Medicine (Austin & Northern Health) - Research Publications

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Author: Bahlo, Melanie × Author: Berkovic, Samuel × End date: 2019 × Start date: 2012 ×

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    Evidence of linkage to chromosome 5p13.2-q11.1 in a large inbred family with genetic generalized epilepsy
    Kinay, D ; Oliver, KL ; Tuzun, E ; Damiano, JA ; Ulusoy, C ; Andermann, E ; Hildebrand, MS ; Bahlo, M ; Berkovic, SF (WILEY, 2018-08)
    The clinical genetics of genetic generalized epilepsy suggests complex inheritance; large pedigrees, with multiple affected individuals, are rare exceptions. We studied a large consanguineous family from Turkey where extensive electroclinical phenotyping revealed a familial phenotype most closely resembling juvenile myoclonic epilepsy. For a subject to be considered affected (n = 14), a diagnostic electroencephalogram was required. Seizure onset ranged between 6 and 19 years (mean = 12 years). Thirteen of 14 experienced myoclonic jerks; in 11, this was associated with eyelid blinking, and in 10 it was interspersed with absences. Generalized tonic-clonic seizures were seen in 11. One individual had generalized tonic-clonic seizures alone. Electroencephalograms demonstrated generalized polyspike and wave discharges that were not associated with photoparoxysmal response. Intellect was normal. Nineteen family members were subsequently chosen for nonparametric multipoint linkage analyses, which identified a 39.5 Mb region on chromosome 5 (P < 0.0001). Iterative analysis, including discovery of a subtly affected individual, narrowed the critical region to 15.4 Mb and possibly to 5.5 Mb. Homozygous versus heterozygous state of the refined 5p13.2-q11.1 haplotype was not associated with phenotypic severity or onset age, suggesting that one versus two pathogenic variants may result in similar phenotypes. Whole exome sequencing (n = 3) failed to detect any rare, protein-coding variants within the highly significant linkage region that includes HCN1 as a promising candidate.
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    In silico prioritization based on coexpression can aid epileptic encephalopathy gene discovery
    Oliver, KL ; Lukic, V ; Freytag, S ; Scheffer, IE ; Berkovic, SF ; Bahlo, M (LIPPINCOTT WILLIAMS & WILKINS, 2016-02)
    OBJECTIVE: To evaluate the performance of an in silico prioritization approach that was applied to 179 epileptic encephalopathy candidate genes in 2013 and to expand the application of this approach to the whole genome based on expression data from the Allen Human Brain Atlas. METHODS: PubMed searches determined which of the 179 epileptic encephalopathy candidate genes had been validated. For validated genes, it was noted whether they were 1 of the 19 of 179 candidates prioritized in 2013. The in silico prioritization approach was applied genome-wide; all genes were ranked according to their coexpression strength with a reference set (i.e., 51 established epileptic encephalopathy genes) in both adult and developing human brain expression data sets. Candidate genes ranked in the top 10% for both data sets were cross-referenced with genes previously implicated in the epileptic encephalopathies due to a de novo variant. RESULTS: Five of 6 validated epileptic encephalopathy candidate genes were among the 19 prioritized in 2013 (odds ratio = 54, 95% confidence interval [7,∞], p = 4.5 × 10(-5), Fisher exact test); one gene was false negative. A total of 297 genes ranked in the top 10% for both the adult and developing brain data sets based on coexpression with the reference set. Of these, 9 had been previously implicated in the epileptic encephalopathies (FBXO41, PLXNA1, ACOT4, PAK6, GABBR2, YWHAG, NBEA, KNDC1, and SELRC1). CONCLUSIONS: We conclude that brain gene coexpression data can be used to assist epileptic encephalopathy gene discovery and propose 9 genes as strong epileptic encephalopathy candidates worthy of further investigation.
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    PRIMA1 mutation: a new cause of nocturnal frontal lobe epilepsy
    Hildebrand, MS ; Tankard, R ; Gazina, EV ; Damiano, JA ; Lawrence, KM ; Dahl, H-HM ; Regan, BM ; Shearer, AE ; Smith, RJH ; Marini, C ; Guerrini, R ; Labate, A ; Gambardella, A ; Tinuper, P ; Lichetta, L ; Baldassari, S ; Bisulli, F ; Pippucci, T ; Scheffer, IE ; Reid, CA ; Petrou, S ; Bahlo, M ; Berkovic, SF (WILEY, 2015-08)
    OBJECTIVE: Nocturnal frontal lobe epilepsy (NFLE) can be sporadic or autosomal dominant; some families have nicotinic acetylcholine receptor subunit mutations. We report a novel autosomal recessive phenotype in a single family and identify the causative gene. METHODS: Whole exome sequencing data was used to map the family, thereby narrowing exome search space, and then to identify the mutation. RESULTS: Linkage analysis using exome sequence data from two affected and two unaffected subjects showed homozygous linkage peaks on chromosomes 7, 8, 13, and 14 with maximum LOD scores between 1.5 and 1.93. Exome variant filtering under these peaks revealed that the affected siblings were homozygous for a novel splice site mutation (c.93+2T>C) in the PRIMA1 gene on chromosome 14. No additional PRIMA1 mutations were found in 300 other NFLE cases. The c.93+2T>C mutation was shown to lead to skipping of the first coding exon of the PRIMA1 mRNA using a minigene system. INTERPRETATION: PRIMA1 is a transmembrane protein that anchors acetylcholinesterase (AChE), an enzyme hydrolyzing acetycholine, to membrane rafts of neurons. PRiMA knockout mice have reduction of AChE and accumulation of acetylcholine at the synapse; our minigene analysis suggests that the c.93+2T>C mutation leads to knockout of PRIMA1. Mutations with gain of function effects in acetylcholine receptor subunits cause autosomal dominant NFLE. Thus, enhanced cholinergic responses are the likely cause of the severe NFLE and intellectual disability segregating in this family, representing the first recessive case to be reported and the first PRIMA1 mutation implicated in disease.
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    Epidemiology and etiology of infantile developmental and epileptic encephalopathies in Tasmania
    Ware, TL ; Huskins, SR ; Grinton, BE ; Liu, Y-C ; Bennett, MF ; Harvey, M ; McMahon, J ; Andreopoulos-Malikotsinas, D ; Bahlo, M ; Howell, KB ; Hildebrand, MS ; Damiano, JA ; Rosenfeld, A ; Mackay, MT ; Mandelstam, S ; Leventer, RJ ; Harvey, AS ; Freeman, JL ; Scheffer, IE ; Jones, DL ; Berkovic, SF (WILEY, 2019-09)
    We sought to determine incidence, etiologies, and yield of genetic testing in infantile onset developmental and epileptic encephalopathies (DEEs) in a population isolate, with an intensive multistage approach. Infants born in Tasmania between 2011 and 2016, with seizure onset <2 years of age, epileptiform EEG, frequent seizures, and developmental impairment, were included. Following review of EEG databases, medical records, brain MRIs, and other investigations, clinical genetic testing was undertaken with subsequent research interrogation of whole exome sequencing (WES) in unsolved cases. The incidence of infantile DEEs was 0.44/1000 per year (95% confidence interval 0.25 to 0.71), with 16 cases ascertained. The etiology was structural in 5/16 cases. A genetic basis was identified in 6 of the remaining 11 cases (3 gene panel, 3 WES). In two further cases, WES identified novel variants with strong in silico data; however, paternal DNA was not available to support pathogenicity. The etiology was not determined in 3/16 (19%) cases, with a candidate gene identified in one of these. Pursuing clinical imaging and genetic testing followed by WES at an intensive research level can give a high diagnostic yield in the infantile DEEs, providing a solid base for prognostic and genetic counseling.
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    Polygenic burden in focal and generalized epilepsies
    Leu, C ; Stevelink, R ; Smith, AW ; Goleva, SB ; Kanai, M ; Ferguson, L ; Campbell, C ; Kamatani, Y ; Okada, Y ; Sisodiya, SM ; Cavalleri, GL ; Koeleman, BPC ; Lerche, H ; Jehi, L ; Davis, LK ; Najm, IM ; Palotie, A ; Daly, MJ ; Busch, RM ; Lal, D (OXFORD UNIV PRESS, 2019-11)
    Rare genetic variants can cause epilepsy, and genetic testing has been widely adopted for severe, paediatric-onset epilepsies. The phenotypic consequences of common genetic risk burden for epilepsies and their potential future clinical applications have not yet been determined. Using polygenic risk scores (PRS) from a European-ancestry genome-wide association study in generalized and focal epilepsy, we quantified common genetic burden in patients with generalized epilepsy (GE-PRS) or focal epilepsy (FE-PRS) from two independent non-Finnish European cohorts (Epi25 Consortium, n = 5705; Cleveland Clinic Epilepsy Center, n = 620; both compared to 20 435 controls). One Finnish-ancestry population isolate (Finnish-ancestry Epi25, n = 449; compared to 1559 controls), two European-ancestry biobanks (UK Biobank, n = 383 656; Vanderbilt biorepository, n = 49 494), and one Japanese-ancestry biobank (BioBank Japan, n = 168 680) were used for additional replications. Across 8386 patients with epilepsy and 622 212 population controls, we found and replicated significantly higher GE-PRS in patients with generalized epilepsy of European-ancestry compared to patients with focal epilepsy (Epi25: P = 1.64×10-15; Cleveland: P = 2.85×10-4; Finnish-ancestry Epi25: P = 1.80×10-4) or population controls (Epi25: P = 2.35×10-70; Cleveland: P = 1.43×10-7; Finnish-ancestry Epi25: P = 3.11×10-4; UK Biobank and Vanderbilt biorepository meta-analysis: P = 7.99×10-4). FE-PRS were significantly higher in patients with focal epilepsy compared to controls in the non-Finnish, non-biobank cohorts (Epi25: P = 5.74×10-19; Cleveland: P = 1.69×10-6). European ancestry-derived PRS did not predict generalized epilepsy or focal epilepsy in Japanese-ancestry individuals. Finally, we observed a significant 4.6-fold and a 4.5-fold enrichment of patients with generalized epilepsy compared to controls in the top 0.5% highest GE-PRS of the two non-Finnish European cohorts (Epi25: P = 2.60×10-15; Cleveland: P = 1.39×10-2). We conclude that common variant risk associated with epilepsy is significantly enriched in multiple cohorts of patients with epilepsy compared to controls-in particular for generalized epilepsy. As sample sizes and PRS accuracy continue to increase with further common variant discovery, PRS could complement established clinical biomarkers and augment genetic testing for patient classification, comorbidity research, and potentially targeted treatment.
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    Unstable TTTTA/TTTCA expansions in MARCH6 are associated with Familial Adult Myoclonic Epilepsy type 3
    Florian, RT ; Kraft, F ; Leitao, E ; Kaya, S ; Klebe, S ; Magnin, E ; van Rootselaar, A-F ; Buratti, J ; Kuehnel, T ; Schroeder, C ; Giesselmann, S ; Tschernoster, N ; Altmueller, J ; lamiral, A ; Keren, B ; Nava, C ; Bouteiller, D ; Forlani, S ; Jornea, L ; Kubica, R ; Ye, T ; Plassard, D ; Jost, B ; Meyer, V ; Deleuze, J-F ; Delpu, Y ; Avarello, MDM ; Vijfhuizen, LS ; Rudolf, G ; Hirsch, E ; Kroes, T ; Reif, PS ; Rosenow, F ; Ganos, C ; Vidailhet, M ; Thivard, L ; Mathieu, A ; Bourgeron, T ; Kurth, I ; Rafehi, H ; Steenpass, L ; Horsthemke, B ; Berkovic, SF ; Bisulli, F ; Brancati, F ; Canafoglia, L ; Casari, G ; Guerrini, R ; Ishiura, H ; Licchetta, L ; Mei, D ; Pippucci, T ; Sadleir, L ; Scheffer, IE ; Striano, P ; Tinuper, P ; Tsuji, S ; Zara, F ; LeGuern, E ; Klein, KM ; Labauge, P ; Bennett, MF ; Bahlo, M ; Gecz, J ; Corbett, MA ; Tijssen, MAJ ; van den Maagdenberg, AMJM ; Depienne, C (NATURE PUBLISHING GROUP, 2019-10-29)
    Familial Adult Myoclonic Epilepsy (FAME) is a genetically heterogeneous disorder characterized by cortical tremor and seizures. Intronic TTTTA/TTTCA repeat expansions in SAMD12 (FAME1) are the main cause of FAME in Asia. Using genome sequencing and repeat-primed PCR, we identify another site of this repeat expansion, in MARCH6 (FAME3) in four European families. Analysis of single DNA molecules with nanopore sequencing and molecular combing show that expansions range from 3.3 to 14 kb on average. However, we observe considerable variability in expansion length and structure, supporting the existence of multiple expansion configurations in blood cells and fibroblasts of the same individual. Moreover, the largest expansions are associated with micro-rearrangements occurring near the expansion in 20% of cells. This study provides further evidence that FAME is caused by intronic TTTTA/TTTCA expansions in distinct genes and reveals that expansions exhibit an unexpectedly high somatic instability that can ultimately result in genomic rearrangements.
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    Intronic ATTTC repeat expansions in STARD7 in familial adult myoclonic epilepsy linked to chromosome 2
    Corbett, MA ; Kroes, T ; Veneziano, L ; Bennett, MF ; Florian, R ; Schneider, AL ; Coppola, A ; Licchetta, L ; Franceschetti, S ; Suppa, A ; Wenger, A ; Mei, D ; Pendziwiat, M ; Kaya, S ; Delledonne, M ; Straussberg, R ; Xumerle, L ; Regan, B ; Crompton, D ; van Rootselaar, A-F ; Correll, A ; Catford, R ; Bisulli, F ; Chakraborty, S ; Baldassari, S ; Tinuper, P ; Barton, K ; Carswell, S ; Smith, M ; Berardelli, A ; Carroll, R ; Gardner, A ; Friend, KL ; Blatt, I ; Iacomino, M ; Di Bonaventura, C ; Striano, S ; Buratti, J ; Keren, B ; Nava, C ; Forlani, S ; Rudolf, G ; Hirsch, E ; Leguern, E ; Labauge, P ; Balestrini, S ; Sander, JW ; Afawi, Z ; Helbig, I ; Ishiura, H ; Tsuji, S ; Sisodiya, SM ; Casari, G ; Sadleir, LG ; van Coller, R ; Tijssen, MAJ ; Klein, KM ; van den Maagdenberg, AMJM ; Zara, F ; Guerrini, R ; Berkovic, SF ; Pippucci, T ; Canafoglia, L ; Bahlo, M ; Striano, P ; Scheffer, IE ; Brancati, F ; Depienne, C ; Gecz, J (NATURE PUBLISHING GROUP, 2019-10-29)
    Familial Adult Myoclonic Epilepsy (FAME) is characterised by cortical myoclonic tremor usually from the second decade of life and overt myoclonic or generalised tonic-clonic seizures. Four independent loci have been implicated in FAME on chromosomes (chr) 2, 3, 5 and 8. Using whole genome sequencing and repeat primed PCR, we provide evidence that chr2-linked FAME (FAME2) is caused by an expansion of an ATTTC pentamer within the first intron of STARD7. The ATTTC expansions segregate in 158/158 individuals typically affected by FAME from 22 pedigrees including 16 previously reported families recruited worldwide. RNA sequencing from patient derived fibroblasts shows no accumulation of the AUUUU or AUUUC repeat sequences and STARD7 gene expression is not affected. These data, in combination with other genes bearing similar mutations that have been implicated in FAME, suggest ATTTC expansions may cause this disorder, irrespective of the genomic locus involved.
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    Genome-wide mega-analysis identifies 16 loci and highlights diverse biological mechanisms in the common epilepsies
    Abou-Khalil, B ; Auce, P ; Avbersek, A ; Bahlo, M ; Balding, DJ ; Bast, T ; Baum, L ; Becker, AJ ; Becker, F ; Berghuis, B ; Berkovic, SF ; Boysen, KE ; Bradfield, JP ; Brody, LC ; Buono, RJ ; Campbell, E ; Cascino, GD ; Catarino, CB ; Cavalleri, GL ; Cherny, SS ; Chinthapalli, K ; Coffey, AJ ; Compston, A ; Coppola, A ; Cossette, P ; Craig, JJ ; de Haan, G-J ; De Jonghe, P ; de Kovel, CGF ; Delanty, N ; Depondt, C ; Devinsky, O ; Dlugos, DJ ; Doherty, CP ; Elger, CE ; Eriksson, JG ; Ferraro, TN ; Feucht, M ; Francis, B ; Franke, A ; French, JA ; Freytag, S ; Gaus, V ; Geller, EB ; Gieger, C ; Glauser, T ; Glynn, S ; Goldstein, DB ; Gui, H ; Guo, Y ; Haas, KF ; Hakonarson, H ; Hallmann, K ; Haut, S ; Heinzen, EL ; Helbig, I ; Hengsbach, C ; Hjalgrim, H ; Iacomino, M ; Ingason, A ; Jamnadas-Khoda, J ; Johnson, MR ; Kalviainen, R ; Kantanen, A-M ; Kasperaviciute, D ; Trenite, DK-N ; Kirsch, HE ; Knowlton, RC ; Koeleman, BPC ; Krause, R ; Krenn, M ; Kunz, WS ; Kuzniecky, R ; Kwan, P ; Lal, D ; Lau, Y-L ; Lehesjoki, A-E ; Lerche, H ; Leu, C ; Lieb, W ; Lindhout, D ; Lo, WD ; Lopes-Cendes, I ; Lowenstein, DH ; Malovini, A ; Marson, AG ; Mayer, T ; McCormack, M ; Mills, JL ; Mirza, N ; Moerzinger, M ; Moller, RS ; Molloy, AM ; Muhle, H ; Newton, M ; Ng, P-W ; Noethen, MM ; Nuernberg, P ; O'Brien, TJ ; Oliver, KL ; Palotie, A ; Pangilinan, F ; Peter, S ; Petrovski, S ; Poduri, A ; Privitera, M ; Radtke, R ; Rau, S ; Reif, PS ; Reinthaler, EM ; Rosenow, F ; Sander, JW ; Sander, T ; Scattergood, T ; Schachter, SC ; Schankin, CJ ; Scheffer, IE ; Schmitz, B ; Schoch, S ; Sham, PC ; Shih, JJ ; Sills, GJ ; Sisodiya, SM ; Slattery, L ; Smith, A ; Smith, DF ; Smith, MC ; Smith, PE ; Sonsma, ACM ; Speed, D ; Sperling, MR ; Steinhoff, BJ ; Stephani, U ; Stevelink, R ; Strauch, K ; Striano, P ; Stroink, H ; Surges, R ; Tan, KM ; Thio, LL ; Thomas, GN ; Todaro, M ; Tozzi, R ; Vari, MS ; Vining, EPG ; Visscher, F ; von Spiczak, S ; Walley, NM ; Weber, YG ; Wei, Z ; Weisenberg, J ; Whelan, CD ; Widdess-Walsh, P ; Wolff, M ; Wolking, S ; Yang, W ; Zara, F ; Zimprich, F (NATURE PUBLISHING GROUP, 2018-12-10)
    The epilepsies affect around 65 million people worldwide and have a substantial missing heritability component. We report a genome-wide mega-analysis involving 15,212 individuals with epilepsy and 29,677 controls, which reveals 16 genome-wide significant loci, of which 11 are novel. Using various prioritization criteria, we pinpoint the 21 most likely epilepsy genes at these loci, with the majority in genetic generalized epilepsies. These genes have diverse biological functions, including coding for ion-channel subunits, transcription factors and a vitamin-B6 metabolism enzyme. Converging evidence shows that the common variants associated with epilepsy play a role in epigenetic regulation of gene expression in the brain. The results show an enrichment for monogenic epilepsy genes as well as known targets of antiepileptic drugs. Using SNP-based heritability analyses we disentangle both the unique and overlapping genetic basis to seven different epilepsy subtypes. Together, these findings provide leads for epilepsy therapies based on underlying pathophysiology.
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    Dominant KCNA2 mutation causes episodic ataxia and pharmacoresponsive epilepsy
    Corbett, MA ; Bellows, ST ; Li, M ; Carroll, R ; Micallef, S ; Carvill, GL ; Myers, CT ; Howell, KB ; Maljevic, S ; Lerche, H ; Gazina, EV ; Mefford, HC ; Bahlo, M ; Berkovic, SF ; Petrou, S ; Scheffer, IE ; Gecz, J (LIPPINCOTT WILLIAMS & WILKINS, 2016-11-08)
    OBJECTIVE: To identify the genetic basis of a family segregating episodic ataxia, infantile seizures, and heterogeneous epilepsies and to study the phenotypic spectrum of KCNA2 mutations. METHODS: A family with 7 affected individuals over 3 generations underwent detailed phenotyping. Whole genome sequencing was performed on a mildly affected grandmother and her grandson with epileptic encephalopathy (EE). Segregating variants were filtered and prioritized based on functional annotations. The effects of the mutation on channel function were analyzed in vitro by voltage clamp assay and in silico by molecular modeling. KCNA2 was sequenced in 35 probands with heterogeneous phenotypes. RESULTS: The 7 family members had episodic ataxia (5), self-limited infantile seizures (5), evolving to genetic generalized epilepsy (4), focal seizures (2), and EE (1). They had a segregating novel mutation in the shaker type voltage-gated potassium channel KCNA2 (CCDS_827.1: c.765_773del; p.255_257del). A rare missense SCN2A (rs200884216) variant was also found in 2 affected siblings and their unaffected mother. The p.255_257del mutation caused dominant negative loss of channel function. Molecular modeling predicted repositioning of critical arginine residues in the voltage-sensing domain. KCNA2 sequencing revealed 1 de novo mutation (CCDS_827.1: c.890G>A; p.Arg297Gln) in a girl with EE, ataxia, and tremor. CONCLUSIONS: A KCNA2 mutation caused dominantly inherited episodic ataxia, mild infantile-onset seizures, and later generalized and focal epilepsies in the setting of normal intellect. This observation expands the KCNA2 phenotypic spectrum from EE often associated with chronic ataxia, reflecting the marked variation in severity observed in many ion channel disorders.
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    Multiplex families with epilepsy Success of clinical and molecular genetic characterization
    Afawi, Z ; Oliver, KL ; Kivity, S ; Mazarib, A ; Blatt, I ; Neufeld, MY ; Helbig, KL ; Goldberg-Stern, H ; Misk, AJ ; Straussberg, R ; Walid, S ; Mahajnah, M ; Lerman-Sagie, T ; Ben-Zeev, B ; Kahana, E ; Masalha, R ; Kramer, U ; Ekstein, D ; Shorer, Z ; Wallace, RH ; Mangelsdorf, M ; MacPherson, JN ; Carvill, GL ; Mefford, HC ; Jackson, GD ; Scheffer, IE ; Bahlo, M ; Gecz, J ; Heron, SE ; Corbett, M ; Mulley, JC ; Dibbens, LM ; Korczyn, AD ; Berkovic, SF (LIPPINCOTT WILLIAMS & WILKINS, 2016-02-23)
    OBJECTIVE: To analyze the clinical syndromes and inheritance patterns of multiplex families with epilepsy toward the ultimate aim of uncovering the underlying molecular genetic basis. METHODS: Following the referral of families with 2 or more relatives with epilepsy, individuals were classified into epilepsy syndromes. Families were classified into syndromes where at least 2 family members had a specific diagnosis. Pedigrees were analyzed and molecular genetic studies were performed as appropriate. RESULTS: A total of 211 families were ascertained over an 11-year period in Israel. A total of 169 were classified into broad familial epilepsy syndrome groups: 61 generalized, 22 focal, 24 febrile seizure syndromes, 33 special syndromes, and 29 mixed. A total of 42 families remained unclassified. Pathogenic variants were identified in 49/211 families (23%). The majority were found in established epilepsy genes (e.g., SCN1A, KCNQ2, CSTB), but in 11 families, this cohort contributed to the initial discovery (e.g., KCNT1, PCDH19, TBC1D24). We expand the phenotypic spectrum of established epilepsy genes by reporting a familial LAMC3 homozygous variant, where the predominant phenotype was epilepsy with myoclonic-atonic seizures, and a pathogenic SCN1A variant in a family where in 5 siblings the phenotype was broadly consistent with Dravet syndrome, a disorder that usually occurs sporadically. CONCLUSION: A total of 80% of families were successfully classified, with pathogenic variants identified in 23%. The successful characterization of familial electroclinical and inheritance patterns has highlighted the value of studying multiplex families and their contribution towards uncovering the genetic basis of the epilepsies.