A CACNB4 mutation shows that altered Cav2.1 function may be a genetic modifier of severe myoclonic epilepsy in infancy

Iori Ohmori; Mamoru Ouchida; Takafumi Miki; Nobuyoshi Mimaki; Shigeki Kiyonaka; Tei-ichi Nishiki; Kazuhito Tomizawa; Yasuo Mori; Hideki Matsui

doi:10.1016/j.nbd.2008.07.017

A CACNB4 mutation shows that altered Ca_v2.1 function may be a genetic modifier of severe myoclonic epilepsy in infancy

Iori Ohmori, Mamoru Ouchida, Takafumi Miki, Nobuyoshi Mimaki, Shigeki Kiyonaka, Tei-ichi Nishiki, Kazuhito Tomizawa, Yasuo Mori, Hideki Matsui

Research output: Contribution to journal › Article › peer-review

49 Citations (Scopus)

Abstract

Mutations of SCN1A, encoding the voltage-gated sodium channel α1 subunit, represent the most frequent genetic cause of severe myoclonic epilepsy in infancy (SMEI). The purpose of this study was to determine if mutations in other seizure susceptibility genes are also present and could modify the disease severity. All coding exons of SCN1B, GABRG2, and CACNB4 genes were screened for mutations in 38 SCN1A-mutation-positive SMEI probands. We identified one proband who was heterozygous for a de novo SCN1A nonsense mutation (R568X) and another missense mutation (R468Q) of the CACNB4 gene. The latter mutation was inherited from his father who had a history of febrile seizures. An electrophysiological analysis of heterologous expression system exhibited that R468Q-CACNB4 showed greater Ba²⁺ current density compared with the wild-type CACNB4. The greater Ca_v2.1 currents caused by the R468Q-CACNB4 mutation may increase the neurotransmitter release in the excitatory neurons under the condition of insufficient inhibitory neurons caused primarily by the SCN1A mutation.

Original language	English
Pages (from-to)	349-354
Number of pages	6
Journal	Neurobiology of Disease
Volume	32
Issue number	3
DOIs	https://doi.org/10.1016/j.nbd.2008.07.017
Publication status	Published - Dec 2008

Keywords

CACNB4
Dravet syndrome
Genetic modifier
SCN1A
Severe myoclonic epilepsy in infancy

ASJC Scopus subject areas

Neurology

Access to Document

10.1016/j.nbd.2008.07.017

Cite this

@article{2d11ab28984b44f587e6ff1f99f22b7c,

title = "A CACNB4 mutation shows that altered Cav2.1 function may be a genetic modifier of severe myoclonic epilepsy in infancy",

abstract = "Mutations of SCN1A, encoding the voltage-gated sodium channel α1 subunit, represent the most frequent genetic cause of severe myoclonic epilepsy in infancy (SMEI). The purpose of this study was to determine if mutations in other seizure susceptibility genes are also present and could modify the disease severity. All coding exons of SCN1B, GABRG2, and CACNB4 genes were screened for mutations in 38 SCN1A-mutation-positive SMEI probands. We identified one proband who was heterozygous for a de novo SCN1A nonsense mutation (R568X) and another missense mutation (R468Q) of the CACNB4 gene. The latter mutation was inherited from his father who had a history of febrile seizures. An electrophysiological analysis of heterologous expression system exhibited that R468Q-CACNB4 showed greater Ba2+ current density compared with the wild-type CACNB4. The greater Cav2.1 currents caused by the R468Q-CACNB4 mutation may increase the neurotransmitter release in the excitatory neurons under the condition of insufficient inhibitory neurons caused primarily by the SCN1A mutation.",

keywords = "CACNB4, Dravet syndrome, Genetic modifier, SCN1A, Severe myoclonic epilepsy in infancy",

author = "Iori Ohmori and Mamoru Ouchida and Takafumi Miki and Nobuyoshi Mimaki and Shigeki Kiyonaka and Tei-ichi Nishiki and Kazuhito Tomizawa and Yasuo Mori and Hideki Matsui",

note = "Funding Information: We are grateful to Dr. AL George Jr. for helpful suggestions. We also thank Drs. H. Yoshinaga and Y. Ohtsuka for referring patients. This work was supported by Grant-in-Aids from the Ministry of Education, Culture, Sports, Science and Technology (Grant Nos. 18591154 to I.O. and 15591110 to M.O.).",

year = "2008",

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doi = "10.1016/j.nbd.2008.07.017",

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volume = "32",

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T1 - A CACNB4 mutation shows that altered Cav2.1 function may be a genetic modifier of severe myoclonic epilepsy in infancy

AU - Ohmori, Iori

AU - Ouchida, Mamoru

AU - Miki, Takafumi

AU - Mimaki, Nobuyoshi

AU - Kiyonaka, Shigeki

AU - Nishiki, Tei-ichi

AU - Tomizawa, Kazuhito

AU - Mori, Yasuo

AU - Matsui, Hideki

N1 - Funding Information: We are grateful to Dr. AL George Jr. for helpful suggestions. We also thank Drs. H. Yoshinaga and Y. Ohtsuka for referring patients. This work was supported by Grant-in-Aids from the Ministry of Education, Culture, Sports, Science and Technology (Grant Nos. 18591154 to I.O. and 15591110 to M.O.).

PY - 2008/12

Y1 - 2008/12

N2 - Mutations of SCN1A, encoding the voltage-gated sodium channel α1 subunit, represent the most frequent genetic cause of severe myoclonic epilepsy in infancy (SMEI). The purpose of this study was to determine if mutations in other seizure susceptibility genes are also present and could modify the disease severity. All coding exons of SCN1B, GABRG2, and CACNB4 genes were screened for mutations in 38 SCN1A-mutation-positive SMEI probands. We identified one proband who was heterozygous for a de novo SCN1A nonsense mutation (R568X) and another missense mutation (R468Q) of the CACNB4 gene. The latter mutation was inherited from his father who had a history of febrile seizures. An electrophysiological analysis of heterologous expression system exhibited that R468Q-CACNB4 showed greater Ba2+ current density compared with the wild-type CACNB4. The greater Cav2.1 currents caused by the R468Q-CACNB4 mutation may increase the neurotransmitter release in the excitatory neurons under the condition of insufficient inhibitory neurons caused primarily by the SCN1A mutation.

AB - Mutations of SCN1A, encoding the voltage-gated sodium channel α1 subunit, represent the most frequent genetic cause of severe myoclonic epilepsy in infancy (SMEI). The purpose of this study was to determine if mutations in other seizure susceptibility genes are also present and could modify the disease severity. All coding exons of SCN1B, GABRG2, and CACNB4 genes were screened for mutations in 38 SCN1A-mutation-positive SMEI probands. We identified one proband who was heterozygous for a de novo SCN1A nonsense mutation (R568X) and another missense mutation (R468Q) of the CACNB4 gene. The latter mutation was inherited from his father who had a history of febrile seizures. An electrophysiological analysis of heterologous expression system exhibited that R468Q-CACNB4 showed greater Ba2+ current density compared with the wild-type CACNB4. The greater Cav2.1 currents caused by the R468Q-CACNB4 mutation may increase the neurotransmitter release in the excitatory neurons under the condition of insufficient inhibitory neurons caused primarily by the SCN1A mutation.

KW - CACNB4

KW - Dravet syndrome

KW - Genetic modifier

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KW - Severe myoclonic epilepsy in infancy

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