or toddler with developmental delay, especially when severe. Although a mechanism explaining the association of UPD, and IC defects with obesity has not been identified, recognition of this correlation may inform investigation of imprinting at the PWS/AS locus and obesity., (© 2014 Wiley Periodicals, Inc.)

Published

2015

14. Influence of the Prader-Willi syndrome imprinting center on the DNA methylation landscape in the mouse brain.

Author

Brant JO, Riva A, Resnick JL, and Yang TP

Subjects

Angelman Syndrome genetics, Animals, Antigens, Neoplasm genetics, Carrier Proteins genetics, CpG Islands, Female, High-Throughput Nucleotide Sequencing, Male, Mice, Inbred C57BL, Mice, Mutant Strains, Neoplasm Proteins genetics, Promoter Regions, Genetic, Proteins genetics, Ribonucleoproteins genetics, Sequence Deletion, Ubiquitin-Protein Ligases, Brain physiology, DNA Methylation, Genomic Imprinting, Prader-Willi Syndrome genetics

Abstract

Reduced representation bisulfite sequencing (RRBS) was used to analyze DNA methylation patterns across the mouse brain genome in mice carrying a deletion of the Prader-Willi syndrome imprinting center (PWS-IC) on either the maternally- or paternally-inherited chromosome. Within the ~3.7 Mb imprinted Angelman/Prader-Willi syndrome (AS/PWS) domain, 254 CpG sites were interrogated for changes in methylation due to PWS-IC deletion. Paternally-inherited deletion of the PWS-IC increased methylation levels ~2-fold at each CpG site (compared to wild-type controls) at differentially methylated regions (DMRs) associated with 5' CpG island promoters of paternally-expressed genes; these methylation changes extended, to a variable degree, into the adjacent CpG island shores. Maternal PWS-IC deletion yielded little or no changes in methylation at these DMRs, and methylation of CpG sites outside of promoter DMRs also was unchanged upon maternal or paternal PWS-IC deletion. Using stringent ascertainment criteria, ~750,000 additional CpG sites were also interrogated across the entire mouse genome. This analysis identified 26 loci outside of the imprinted AS/PWS domain showing altered DNA methylation levels of ≥25% upon PWS-IC deletion. Curiously, altered methylation at 9 of these loci was a consequence of maternal PWS-IC deletion (maternal PWS-IC deletion by itself is not known to be associated with a phenotype in either humans or mice), and 10 of these loci exhibited the same changes in methylation irrespective of the parental origin of the PWS-IC deletion. These results suggest that the PWS-IC may affect DNA methylation at these loci by directly interacting with them, or may affect methylation at these loci through indirect downstream effects due to PWS-IC deletion. They further suggest the PWS-IC may have a previously uncharacterized function outside of the imprinted AS/PWS domain.

Published

2014

15. Targeted methylation testing of a patient cohort broadens the epigenetic and clinical description of imprinting disorders.

Author

Poole RL, Docherty LE, Al Sayegh A, Caliebe A, Turner C, Baple E, Wakeling E, Harrison L, Lehmann A, Temple IK, and Mackay DJ

Subjects

Cohort Studies, Genetic Heterogeneity, Genetic Loci, Genetic Testing, Humans, Phenotype, DNA Methylation, Epigenomics methods, Genetic Diseases, Inborn diagnosis, Genetic Diseases, Inborn genetics, Genomic Imprinting

Abstract

Imprinting disorders are associated with mutations and epimutations affecting imprinted genes, that is those whose expression is restricted by parent of origin. Their diagnosis is challenging for two reasons: firstly, their clinical features, particularly prenatal and postnatal growth disturbance, are heterogeneous and partially overlapping; secondly, their underlying molecular defects include mutation, epimutation, copy number variation, and chromosomal errors, and can be further complicated by somatic mosaicism and multi-locus methylation defects. It is currently unclear to what extent the observed phenotypic heterogeneity reflects the underlying molecular pathophysiology; in particular, the molecular and clinical diversity of multilocus methylation defects remains uncertain. To address these issues we performed comprehensive methylation analysis of imprinted genes in a research cohort of 285 patients with clinical features of imprinting disorders, with or without a positive molecular diagnosis. 20 of 91 patients (22%) with diagnosed epimutations had methylation defects of additional imprinted loci, and the frequency of developmental delay and congenital anomalies was higher among these patients than those with isolated epimutations, indicating that hypomethylation of multiple imprinted loci is associated with increased diversity of clinical presentation. Among 194 patients with clinical features of an imprinting disorder but no molecular diagnosis, we found 15 (8%) with methylation anomalies, including missed and unexpected molecular diagnoses. These observations broaden the phenotypic and epigenetic definitions of imprinting disorders, and show the importance of comprehensive molecular testing for patient diagnosis and management., (Copyright © 2013 Wiley Periodicals, Inc.)

Published

2013

16. Integration of CTCF loops, methylome, and transcriptome in differentiating LUHMES as a model for imprinting dynamics of the 15q11-q13 locus in human neurons

Author

Fugón, Orangel J Gutierrez, Sharifi, Osman, Heath, Nicholas, Soto, Daniela C, Gomez, J Antonio, Yasui, Dag H, Mendiola, Aron Judd P, O’Geen, Henriette, Beitnere, Ulrika, Tomkova, Marketa, Haghani, Viktoria, Dillon, Greg, Segal, David J, and LaSalle, Janine M

Subjects

Biological Sciences, Genetics, Stem Cell Research - Induced Pluripotent Stem Cell, Human Genome, Rare Diseases, Stem Cell Research, Pediatric, Neurosciences, Intellectual and Developmental Disabilities (IDD), Brain Disorders, 1.1 Normal biological development and functioning, Generic health relevance, Humans, Genomic Imprinting, CCCTC-Binding Factor, Chromosomes, Human, Pair 15, Neurons, DNA Methylation, Transcriptome, Ubiquitin-Protein Ligases, Cell Differentiation, Angelman Syndrome, RNA, Long Noncoding, Prader-Willi Syndrome, snRNP Core Proteins, Alleles, Cell Line, Epigenome, chromatin, imprinting, human cell models, Angelman, LUHMES, methylation, UBE3A, Medical and Health Sciences, Genetics & Heredity

Abstract

Human cell line models, including the neuronal precursor line LUHMES, are important for investigating developmental transcriptional dynamics within imprinted regions, particularly the 15q11-q13 Angelman (AS) and Prader-Willi (PWS) syndrome locus. AS results from loss of maternal UBE3A in neurons, where the paternal allele is silenced by a convergent antisense transcript UBE3A-ATS, a lncRNA that terminates at PWAR1 in non-neurons. qRT-PCR analysis confirmed the exclusive and progressive increase in UBE3A-ATS in differentiating LUHMES neurons, validating their use for studying UBE3A silencing. Genome-wide transcriptome analyses revealed changes to 11 834 genes during neuronal differentiation, including the upregulation of most genes within the 15q11-q13 locus. To identify dynamic changes in chromatin loops linked to transcriptional activity, we performed a HiChIP validated by 4C, which identified two neuron-specific CTCF loops between MAGEL2-SNRPN and PWAR1-UBE3A. To determine if allele-specific differentially methylated regions (DMR) may be associated with CTCF loop anchors, whole genome long-read nanopore sequencing was performed. We identified a paternally hypomethylated DMR near the SNRPN upstream loop anchor exclusive to neurons and a paternally hypermethylated DMR near the PWAR1 CTCF anchor exclusive to undifferentiated cells, consistent with increases in neuronal transcription. Additionally, DMRs near CTCF loop anchors were observed in both cell types, indicative of allele-specific differences in chromatin loops regulating imprinted transcription. These results provide an integrated view of the 15q11-q13 epigenetic landscape during LUHMES neuronal differentiation, underscoring the complex interplay of transcription, chromatin looping, and DNA methylation. They also provide insights for future therapeutic approaches for AS and PWS.

Published

2024

17. Expanding deep phenotypic spectrum associated with atypical pathogenic structural variations overlapping 15q11–q13 imprinting region.

Author

Mim, Rabeya Akter, Soorajkumar, Anjana, Kosaji, Noor, Rahman, Muhammad Mizanur, Sarker, Shaoli, Karuvantevida, Noushad, Eshaque, Tamannyat Binte, Rahaman, Md Atikur, Islam, Amirul, Chowdhury, Mohammod Shah Jahan, Shams, Nusrat, Uddin, K. M. Furkan, Akter, Hosneara, and Uddin, Mohammed

Subjects

*GENOMIC imprinting, *PRADER-Willi syndrome, *GENE expression, *PHENOTYPES, *GENETIC variation, *BRUGADA syndrome

Abstract

Background: The 15q11–q13 region is a genetic locus with genes subject to genomic imprinting, significantly influencing neurodevelopment. Genomic imprinting is an epigenetic phenomenon that causes differential gene expression based on the parent of origin. In most diploid organisms, gene expression typically involves an equal contribution from both maternal and paternal alleles, shaping the phenotype. Nevertheless, in mammals, including humans, mice, and marsupials, the functional equivalence of parental alleles is not universally maintained. Notably, during male and female gametogenesis, parental alleles may undergo differential marking or imprinting, thereby modifying gene expression without altering the underlying DNA sequence. Neurodevelopmental disorders, such as Prader–Willi syndrome (PWS) (resulting from the absence of paternally expressed genes in this region), Angelman syndrome (AS) (associated with the absence of the maternally expressed UBE3A gene), and 15q11–q13 duplication syndrome (resulting from the two common forms of duplications—either an extra isodicentric 15 chromosome or an interstitial 15 duplication), are the outcomes of genetic variations in this imprinting region. Methods: Conducted a genomic study to identify the frequency of pathogenic variants impacting the 15q11–q13 region in an ethnically homogenous population from Bangladesh. Screened all known disorders from the DECIPHER database and identified variant enrichment within this cohort. Using the Horizon analysis platform, performed enrichment analysis, requiring at least >60% overlap between a copy number variation and a disorder breakpoint. Deep clinical phenotyping was carried out through multiple examination sessions to evaluate a range of clinical symptoms. Results: This study included eight individuals with clinically suspected PWS/AS, all previously confirmed through chromosomal microarray analysis, which revealed chromosomal breakpoints within the 15q11–q13 region. Among this cohort, six cases (75%) exhibited variable lengths of deletions, whereas two cases (25%) showed duplications. These included one type 2 duplication, one larger atypical duplication, one shorter type 2 deletion, one larger type 1 deletion, and four cases with atypical deletions. Furthermore, thorough clinical assessments led to the diagnosis of four PWS patients, two AS patients, and two individuals with 15q11–q13 duplication syndrome. Conclusion: Our deep phenotypic observations identified a spectrum of clinical features that overlap and are unique to PWS, AS, and Dup15q syndromes. Our findings establish genotype–phenotype correlation for patients impacted by variable structural variations within the 15q11–q13 region. [ABSTRACT FROM AUTHOR]

Published

2024

18. Angelman syndrome genotypes manifest varying degrees of clinical severity and developmental impairment

Author

Keute, Marius, Miller, Meghan T, Krishnan, Michelle L, Sadhwani, Anjali, Chamberlain, Stormy, Thibert, Ronald L, Tan, Wen-Hann, Bird, Lynne M, and Hipp, Joerg F

Subjects

Biomedical and Clinical Sciences, Clinical Sciences, Brain Disorders, Neurosciences, Behavioral and Social Science, Clinical Research, Pediatric, Rare Diseases, Intellectual and Developmental Disabilities (IDD), Human Genome, Mental Health, Genetics, Aetiology, 2.1 Biological and endogenous factors, Mental health, Angelman Syndrome, Chromosomes, Human, Pair 15, Genomic Imprinting, Genotype, Humans, Phenotype, Ubiquitin-Protein Ligases, Biological Sciences, Medical and Health Sciences, Psychology and Cognitive Sciences, Psychiatry, Clinical sciences, Biological psychology, Clinical and health psychology

Abstract

Angelman Syndrome (AS) is a severe neurodevelopmental disorder due to impaired expression of UBE3A in neurons. There are several genetic mechanisms that impair UBE3A expression, but they differ in how neighboring genes on chromosome 15 at 15q11-q13 are affected. There is evidence that different genetic subtypes present with different clinical severity, but a systematic quantitative investigation is lacking. Here we analyze natural history data on a large sample of individuals with AS (n = 250, 848 assessments), including clinical scales that quantify development of motor, cognitive, and language skills (Bayley Scales of Infant Development, Third Edition; Preschool Language Scale, Fourth Edition), adaptive behavior (Vineland Adaptive Behavioral Scales, Second Edition), and AS-specific symptoms (AS Clinical Severity Scale). We found that clinical severity, as captured by these scales, differs between genetic subtypes: individuals with UBE3A pathogenic variants and imprinting defects (IPD) are less affected than individuals with uniparental paternal disomy (UPD); of those with UBE3A pathogenic variants, individuals with truncating mutations are more impaired than those with missense mutations. Individuals with a deletion that encompasses UBE3A and other genes are most impaired, but in contrast to previous work, we found little evidence for an influence of deletion length (class I vs. II) on severity of manifestations. The results of this systematic analysis highlight the relevance of genomic regions beyond UBE3A as contributing factors in the AS phenotype, and provide important information for the development of new therapies for AS. More generally, this work exemplifies how increasing genetic irregularities are reflected in clinical severity.

Published

2021

19. Prader-Willi and Angelman Syndromes: Mechanisms and Management.

Author

Ma, Van K, Mao, Rong, Toth, Jessica N, Fulmer, Makenzie L, Egense, Alena S, and Shankar, Suma P

Subjects

PRADER-Willi syndrome, ANGELMAN syndrome, GENOMIC imprinting, INDIVIDUALIZED education programs, SCHOOL children

Abstract

Prader-Willi syndrome (PWS) and Angelman syndrome (AS) are genetic imprinting disorders resulting from absent or reduced expression of paternal or maternal genes in chromosome 15q11q13 region, respectively. The most common etiology is deletion of the maternal or paternal 15q11q13 region. Methylation is the first line for molecular diagnostic testing; MS-MLPA is the most sensitive test. The molecular subtype of PWS/AS provides more accurate recurrence risk information for parents and for the individual affected with the condition. Management should include a multidisciplinary team by various medical subspecialists and therapists. Developmental and behavioral management of PWS and AS in infancy and early childhood includes early intervention services and individualized education programs for school-aged children. Here, we compare and discuss the mechanisms, pathophysiology, clinical features, and management of the two imprinting disorders, PWS and AS. [ABSTRACT FROM AUTHOR]

Published

2023

20. Imprinting effects of UBE3A loss on synaptic gene networks and Wnt signaling pathways

Author

Lopez, S Jesse, Laufer, Benjamin I, Beitnere, Ulrika, Berg, Elizabeth L, Silverman, Jill L, O’Geen, Henriette, Segal, David J, and LaSalle, Janine M

Subjects

Biological Sciences, Bioinformatics and Computational Biology, Genetics, Rare Diseases, Neurosciences, Human Genome, Biotechnology, Intellectual and Developmental Disabilities (IDD), Brain Disorders, Pediatric, Reproductive health and childbirth, Neurological, Angelman Syndrome, Animals, Brain, Cerebral Cortex, Epigenesis, Genetic, Female, Gene Expression, Gene Expression Profiling, Gene Regulatory Networks, Genomic Imprinting, Hypothalamus, Neuroglia, Neurons, Rats, Rats, Sprague-Dawley, Synapses, Systems Biology, Transcriptome, Ubiquitin-Protein Ligases, Wnt Signaling Pathway, Medical and Health Sciences, Genetics & Heredity

Abstract

Ubiquitin E3 ligase 3A (UBE3A) encodes an E3 ubiquitin ligase whose loss from the maternal allele causes the neurodevelopmental disorder Angelman syndrome (AS). Previous studies of UBE3A function have not examined full Ube3a deletion in mouse, the complexity of imprinted gene networks in brain nor the molecular basis of systems-level cognitive dysfunctions in AS. We therefore utilized a systems biology approach to elucidate how UBE3A loss impacts the early postnatal brain in a novel CRISPR/Cas9-engineered rat Angelman model of a complete Ube3a deletion. Strand-specific transcriptome analysis of offspring from maternally or paternally inherited Ube3a deletions revealed the expected parental expression patterns of Ube3a sense and antisense transcripts by postnatal day 2 (P2) in hypothalamus and day 9 (P9) in cortex, compared to wild-type littermates. The dependency of genome-wide effects on parent-of-origin, Ube3a genotype and time (P2 and P9) was investigated through transcriptome (RNA sequencing of cortex and hypothalamus) and methylome (whole-genome bisulfite sequencing of hypothalamus). Weighted gene co-expression and co-methylation network analyses identified co-regulated networks in maternally inherited Ube3a deletion offspring enriched in postnatal developmental processes including Wnt signaling, synaptic regulation, neuronal and glial functions, epigenetic regulation, ubiquitin, circadian entrainment and splicing. Furthermore, we showed that loss of the paternal Ube3a antisense transcript resulted in both unique and overlapping dysregulated gene pathways with maternal loss, predominantly at the level of differential methylation. Together, these results provide a holistic examination of the molecular impacts of UBE3A loss in brain, supporting the existence of interactive epigenetic networks between maternal and paternal transcripts at the Ube3a locus.

Published

2019

21. Multiscale spatio-temporal dynamics of UBE3A gene in brain physiology and neurodevelopmental disorders.

Author

Biagioni, Martina, Baronchelli, Federica, and Fossati, Matteo

Subjects

*GENOMIC imprinting, *BRAIN physiology, *ANGELMAN syndrome, *NEURAL development, *RESEARCH questions

Abstract

The UBE3A gene, located in the chromosomal region 15q11-13, is subject to neuron-specific genomic imprinting and it plays a critical role in brain development. Genetic defects of UBE3A cause severe neurodevelopmental disorders, namely the Angelman syndrome (AS) and the 15q11.2-q13.3 duplication syndrome (Dup15q). In the last two decades, the development of in vitro and in vivo models of AS and Dup15q were fundamental to improve the understanding of UBE3A function in the brain. However, the pathogenic mechanisms of these diseases remain elusive and effective treatments are lacking. Recent evidence suggests that UBE3A functions are both spatially and temporally specific, varying across subcellular compartments, brain regions, and neuronal circuits. In the present review, we summarize current knowledge on the role of UBE3A in neuronal pathophysiology under this spatio-temporal perspective. Additionally, we propose key research questions that will be instrumental to better understand the pathogenic mechanisms underpinning AS and Dup15q disorders and provide the rationale to develop novel therapies. • Genetic defects of the imprinted gene UBE3A cause neurodevelopmental disorders. • UBE3A critically regulate the function of distinct neuronal circuits and behaviors. • The molecular diversity of UBE3A is a key determinant of disease pathophysiology. • UBE3A operates during precise temporal windows to regulate neurodevelopment. [ABSTRACT FROM AUTHOR]

Published

2024

22. IPSC Models of Chromosome 15Q Imprinting Disorders: From Disease Modeling to Therapeutic Strategies

Author

Germain, Noelle D., Levine, Eric S., Chamberlain, Stormy J., Schousboe, Arne, Series Editor, DiCicco-Bloom, Emanuel, editor, and Millonig, James H., editor

Published

2020

23. Imprinted Genes and Hypothalamic Function

Author

Pulix, Michela, Plagge, Antonius, Russell, John A., Series Editor, Armstrong, William E., Series Editor, Wray, Susan, editor, and Blackshaw, Seth, editor

Published

2020

24. Imprinting analysis by droplet digital PCR coupled with locked nucleic acid TaqMan probes

Author

Maiko Mitake, Shiori Hirano, and Tatsuya Kishino

Subjects

genomic imprinting, droplet digital pcr, locked nucleic acid, taqman probe, ube3a gene, angelman syndrome, Genetics, QH426-470

Abstract

Imprinted genes are differentially expressed in a parent-of-origin-specific manner. Parental origin of the alleles is discriminated by intragenic DNA polymorphisms. Comparisons of parental allelic expression have been analysed by semiquantitative RT-PCR. Here, we developed a novel quantitative method for allelic expression of the imprinted gene Ube3a, which inactivation and mutations cause Angelman syndrome and predominantly expressed by the maternal allele in neuronal tissues. In this method, cDNA was amplified by droplet digital PCR (ddPCR) coupled with allele-specific locked nucleic acid (LNA) TaqMan probes, which labelled by FAM and HEX were designed to detect the SNPs in the target regions. ddPCR assay demonstrated that the sense transcript of Ube3a was equally expressed from both parental alleles in adult tissues except neuronal tissues, where Ube3a expression from the paternal allele was about 10 to 14% of total Ube3a expression in adult brain, and 20% in spinal cord. The antisense transcript of Ube3a was expressed at 60% to 70% of the sense transcript of Ube3a in adult brain. Changes in the Ube3a transcripts during postnatal brain development were also evaluated by ddPCR. The ddPCR method is far more reliable and simpler to use than semiquantitative PCR to analyse skewed or faint allelic expression of imprinted genes.

Published

2021

25. Clinical Utility of Methylation-Specific Multiplex Ligation-Dependent Probe Amplification for the Diagnosis of Prader-Willi Syndrome and Angelman Syndrome.

Author

Boram Kim, Yongsook Park, Sung Im Cho, Man Jin Kim, Jong-Hee Chae, Ji Yeon Kim, Moon-Woo Seong, and Sung Sup Park

Subjects

PRADER-Willi syndrome, ANGELMAN syndrome, GENOMIC imprinting, POLYMERASE chain reaction, MOLECULAR probes, DIAGNOSIS, GENE amplification

Abstract

Background: Prader-Willi syndrome (PWS) and Angelman syndrome (AS) are genomic imprinting disorders that are mainly caused by a deletion on 15q11-q13, the uniparental disomy of chromosome 15, or an imprinting defect. We evaluated the utility of methylation-specific multiplex ligation-dependent probe amplification (MS-MLPA) as a diagnostic tool and for demonstrating the relationship between molecular mechanisms and clinical presentation. Methods: We performed MS-MLPA using DNA samples from 93 subjects (45 PWS, 24 AS, and 24 non-PWS/AS controls) who had previously undergone MS-PCR for the diagnosis of PWS/AS. We compared the results of both assays, and patients' clinical phenotypes were reviewed retrospectively. Results: MS-MLPA showed a 100% concordance rate with MS-PCR. Among the 45 PWS patients, 26 (57.8%) had a deletion of 15q11-q13, and the others (42.2%) had uniparental disomy 15 or an imprinting defect. Among the 24 AS patients, 16 (66.7%) had a deletion of 15q11-q13, 7 AS patients (29.2%) had uniparental disomy 15 or an imprinting defect, and one AS patient (4.2%) showed an imprinting center deletion. Conclusions: MS-MLPA has clinical utility for the diagnosis of PWS/AS, and it is superior to MS-PCR in that it can identify the molecular mechanism underlying the disease. [ABSTRACT FROM AUTHOR]

Published

2022

26. Clinical characteristics and epilepsy in genomic imprinting disorders: Angelman syndrome and Prader–Willi syndrome

Author

Tzong-Shi Wang, Wen-Hsin Tsai, Li-Ping Tsai, and Shi-Bing Wong

Subjects

angelman syndrome, epilepsy, genomic imprinting, prader–willi syndrome, Medicine

Abstract

Angelman syndrome (AS) and Prader–Willi syndrome (PWS) are considered sister imprinting disorders. Although both AS and PWS congenital neurodevelopmental disorders have chromosome 15q11.3-q13 dysfunction, their molecular mechanisms differ owing to genomic imprinting, which results in different parent-of-the-origin gene expressions. Recently, several randomized controlled trials have been proceeded to treat specific symptoms of AS and PWS. Due to the advance of clinical management, early diagnosis for patients with AS and PWS is important. PWS is induced by multiple paternal gene dysfunctions, including those in MKRN3, MAGEL2, NDN, SNURF-SNPRPN, NPAP1, and a cluster of small nucleolar RNA genes. PWS patients exhibit characteristic facial features, endocrinological, and behavioral phenotypes, including short and obese figures, hyperphagia, growth hormone deficiency, hypogonadism, autism, or obsessive–compulsive-like behaviors. In addition, hypotonia, poor feeding, failure to thrive, and typical facial features are major factors for early diagnosis of PWS. For PWS patients, epilepsy is not common and easy to treat. Conversely, AS is a single-gene disorder induced by ubiquitin-protein ligase E3A dysfunction, which only expresses from a maternal allele. AS patients develop epilepsy in their early lives and their seizures are difficult to control. The distinctive gait pattern, excessive laughter, and characteristic electroencephalography features, which contain anterior-dominated, high-voltage triphasic delta waves intermixed with epileptic spikes, result in early suspicion of AS. Often, polytherapy, including the combination of valproate, levetiracetam, lamotrigine, and benzodiazepines, is required for controlling seizures of AS patients. Notably, carbamazepine, oxcarbazepine, and vigabatrin should be avoided, since these may induce nonconvulsive status epilepticus. AS and PWS presented with distinct clinical manifestations according to specific molecular defects due to genomic imprinting. Early diagnosis and teamwork intervention, including geneticists, neurologists, rehabilitation physicians, and pulmonologists, are important. Epilepsy is common in patients with AS, and after proper treatment, seizures could be effectively controlled in late childhood or early adulthood for both AS and PWS patients.

Published

2020

27. Refining the Behavioral Phenotype of Angelman Syndrome: Examining Differences in Motivation for Social Contact Between Genetic Subgroups

Author

Mary Heald, Dawn Adams, Emily Walls, and Christopher Oliver

Subjects

Angelman syndrome, genomic imprinting, kinship theory, social behavior, operant learning, behavioral phenotype, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Abstract

Angelman syndrome (AS) is caused by loss of information from the 15q11.2-13 region on the maternal chromosome with striking phenotypic difference from Prader–Willi syndrome in which information is lost from the same region on the paternal chromosome. Motivation for social contact and sensory seeking behaviors are often noted as characteristics of the phenotype of AS and it has been argued that the strong drive for social contact supports a kinship theory interpretation of genomic imprinting. In this study we developed an experimental paradigm for quantifying the motivation for social contact in AS and examined differences across the genetic subtypes that cause AS [deletion, imprinting centre defect (ICD), uniparental disomy and UBE3A mutation]. Using single case experimental designs we examined the rate of acquisition of behavioral responses using operant learning paradigms for 21 children with AS whilst systematically varying the nature of social and sensory reinforcement. Variability in rates of acquisition was influenced by the nature of rewarding stimuli. Across the total sample both sensory stimuli and social contact could increase the rate of rewarded behavior with difference between children in the most effective reward. A striking difference in the rewarding properties of social contact across genetic subtypes was evidenced by non-deletion genetic causes of AS showing significantly higher rates of responding than the deletion cause in the social reinforcement paradigm. The results indicate that reinforcer assessment can beneficially inform behavioral interventions and that within syndrome variability in the behavioral phenotype of AS is likely driven by genetic difference. The non-deletion cause of AS, and particularly the ICD group, may be the optimal group for further study of genomic imprinting.

Published

2021

28. R-loop formation at Snord116 mediates topotecan inhibition of Ube3a-antisense and allele-specific chromatin decondensation

Author

Powell, Weston T, Coulson, Rochelle L, Gonzales, Michael L, Crary, Florence K, Wong, Spencer S, Adams, Sarrita, Ach, Robert A, Tsang, Peter, Yamada, Nazumi Alice, Yasui, Dag H, Chédin, Frédéric, and LaSalle, Janine M

Subjects

Biological Sciences, Biomedical and Clinical Sciences, Genetics, Brain Disorders, Intellectual and Developmental Disabilities (IDD), Neurosciences, Pediatric, Mental Health, Rare Diseases, Neurological, Angelman Syndrome, Animals, Chromatin, Chromatin Immunoprecipitation, Chromosomes, Human, Pair 15, Gene Expression Regulation, Gene Silencing, Genetic Loci, Genomic Imprinting, HEK293 Cells, Humans, Immunoblotting, In Situ Hybridization, Fluorescence, Locus Control Region, Mice, Mice, Knockout, Neurons, Prader-Willi Syndrome, RNA, Antisense, RNA, Small Nucleolar, Real-Time Polymerase Chain Reaction, Statistics, Nonparametric, Topotecan, Ubiquitin-Protein Ligases, snRNP Core Proteins, neurodevelopment, brain, HBII85, MBII85, snoRNA

Abstract

Prader-Willi syndrome (PWS) and Angelman syndrome (AS) are oppositely imprinted autism-spectrum disorders with known genetic bases, but complex epigenetic mechanisms underlie their pathogenesis. The PWS/AS locus on 15q11-q13 is regulated by an imprinting control region that is maternally methylated and silenced. The PWS imprinting control region is the promoter for a one megabase paternal transcript encoding the ubiquitous protein-coding Snrpn gene and multiple neuron-specific noncoding RNAs, including the PWS-related Snord116 repetitive locus of small nucleolar RNAs and host genes, and the antisense transcript to AS-causing ubiquitin ligase encoding Ube3a (Ube3a-ATS). Neuron-specific transcriptional progression through Ube3a-ATS correlates with paternal Ube3a silencing and chromatin decondensation. Interestingly, topoisomerase inhibitors, including topotecan, were recently identified in an unbiased drug screen for compounds that could reverse the silent paternal allele of Ube3a in neurons, but the mechanism of topotecan action on the PWS/AS locus is unknown. Here, we demonstrate that topotecan treatment stabilizes the formation of RNA:DNA hybrids (R loops) at G-skewed repeat elements within paternal Snord116, corresponding to increased chromatin decondensation and inhibition of Ube3a-ATS expression. Neural precursor cells from paternal Snord116 deletion mice exhibit increased Ube3a-ATS levels in differentiated neurons and show a reduced effect of topotecan compared with wild-type neurons. These results demonstrate that the AS candidate drug topotecan acts predominantly through stabilizing R loops and chromatin decondensation at the paternally expressed PWS Snord116 locus. Our study holds promise for targeted therapies to the Snord116 locus for both AS and PWS.

Published

2013

29. CRISPR/Cas9 directed to the Ube3a antisense transcript improves Angelman syndrome phenotype in mice.

Author

Schmid, Ralf S., Xuefeng Deng, Panikker, Priyalakshmi, Msackyi, Msema, Breton, Camilo, Wilson, James M., and Deng, Xuefeng

Subjects

*ANGELMAN syndrome, *PHENOTYPES, *GENOMIC imprinting, *CRISPRS, *GENOME editing, *RNA metabolism, *ENZYME metabolism, *RESEARCH, *ANIMAL experimentation, *RESEARCH methodology, *RNA, *MEDICAL cooperation, *EVALUATION research, *GENE expression, *COMPARATIVE studies, *ENZYMES, *MICE, BRAIN metabolism

Abstract

Gene editing holds the potential to correct mutations and cure devastating genetic disorders. The technology has not yet proven efficacious for therapeutic use in CNS diseases with ubiquitous neuronal defects. Angelman syndrome (AS), a severe neurodevelopmental disorder, is caused by a lack of maternal expression of the UBE3A gene. Because of genomic imprinting, only neurons are affected. One therapeutic approach focuses on the intact paternal UBE3A copy in patients with AS that is silenced by an antisense transcript (UBE3A-ATS). We show here that gene editing of Ube3a-ATS in the mouse brain resulted in the formation of base pair insertions/deletions (indels) in neurons and the subsequent unsilencing of the paternal Ube3a allele in neurons, which partially corrected the behavioral phenotype of a murine AS model. This study provides compelling evidence to further investigate editing of the homologous region of the human UBE3A-ATS because this may provide a lasting therapeutic effect for patients with AS. [ABSTRACT FROM AUTHOR]

Published

2021

30. Refining the Behavioral Phenotype of Angelman Syndrome: Examining Differences in Motivation for Social Contact Between Genetic Subgroups.

Author

Heald, Mary, Adams, Dawn, Walls, Emily, and Oliver, Christopher

Subjects

SOCIAL contact, ANGELMAN syndrome, PHENOTYPES, REWARD (Psychology), GENOMIC imprinting

Abstract

Angelman syndrome (AS) is caused by loss of information from the 15q11.2-13 region on the maternal chromosome with striking phenotypic difference from Prader–Willi syndrome in which information is lost from the same region on the paternal chromosome. Motivation for social contact and sensory seeking behaviors are often noted as characteristics of the phenotype of AS and it has been argued that the strong drive for social contact supports a kinship theory interpretation of genomic imprinting. In this study we developed an experimental paradigm for quantifying the motivation for social contact in AS and examined differences across the genetic subtypes that cause AS [deletion, imprinting centre defect (ICD), uniparental disomy and UBE3A mutation]. Using single case experimental designs we examined the rate of acquisition of behavioral responses using operant learning paradigms for 21 children with AS whilst systematically varying the nature of social and sensory reinforcement. Variability in rates of acquisition was influenced by the nature of rewarding stimuli. Across the total sample both sensory stimuli and social contact could increase the rate of rewarded behavior with difference between children in the most effective reward. A striking difference in the rewarding properties of social contact across genetic subtypes was evidenced by non-deletion genetic causes of AS showing significantly higher rates of responding than the deletion cause in the social reinforcement paradigm. The results indicate that reinforcer assessment can beneficially inform behavioral interventions and that within syndrome variability in the behavioral phenotype of AS is likely driven by genetic difference. The non-deletion cause of AS, and particularly the ICD group, may be the optimal group for further study of genomic imprinting. [ABSTRACT FROM AUTHOR]

Published

2021

31. Communication‐related assessments in an Angelman syndrome mouse model.

Author

Perrino, Peter A., Chamberlain, Stormy J., Eigsti, Inge‐Marie, and Fitch, Roslyn Holly

Subjects

*ANGELMAN syndrome, *AUDITORY processing disorder, *ULTRASONIC motors, *SOUNDS, *TRANSGENIC mice, *GENOMIC imprinting, *SPEECH apraxia, *HUMAN voice

Abstract

Introduction: Angelman syndrome (AS) is a neurodevelopmental disorder characterized by motor deficits, seizures, some autistic‐like behaviors, and severe impairment of speech. A dysfunction of the maternally imprinted UBE3A gene, coupled with a functional yet silenced paternal copy, results in AS. Although studies of transgenic mouse models have revealed a great deal about neural populations and rescue timeframes for specific features of AS, these studies have largely failed to examine intermediate phenotypes that contribute to the profound communicative disabilities associated with AS. Methods: Here, we use a variety of tasks, including assessments of rapid auditory processing and social communication. Expressive vocalizations were directly assessed and correlated against other core behavioral measures (motor, social, acoustic perception) to model putative influences on communication. Results: AS mice displayed the characteristic phenotypes associated with Angelman syndrome (i.e., social and motor deficits), as well as marginal enhancements in rapid auditory processing ability. Our characterization of adult ultrasonic vocalizations further showed that AS mice produce fewer vocalizations and vocalized for a shorter amount of time when compared to controls. Additionally, a strong correlation between motor indices and ultrasonic vocalization output was shown, suggesting that the motor impairments in AS may contribute heavily to communication impairments. Conclusion: In summary, the combination of motor deficits, social impairment, marginal rapid auditory enhancements, and altered ultrasonic vocalizations reported in a mouse model of AS clearly parallel the human symptoms of the disorder. This mouse model offers a novel route to interrogate the underlying genetic, physiologic, and behavioral influences on the under‐studied topic of impaired communication in AS. [ABSTRACT FROM AUTHOR]

Published

2021

32. Methylation-Specific Multiplex Ligation-Dependent Probe Amplification and Identification of Deletion Genetic Subtypes in Prader-Willi Syndrome

Author

Henkhaus, Rebecca S, Kim, Soo-Jeong, Kimonis, Virginia E, Gold, June-Anne, Dykens, Elisabeth M, Driscoll, Daniel J, and Butler, Merlin G

Subjects

Biological Sciences, Biomedical and Clinical Sciences, Genetics, Brain Disorders, Neurological, Angelman Syndrome, Chromosomes, Human, Pair 15, DNA Methylation, DNA Probes, Female, Genomic Imprinting, Humans, Male, Nucleic Acid Amplification Techniques, Prader-Willi Syndrome, Reagent Kits, Diagnostic, Sequence Deletion, Telomere, Clinical Sciences, Genetics & Heredity, Clinical sciences

Abstract

PurposePrader-Willi syndrome (PWS) and Angelman syndrome (AS) are complex neurodevelopmental disorders caused by loss of expression of imprinted genes from the 15q11-q13 region depending on the parent of origin. Methylation-specific multiplex ligation-dependent probe amplification (MS-MLPA) kits from MRC-Holland (Amsterdam, The Netherlands) were used to detect PWS and AS deletion subtypes. We report our experience with two versions of the MS-MLPA-PWS/AS kit (original A1 and newer B1) in determining methylation status and deletion subtypes in individuals with PWS.MethodsMS-MLPA analysis was performed on DNA isolated from a large cohort of PWS subjects with the MS-MLPA-PWS/AS-A1 and -B1 probe sets.ResultsBoth MS-MLPA kits will identify deletions in the 15q11-q13 region but the original MS-MLPA-A1 kit has a higher density of probes at the telomeric end of the 15q11-q13 region, which is more useful for identifying individuals with atypical deletions. The newer B1 kit contains more probes in the imprinting center (IC) and adjoining small noncoding RNAs useful in identifying small microdeletions.ConclusionThe A1 kit identified the typical deletions and smaller atypical deletions, whereas the B1 kit was more informative for identifying microdeletions including the IC and SNORD116 regions. Both kits should be made available for accurate characterization of PWS/AS deletion subtypes as well as evaluating for IC and SNORD116 microdeletions.

Published

2012

33. Double‐blind therapeutic trial in Angelman syndrome using betaine and folic acid

Author

Peters, Sarika U, Bird, Lynne M, Kimonis, Virginia, Glaze, Daniel G, Shinawi, Lina M, Bichell, Terry Jo, Barbieri‐Welge, Rene, Nespeca, Mark, Anselm, Irina, Waisbren, Susan, Sanborn, Erica, Sun, Qin, O'Brien, William E, Beaudet, Arthur L, and Bacino, Carlos A

Subjects

Nutrition, Pediatric, Clinical Research, Rare Diseases, Brain Disorders, Biotechnology, Intellectual and Developmental Disabilities (IDD), Neurosciences, Clinical Trials and Supportive Activities, Human Genome, Genetics, Adolescent, Angelman Syndrome, Betaine, Child, Child, Preschool, Chromosomes, Human, Pair 15, DNA Methylation, Double-Blind Method, Drug Combinations, Female, Folic Acid, Genomic Imprinting, Humans, Infant, Lipotropic Agents, Male, Phenotype, Placebos, Ubiquitin-Protein Ligases, Vitamin B Complex, Angelman syndrome, methylation, high dose folic acid, betaine, imprinting disorders, treatment, promotion of methylation, Clinical Sciences

Abstract

Angelman syndrome (AS) is caused by reduced or absent expression of the maternally inherited ubiquitin protein ligase 3A gene (UBE3A), which maps to chromosome 15q11-q13. UBE3A is subject to genomic imprinting in neurons in most regions of the brain. Expression of UBE3A from the maternal chromosome is essential to prevent AS, because the paternally inherited gene is not expressed, probably mediated by antisense UBE3A RNA. We hypothesized that increasing methylation might reduce expression of the antisense UBE3A RNA, thereby increasing UBE3A expression from the paternal gene and ameliorating the clinical phenotype. We conducted a trial using two dietary supplements, betaine and folic acid to promote global levels of methylation and attempt to activate the paternally inherited UBE3A gene. We performed a number of investigations at regular intervals including general clinical and developmental evaluations, biochemical determinations on blood and urine, and electroencephalographic studies. We report herein the data on 48 children with AS who were enrolled in a double-blind placebo-controlled protocol using betaine and folic acid for 1 year. There were no statistically significant changes between treated and untreated children; however, in a small subset of patients we observed some positive trends.

Published

2010

34. Clinical characteristics and epilepsy in genomic imprinting disorders: Angelman syndrome and Prader–Willi syndrome.

Author

Wang, Tzong-Shi, Tsai, Wen-Hsin, Tsai, Li-Ping, and Wong, Shi-Bing

Abstract

Angelman syndrome (AS) and Prader–Willi syndrome (PWS) are considered sister imprinting disorders. Although both AS and PWS congenital neurodevelopmental disorders have chromosome 15q11.3-q13 dysfunction, their molecular mechanisms differ owing to genomic imprinting, which results in different parent-of-the-origin gene expressions. Recently, several randomized controlled trials have been proceeded to treat specific symptoms of AS and PWS. Due to the advance of clinical management, early diagnosis for patients with AS and PWS is important. PWS is induced by multiple paternal gene dysfunctions, including those in MKRN3, MAGEL2, NDN, SNURF-SNPRPN, NPAP1, and a cluster of small nucleolar RNA genes. PWS patients exhibit characteristic facial features, endocrinological, and behavioral phenotypes, including short and obese figures, hyperphagia, growth hormone deficiency, hypogonadism, autism, or obsessive–compulsive-like behaviors. In addition, hypotonia, poor feeding, failure to thrive, and typical facial features are major factors for early diagnosis of PWS. For PWS patients, epilepsy is not common and easy to treat. Conversely, AS is a single-gene disorder induced by ubiquitin-protein ligase E3A dysfunction, which only expresses from a maternal allele. AS patients develop epilepsy in their early lives and their seizures are difficult to control. The distinctive gait pattern, excessive laughter, and characteristic electroencephalography features, which contain anterior-dominated, high-voltage triphasic delta waves intermixed with epileptic spikes, result in early suspicion of AS. Often, polytherapy, including the combination of valproate, levetiracetam, lamotrigine, and benzodiazepines, is required for controlling seizures of AS patients. Notably, carbamazepine, oxcarbazepine, and vigabatrin should be avoided, since these may induce nonconvulsive status epilepticus. AS and PWS presented with distinct clinical manifestations according to specific molecular defects due to genomic imprinting. Early diagnosis and teamwork intervention, including geneticists, neurologists, rehabilitation physicians, and pulmonologists, are important. Epilepsy is common in patients with AS, and after proper treatment, seizures could be effectively controlled in late childhood or early adulthood for both AS and PWS patients. [ABSTRACT FROM AUTHOR]

Published

2020

35. Atypical cases of Angelman syndrome

Author

Lawson‐Yuen, Amy, Wu, Bai‐Lin, Lip, Va, Sahoo, Trilochan, and Kimonis, Virginia

Subjects

Biological Sciences, Biomedical and Clinical Sciences, Genetics, Mental Health, Pediatric, Rare Diseases, Clinical Research, Intellectual and Developmental Disabilities (IDD), Brain Disorders, Human Genome, Congenital, Angelman Syndrome, Child, Preschool, Chromosomes, Human, Pair 15, Female, Gene Deletion, Gene Dosage, Genomic Imprinting, Humans, Male, Phenotype, Ubiquitin-Protein Ligases, Clinical Sciences, Clinical sciences

Abstract

Angelman syndrome (AS) is a profound disorder notable for mental retardation and severe language deficits that results from lack of function of the maternally inherited copy of the UBE3A gene. Chromosome deletions of 15q11q13, paternal uniparental disomy (UPD), UBE3A gene mutations, and imprinting center defects are all commonly recognized mechanisms that disrupt the function of the maternal copy of the UBE3A gene. We report here two patients with different atypical etiologies of AS. The first patient is a 3-year-old boy with global developmental delay, severe speech deficits, seizures, and very happy disposition. Southern blot analysis for the maternal and paternal chromosome 15 methylation products showed a mosaic methylation pattern, suggesting an imprinting center defect. The second patient is a 4(1/2)-year-old boy with global developmental delay, no expressive language, microcephaly, seizures, and ataxic gait. Array-based comparative genomic hybridization (CGH) demonstrated a loss in copy number for two overlapping clones encompassing the UBE3A gene, indicating a partial deletion within UBE3A. His mother, who was adopted, had an identical pattern, suggesting that her deletion was probably on her paternally imprinted allele. These patients illustrate the expanding spectrum of molecular findings in AS, reinforce the need to maintain suspicion when clinical features suggest AS but initial testing is normal, and show the power of CGH as a tool to uncover partial UBE3A deletions.

Published

2006

36. Genomic imprinting does not reduce the dosage of UBE3A in neurons

Author

Paul R. Hillman, Sarah G. B. Christian, Ryan Doan, Noah D. Cohen, Kranti Konganti, Kory Douglas, Xu Wang, Paul B. Samollow, and Scott V. Dindot

Subjects

Ube3a, Genomic imprinting, Dosage compensation, Angelman syndrome, Ube3a antisense, Evolution, Genetics, QH426-470

Abstract

Abstract Background The ubiquitin protein E3A ligase gene (UBE3A) gene is imprinted with maternal-specific expression in neurons and biallelically expressed in all other cell types. Both loss-of-function and gain-of-function mutations affecting the dosage of UBE3A are associated with several neurodevelopmental syndromes and psychological conditions, suggesting that UBE3A is dosage-sensitive in the brain. The observation that loss of imprinting increases the dosage of UBE3A in brain further suggests that inactivation of the paternal UBE3A allele evolved as a dosage-regulating mechanism. To test this hypothesis, we examined UBE3A transcript and protein levels among cells, tissues, and species with different imprinting states of UBE3A. Results Overall, we found no correlation between the imprinting status and dosage of UBE3A. Importantly, we found that maternal Ube3a protein levels increase in step with decreasing paternal Ube3a protein levels during neurogenesis in mouse, fully compensating for loss of expression of the paternal Ube3a allele in neurons. Conclusions Based on our findings, we propose that imprinting of UBE3A does not function to reduce the dosage of UBE3A in neurons but rather to regulate some other, as yet unknown, aspect of gene expression or protein function.

Published

2017

37. Response to vocal music in Angelman syndrome contrasts with Prader-Willi syndrome.

Author

Kotler, Jennifer, Mehr, Samuel A., Egner, Alena, Haig, David, and Krasnow, Max M.

Subjects

PRADER-Willi syndrome, ANGELMAN syndrome, VOCAL music, GENOMIC imprinting, GENE expression, BIRDSONGS

Abstract

Parent-offspring conflict—conflict over resource distribution within families due to differences in genetic relatedness—is the biological foundation for many psychological phenomena. In genomic imprinting disorders, parent-specific genetic expression is altered, causing imbalances in behaviors influenced by parental investment. We use this natural experiment to test the theory that parent-offspring conflict contributed to the evolution of vocal music by moderating infant demands for parental attention. Individuals with Prader-Willi syndrome, a genomic imprinting disorder resulting from increased relative maternal genetic contribution, show enhanced relaxation responses to song, consistent with reduced demand for parental investment (Mehr, Kotler, Howard, Haig, & Krasnow, 2017 , Psychological Science). We report the necessary complementary pattern here: individuals with Angelman syndrome, a genomic imprinting disorder resulting from increased relative paternal genetic contribution, demonstrate a relatively reduced relaxation response to song, suggesting increased demand for parental attention. These results support the extension of genetic conflict theories to psychological resources like parental attention. [ABSTRACT FROM AUTHOR]

Published

2019

38. Whole exome sequencing and methylation-specific multiplex ligation-dependent probe amplification applied to identify Angelman syndrome due to paternal uniparental disomy in two unrelated patients.

Author

Li, Haibei, Yang, Haiqi, Lv, Nan, Ma, Caiyun, Li, Jingjie, and Shang, Qing

Subjects

*ANGELMAN syndrome, *HOMOZYGOSITY, *EXOMES, *CHROMOSOMAL translocation, *GENOMIC imprinting, *SINGLE nucleotide polymorphisms, *HUMAN chromosome abnormality diagnosis, *CHROMOSOMES

Abstract

Angelman syndrome (AS) is a congenital neurodevelopmental disorder typically occurring due to functional defects of the UBE3A gene caused by uniparental disomy (UPD), translocation or single gene mutation. UBE3A gene exhibits imprinting expression, and only maternal inherited alleles express functional UBE3A protein in the brain. The common method to diagnose AS is single nucleotide polymorphism array or methylation-specific multiplex ligation-dependent probe amplification (MS-MLPA). In recent years, whole exome sequencing (WES) has been increasingly used in the genetic diagnosis of a variety of indications, exhibiting great advantages as a comprehensive and unbiased testing method. In the present study, the cases of two unrelated patients with Robertsonian-like translocation in chromosome 15, namely 45,XX,der(15;15)(q10;q10) and 45,XY,der(15;15)(q10;q10), are reported. The first case was diagnosed with AS by WES and validated by Sanger sequencing. In contrast to 42.84% homozygous variants on all chromosomes, 92.69% homozygosity variants were observed on chromosome 15. A homozygous stretch identifier was applied and identified a homozygous region across the entire chromosome 15. Sanger sequencing was used to further determine the subtype and confirm that two homozygous variants on chromosome 15 with low allele frequency (<0.01) were derived only from the father and not from the mother, thereby indicating a paternal UPD case, classified as isodisomy. MS-MLPA results of the other AS patient with the same karyotype indicated that he had a high possibility of paternal UPD at chromosome 15. Taken together, the current study suggested the potential application of WES in detecting and facilitating the diagnosis of UPD. [ABSTRACT FROM AUTHOR]

Published

2019

39. Imprinting methylation in SNRPN and MEST1 in adult blood predicts cognitive ability.

Author

Lorgen-Ritchie, Marlene, Murray, Alison D., Ferguson-Smith, Anne C., Richards, Marcus, Horgan, Graham W., Phillips, Louise H., Hoad, Gwen, Gall, Ishbel, Harrison, Kristina, McNeill, Geraldine, Ito, Mitsuteru, and Haggarty, Paul

Subjects

*GENOMIC imprinting, *DNA methylation, *COGNITIVE ability, *PSYCHOLOGY of adults, *BLOOD testing

Abstract

Genomic imprinting is important for normal brain development and aberrant imprinting has been associated with impaired cognition. We studied the imprinting status in selected imprints (H19, IGF2, SNRPN, PEG3, MEST1, NESPAS, KvDMR, IG-DMR and ZAC1) by pyrosequencing in blood samples from longitudinal cohorts born in 1936 (n = 485) and 1921 (n = 223), and anterior hippocampus, posterior hippocampus, periventricular white matter, and thalamus from brains donated to the Aberdeen Brain Bank (n = 4). MEST1 imprint methylation was related to childhood cognitive ability score (-0.416 95% CI -0.792,-0.041; p = 0.030), with the strongest effect evident in males (-0.929 95% CI -1.531,-0.326; p = 0.003). SNRPN imprint methylation was also related to childhood cognitive ability (+0.335 95%CI 0.008,0.663; p = 0.045). A significant association was also observed for SNRPN methylation and adult crystallised cognitive ability (+0.262 95%CI 0.007,0.517; p = 0.044). Further testing of significant findings in a second cohort from the same region, but born in 1921, resulted in similar effect sizes and greater significance when the cohorts were combined (MEST1; -0.371 95% CI -0.677,-0.065; p = 0.017; SNRPN; +0.361 95% CI 0.079,0.643; p = 0.012). For SNRPN and MEST1 and four other imprints the methylation levels in blood and in the five brain regions were similar. Methylation of the paternally expressed, maternally methylated genes SNRPN and MEST1 in adult blood was associated with cognitive ability in childhood. This is consistent with the known importance of the SNRPN containing 15q11-q13 and the MEST1 containing 7q31-34 regions in cognitive function. These findings, and their sex specific nature in MEST1, point to new mechanisms through which complex phenotypes such as cognitive ability may be inherited. These mechanisms are potentially relevant to both the heritable and non-heritable components of cognitive ability. The process of epigenetic imprinting—within SNRPN and MEST1 in particular—and the factors that influence it, are worthy of further study in relation to the determinants of cognitive ability. [ABSTRACT FROM AUTHOR]

Published

2019

40. Patent Issued for Oligonucleotides for inducing paternal UBE3A expression (USPTO 11852627).

Subjects

GENE expression, OLIGONUCLEOTIDES, NON-coding RNA, GENOMIC imprinting, PATENTS, CENTRAL nervous system diseases

Abstract

A patent has been issued to F. Hoffmann-La Roche Inc. for oligonucleotides that can induce the expression of the UBE3A gene, specifically the paternal copy, in neuronal cells. This is significant because Angelman syndrome, a neuro-genetic disorder, is caused by the deletion or inactivation of the UBE3A gene on the maternally inherited chromosome 15q11.2. The patent describes the design and use of antisense oligonucleotides to target a specific region of the SNHG14 long non-coding RNA, which suppresses UBE3A expression. The invention also includes methods for treating or preventing diseases associated with decreased UBE3A activity, such as Angelman syndrome. [Extracted from the article]

Published

2024

41. Clinical Utility of Methylation-Specific Multiplex Ligation-Dependent Probe Amplification for the Diagnosis of Prader–Willi Syndrome and Angelman Syndrome

Author

Yongsook Park, Sung Sup Park, Sung Im Cho, Boram Kim, Jong-Hee Chae, Jiyeon Kim, Man Jin Kim, and Moon Woo Seong

Subjects

Oncology, medicine.medical_specialty, congenital, hereditary, and neonatal diseases and abnormalities, Prader–Willi syndrome, Concordance, Clinical Biochemistry, Bisulfite sequencing, Methylation, Chromosome 15, Utility, Angelman syndrome, Internal medicine, Diagnosis, Medicine, Humans, Multiplex ligation-dependent probe amplification, Imprinting (psychology), Retrospective Studies, Chromosomes, Human, Pair 15, business.industry, Biochemistry (medical), nutritional and metabolic diseases, General Medicine, Methylation-specific multiplex ligation-dependent probe amplification, DNA Methylation, medicine.disease, Uniparental disomy, nervous system diseases, Methylation-specific PCR, Original Article, business, Genomic imprinting, Diagnostic Genetics, Multiplex Polymerase Chain Reaction, Prader-Willi Syndrome

Abstract

Background Prader-Willi syndrome (PWS) and Angelman syndrome (AS) are genomic imprinting disorders that are mainly caused by a deletion on 15q11-q13, the uniparental disomy of chromosome 15, or an imprinting defect. We evaluated the utility of methylation-specific multiplex ligation-dependent probe amplification (MS-MLPA) as a diagnostic tool and for demonstrating the relationship between molecular mechanisms and clinical presentation. Methods We performed MS-MLPA using DNA samples from 93 subjects (45 PWS, 24 AS, and 24 non-PWS/AS controls) who had previously undergone MS-PCR for the diagnosis of PWS/AS. We compared the results of both assays, and patients' clinical phenotypes were reviewed retrospectively. Results MS-MLPA showed a 100% concordance rate with MS-PCR. Among the 45 PWS patients, 26 (57.8%) had a deletion of 15q11-q13, and the others (42.2%) had uniparental disomy 15 or an imprinting defect. Among the 24 AS patients, 16 (66.7%) had a deletion of 15q11-q13, 7 AS patients (29.2%) had uniparental disomy 15 or an imprinting defect, and one AS patient (4.2%) showed an imprinting center deletion. Conclusions MS-MLPA has clinical utility for the diagnosis of PWS/AS, and it is superior to MS-PCR in that it can identify the molecular mechanism underlying the disease.

Published

2022

42. CRISPR/Cas9 Epigenome Editing Potential for Rare Imprinting Diseases: A Review

Author

Linn Amanda Syding, Petr Nickl, Petr Kasparek, and Radislav Sedlacek

Subjects

rare disease, CRISPR/Cas9, epigenome editing, transcriptome editing, genomic imprinting, Angelman syndrome, Cytology, QH573-671

Abstract

Imprinting diseases (IDs) are rare congenital disorders caused by aberrant dosages of imprinted genes. Rare IDs are comprised by a group of several distinct disorders that share a great deal of homology in terms of genetic etiologies and symptoms. Disruption of genetic or epigenetic mechanisms can cause issues with regulating the expression of imprinted genes, thus leading to disease. Genetic mutations affect the imprinted genes, duplications, deletions, and uniparental disomy (UPD) are reoccurring phenomena causing imprinting diseases. Epigenetic alterations on methylation marks in imprinting control centers (ICRs) also alters the expression patterns and the majority of patients with rare IDs carries intact but either silenced or overexpressed imprinted genes. Canonical CRISPR/Cas9 editing relying on double-stranded DNA break repair has little to offer in terms of therapeutics for rare IDs. Instead CRISPR/Cas9 can be used in a more sophisticated way by targeting the epigenome. Catalytically dead Cas9 (dCas9) tethered with effector enzymes such as DNA de- and methyltransferases and histone code editors in addition to systems such as CRISPRa and CRISPRi have been shown to have high epigenome editing efficiency in eukaryotic cells. This new era of CRISPR epigenome editors could arguably be a game-changer for curing and treating rare IDs by refined activation and silencing of disturbed imprinted gene expression. This review describes major CRISPR-based epigenome editors and points out their potential use in research and therapy of rare imprinting diseases.

Published

2020

43. Parent of origin gene expression in a founder population identifies two new candidate imprinted genes at known imprinted regions.

Author

Mozaffari, Sahar V., Stein, Michelle M., Magnaye, Kevin M., Nicolae, Dan L., and Ober, Carole

Subjects

*LEUCOCYTES, *GENE expression, *GROUP identity, *LYMPHOBLASTOID cell lines, *RNA sequencing

Abstract

Genomic imprinting is the phenomena that leads to silencing of one copy of a gene inherited from a specific parent. Mutations in imprinted regions have been involved in diseases showing parent of origin effects. Identifying genes with evidence of parent of origin expression patterns in family studies allows the detection of more subtle imprinting. Here, we use allele specific expression in lymphoblastoid cell lines from 306 Hutterites related in a single pedigree to provide formal evidence for parent of origin effects. We take advantage of phased genotype data to assign parent of origin to RNA-seq reads in individuals with gene expression data. Our approach identified known imprinted genes, two putative novel imprinted genes, PXDC1 and PWAR6, and 14 genes with asymmetrical parent of origin gene expression. We used gene expression in peripheral blood leukocytes (PBL) to validate our findings, and then confirmed imprinting control regions (ICRs) using DNA methylation levels in the PBLs. [ABSTRACT FROM AUTHOR]

Published

2018

44. "Angelman Syndrome Antisense Treatment" in Patent Application Approval Process (USPTO 20230332152).

Subjects

PATENT applications, ANGELMAN syndrome, NUCLEIC acid hybridization, GENOMIC imprinting, GENE expression, EPILEPSY

Abstract

Keywords: Angelman Syndrome; Antisense Technology; Bioengineering; Biotechnology; Central Nervous System; Central Nervous System Diseases and Conditions; Chromosome Disorders; Congenital Abnormalities; Enzymes and Coenzymes; Genetics; Health and Medicine; Movement Disorders; Musculoskeletal Diseases and Conditions; Nuclease; Patent Application EN Angelman Syndrome Antisense Technology Bioengineering Biotechnology Central Nervous System Central Nervous System Diseases and Conditions Chromosome Disorders Congenital Abnormalities Enzymes and Coenzymes Genetics Health and Medicine Movement Disorders Musculoskeletal Diseases and Conditions Nuclease Patent Application 170 170 1 11/06/23 20231110 NES 231110 2023 NOV 9 (NewsRx) -- By a News Reporter-Staff News Editor at Gene Therapy Weekly -- A patent application by the inventor Dindot, Scott Victor (College Station, TX, US), filed on June 30, 2023, was made available online on October 19, 2023, according to news reporting originating from Washington, D.C., by NewsRx correspondents. The modified oligonucleotide of claim 14, wherein the modified oligonucleotide is a nuclease guide RNA oligonucleotide (gRNA)." A modified oligonucleotide comprising a contiguous nucleotide sequence of 10 to 30 nucleotides in length with nucleic acid complementarity to a contiguous portion of the nucleotide sequence set forth in SEQ ID NO: 2. The modified oligonucleotide of claim 14, wherein the modified oligonucleotide is a short hairpin RNA oligonucleotide (shRNA). [Extracted from the article]

Published

2023

45. Patent Application Titled "Oligonucleotides For Inducing Paternal Ube3a Expression" Published Online (USPTO 20230296587).

Subjects

GENE expression, PATENT applications, OLIGONUCLEOTIDES, GENOMIC imprinting, NUCLEOTIDE sequence

Abstract

An antisense oligonucleotide which comprises a contiguous nucleotide sequence of 10 to 30 nucleotides in length with at least 98% complementarity to position 25278410 to 25419462 on human chromosome 15, wherein the antisense oligonucleotide is capable of inducing human paternal UBE3A expression. The oligonucleotide of claim 15, wherein the oligonucleotide is a gapmer of formula 5'-F-G-F'-3', where region F and F' independently comprise 1 to 7 modified nucleosides and G is a region between 6 and 16 nucleosides which are capable of recruiting RNaseH. The oligonucleotide of claim 1 wherein the oligonucleotide is a gapmer of the formula F-G-F' wherein each of regions F and F' independently consists of 2, 3, 4, or 5 modified nucleoside units and region G consists of 9, 10, 11, 12, 13, 14, or 15 nucleoside units. The oligonucleotide of claim 13, wherein at least 60% of the internucleoside linkages in the oligonucleotide are phosphorothioate internucleoside linkages. [Extracted from the article]

Published

2023

46. Atypical presentation of Angelman syndrome with intact expressive language due to <scp>low‐level</scp> mosaicism

Author

Ruchi Punatar, Alena Egense, Rong Mao, Melinda Procter, Michelle Bosworth, Denise I. Quigley, Kathleen Angkustsiri, and Suma P. Shankar

Subjects

Male, Genomic Imprinting, Mosaicism, Genetics, Humans, Angelman Syndrome, Prader-Willi Syndrome, Molecular Biology, Genetics (clinical), Language

Abstract

Angelman syndrome (AS) occurs due to a lack of expression or function of the maternally inherited UBE3A gene. Individuals with AS typically have significant developmental delay, severe speech impairment with absent to minimal verbal language, gait abnormalities including ataxia, and an incongruous happy demeanor. The majority of individuals with AS also have seizures and microcephaly. Some individuals with mosaic AS have been reported to have expressive language and milder levels of developmental delay.We report a male patient presenting with mild to moderate intellectual disability, hyperphagia, obesity, and the ability to communicate verbally. His phenotype was suggestive of Prader-Willi syndrome. However, methylation testing was positive for Angelman syndrome and additional methylation specific multiplex ligation-dependent amplification (MS-MLPA) study revealed low-level mosaicism for AS.A broader phenotypic spectrum should be considered for AS as patients with atypical presentations may otherwise elude diagnosis.

Published

2022

47. Genomic Imprinting and Uniparental Disomy

Author

Wang, Jin-Chen C., Gersen, Steven L., editor, and Keagle, Martha B., editor

Published

2005

48. Novel intragenic deletions within the UBE3A gene in two unrelated patients with Angelman syndrome: case report and review of the literature.

Author

Aguilera, Cinthia, Viñas-Jornet, Marina, Baena, Neus, Gabau, Elisabeth, Fernández, Concepción, Capdevila, Nuria, Cirkovic, Sanja, Sarajlija, Adrijan, Miskovic, Marijana, Radivojevic, Danijela, Ruiz, Anna, and Guitart, Miriam

Subjects

*ANGELMAN syndrome, *BODY dysmorphic disorder, *GENOMIC imprinting, *METHYLATION, *EXONS (Genetics)

Abstract

Background: Patients with Angelman syndrome (AS) are affected by severe intellectual disability with absence of speech, distinctive dysmorphic craniofacial features, ataxia and a characteristic behavioral phenotype. AS is caused by the lack of expression in neurons of the UBE3A gene, which is located in the 15q11.2-q13 imprinted region. Functional loss of UBE3A is due to 15q11.2-q13 deletion, mutations in the UBE3A gene, paternal uniparental disomy and genomic imprinting defects. Case presentation: We report here two patients with clinical features of AS referred to our hospital for clinical follow-up and genetic diagnosis. Methylation Specific-Multiplex Ligation-Dependent Probe Amplification (MS-MLPA) of the 15q11.2-q13 region was carried out in our laboratory as the first diagnostic tool detecting two novel UBE3A intragenic deletions. Subsequently, the MLPA P336-A2 kit was used to confirm and determine the size of the UBE3A deletion in the two patients. A review of the clinical features of previously reported patients with whole UBE3A gene or partial intragenic deletions is presented here together with these two new patients. Conclusion: Although rare, UBE3A intragenic deletions may represent a small fraction of AS patients without a genetic diagnosis. Testing for UBE3A intragenic exonic deletions should be performed in those AS patients with a normal methylation pattern and no mutations in the UBE3A gene. [ABSTRACT FROM AUTHOR]

Published

2017

49. Diagnosis of the Genomic Imprinting Diseases by the Usage of Conventional and Molecular Analyses.

Author

Kaymak, Ayşegül Öztürk, Karaoğuz, Meral Yirmibeş, Gücüyener, Kıvılcım, and Perçin, Ferda Emriye

Subjects

*PRADER-Willi syndrome diagnosis, *GENOMIC imprinting, *INTELLECTUAL disabilities

Abstract

Objective: Prader-Willi (PWS) and Angelman syndromes (AS) are genomic imprinting diseases with intellectual disability. In approximately 70 % of the cases, there is a cytogenetic deletion involving the chromosome 15q11-q13 inherited from patient's father (in PWS) and from patient's mother (in AS). In approximately 20-25% and 3-7% of the cases, there is an uniparental disomy (UPD) of chromosome 15 in PWS and AS patients, respectively. The mutation ratio in AS patients is approximately 10 %, while the ratio is two percent in PWS patients. Methods: In the first step cytogenetic analyses were performed by using high resolution banding (HRB) for 20 patients who were selected by diagnostic criteria (11 pre-diagnosed with AS and 9 pre-diagnosed with PWS). Then, via Fluorescent in situ Hybridization (FISH) technique, SNRPN gene (small nuclear ribonucleoprotein polypeptide N gene) locus for PWS, D15S10 locus for AS were searched. Finally the uniparental disomy of chromosome 15 along with the mutation/deletion of imprinting center were examined. Results: HRB and FISH analyses revealed no deletion except in one AS patient whose D15S10 region was found deleted via FISH technique. Mutation/deletion of imprinting center analyses in all of them were evaluated as normal. Conclusion: As a result, by this project patients with PWS and AS, who were selected by the diagnostic criteria for each syndrome, were evaluated via conventional genetic and molecular genetics methods and they were offered with the efficient genetic counseling. [ABSTRACT FROM AUTHOR]

Published

2017

50. Angelman Syndrome: Identification and Management.

Author

Bonello, Daniela, Camilleri, Francesca, and Calleja-Agius, Jean

Subjects

DIFFERENTIAL diagnosis, GENETIC counseling, HUMAN reproductive technology, ANGELMAN syndrome, MEDICAL protocols, CONTINUING education units, DNA methylation, SYMPTOMS, GENETICS, PROGNOSIS, DIAGNOSIS, THERAPEUTICS

Abstract

Angelman syndrome (AS) is a neurobehavioral and genetically determined condition, which affects approximately 1 in 15,000 individuals. It is caused by various genetic mutations and deletions of the maternally-inherited UBE3Agene, on the 15q11-13 chromosomal region. The UBE3A gene, which encodes E3 ubiquitin ligase, shows tissue-specific imprinting, being expressed entirely from die maternal allele. The diagnosis of AS is confirmed either by methylation test or by mutation analysis. A more severe clinical picture is linked with the deletion phenotype. Patients with AS have a behavioral and motor pattern defined as "happy puppet" because it is characterized by puppet-like ataxic jerky movements; a happy, sociable disposition; and paroxysms of laughter. There is currently no cure for AS, and management is mainly symptomatic. Novel therapeutic options are directed toward the possibility of activating the silenced paternal copy of the UBE3A gene. [ABSTRACT FROM AUTHOR]

Published

2017