Zebrafish knockout of Down syndrome gene, DYRK1A, shows social impairments relevant to autism

Oc Hee Kim; Hyun Ju Cho; Enna Han; Ted Inpyo Hong; Krishan Ariyasiri; Jung Hwa Choi; Kyu Seok Hwang; Yun Mi Jeong; Se Yeol Yang; Kweon Yu; Doo Sang Park; Hyun Woo Oh; Erica E. Davis; Charles E. Schwartz; Jeong Soo Lee; Hyung Goo Kim; Cheol Hee Kim

doi:10.1186/s13229-017-0168-2

Zebrafish knockout of Down syndrome gene, DYRK1A, shows social impairments relevant to autism

Oc Hee Kim, Hyun Ju Cho, Enna Han, Ted Inpyo Hong, Krishan Ariyasiri, Jung Hwa Choi, Kyu Seok Hwang, Yun Mi Jeong, Se Yeol Yang, Kweon Yu, Doo Sang Park, Hyun Woo Oh, Erica E. Davis, Charles E. Schwartz, Jeong Soo Lee, Hyung Goo Kim, Cheol Hee Kim

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

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Abstract

Background: DYRK1A maps to the Down syndrome critical region at 21q22. Mutations in this kinase-encoding gene have been reported to cause microcephaly associated with either intellectual disability or autism in humans. Intellectual disability accompanied by microcephaly was recapitulated in a murine model by overexpressing Dyrk1a which mimicked Down syndrome phenotypes. However, given embryonic lethality in homozygous knockout (KO) mice, no murine model studies could present sufficient evidence to link Dyrk1a dysfunction with autism. To understand the molecular mechanisms underlying microcephaly and autism spectrum disorders (ASD), we established an in vivo dyrk1aa KO model using zebrafish. Methods: We identified a patient with a mutation in the DYRK1A gene using microarray analysis. Circumventing the barrier of murine model studies, we generated a dyrk1aa KO zebrafish using transcription activator-like effector nuclease (TALEN)-mediated genome editing. For social behavioral tests, we have established a social interaction test, shoaling assay, and group behavior assay. For molecular analysis, we examined the neuronal activity in specific brain regions of dyrk1aa KO zebrafish through in situ hybridization with various probes including c-fos and crh which are the molecular markers for stress response. Results: Microarray detected an intragenic microdeletion of DYRK1A in an individual with microcephaly and autism. From behavioral tests of social interaction and group behavior, dyrk1aa KO zebrafish exhibited social impairments that reproduce human phenotypes of autism in a vertebrate animal model. Social impairment in dyrk1aa KO zebrafish was further confirmed by molecular analysis of c-fos and crh expression. Transcriptional expression of c-fos and crh was lower than that of wild type fish in specific hypothalamic regions, suggesting that KO fish brains are less activated by social context. Conclusions: In this study, we established a zebrafish model to validate a candidate gene for autism in a vertebrate animal. These results illustrate the functional deficiency of DYRK1A as an underlying disease mechanism for autism. We also propose simple social behavioral assays as a tool for the broader study of autism candidate genes.

Original language	English (US)
Article number	168
Journal	Molecular Autism
Volume	8
Issue number	1
DOIs	https://doi.org/10.1186/s13229-017-0168-2
State	Published - Sep 29 2017
Externally published	Yes

Keywords

Autism
DYRK1A
Down syndrome
Group behavior
Knockout
Shoaling
Social interaction
Zebrafish

ASJC Scopus subject areas

Molecular Biology
Developmental Neuroscience
Developmental Biology
Psychiatry and Mental health

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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10.1186/s13229-017-0168-2

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Kim, O. H., Cho, H. J., Han, E., Hong, T. I., Ariyasiri, K., Choi, J. H., Hwang, K. S., Jeong, Y. M., Yang, S. Y., Yu, K., Park, D. S., Oh, H. W., Davis, E. E., Schwartz, C. E., Lee, J. S., Kim, H. G., & Kim, C. H. (2017). Zebrafish knockout of Down syndrome gene, DYRK1A, shows social impairments relevant to autism. Molecular Autism, 8(1), Article 168. https://doi.org/10.1186/s13229-017-0168-2

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abstract = "Background: DYRK1A maps to the Down syndrome critical region at 21q22. Mutations in this kinase-encoding gene have been reported to cause microcephaly associated with either intellectual disability or autism in humans. Intellectual disability accompanied by microcephaly was recapitulated in a murine model by overexpressing Dyrk1a which mimicked Down syndrome phenotypes. However, given embryonic lethality in homozygous knockout (KO) mice, no murine model studies could present sufficient evidence to link Dyrk1a dysfunction with autism. To understand the molecular mechanisms underlying microcephaly and autism spectrum disorders (ASD), we established an in vivo dyrk1aa KO model using zebrafish. Methods: We identified a patient with a mutation in the DYRK1A gene using microarray analysis. Circumventing the barrier of murine model studies, we generated a dyrk1aa KO zebrafish using transcription activator-like effector nuclease (TALEN)-mediated genome editing. For social behavioral tests, we have established a social interaction test, shoaling assay, and group behavior assay. For molecular analysis, we examined the neuronal activity in specific brain regions of dyrk1aa KO zebrafish through in situ hybridization with various probes including c-fos and crh which are the molecular markers for stress response. Results: Microarray detected an intragenic microdeletion of DYRK1A in an individual with microcephaly and autism. From behavioral tests of social interaction and group behavior, dyrk1aa KO zebrafish exhibited social impairments that reproduce human phenotypes of autism in a vertebrate animal model. Social impairment in dyrk1aa KO zebrafish was further confirmed by molecular analysis of c-fos and crh expression. Transcriptional expression of c-fos and crh was lower than that of wild type fish in specific hypothalamic regions, suggesting that KO fish brains are less activated by social context. Conclusions: In this study, we established a zebrafish model to validate a candidate gene for autism in a vertebrate animal. These results illustrate the functional deficiency of DYRK1A as an underlying disease mechanism for autism. We also propose simple social behavioral assays as a tool for the broader study of autism candidate genes.",

keywords = "Autism, DYRK1A, Down syndrome, Group behavior, Knockout, Shoaling, Social interaction, Zebrafish",

author = "Kim, {Oc Hee} and Cho, {Hyun Ju} and Enna Han and Hong, {Ted Inpyo} and Krishan Ariyasiri and Choi, {Jung Hwa} and Hwang, {Kyu Seok} and Jeong, {Yun Mi} and Yang, {Se Yeol} and Kweon Yu and Park, {Doo Sang} and Oh, {Hyun Woo} and Davis, {Erica E.} and Schwartz, {Charles E.} and Lee, {Jeong Soo} and Kim, {Hyung Goo} and Kim, {Cheol Hee}",

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year = "2017",

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day = "29",

doi = "10.1186/s13229-017-0168-2",

language = "English (US)",

volume = "8",

journal = "Molecular Autism",

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T1 - Zebrafish knockout of Down syndrome gene, DYRK1A, shows social impairments relevant to autism

AU - Kim, Oc Hee

AU - Cho, Hyun Ju

AU - Han, Enna

AU - Hong, Ted Inpyo

AU - Ariyasiri, Krishan

AU - Choi, Jung Hwa

AU - Hwang, Kyu Seok

AU - Jeong, Yun Mi

AU - Yang, Se Yeol

AU - Yu, Kweon

AU - Park, Doo Sang

AU - Oh, Hyun Woo

AU - Davis, Erica E.

AU - Schwartz, Charles E.

AU - Lee, Jeong Soo

AU - Kim, Hyung Goo

AU - Kim, Cheol Hee

PY - 2017/9/29

Y1 - 2017/9/29

N2 - Background: DYRK1A maps to the Down syndrome critical region at 21q22. Mutations in this kinase-encoding gene have been reported to cause microcephaly associated with either intellectual disability or autism in humans. Intellectual disability accompanied by microcephaly was recapitulated in a murine model by overexpressing Dyrk1a which mimicked Down syndrome phenotypes. However, given embryonic lethality in homozygous knockout (KO) mice, no murine model studies could present sufficient evidence to link Dyrk1a dysfunction with autism. To understand the molecular mechanisms underlying microcephaly and autism spectrum disorders (ASD), we established an in vivo dyrk1aa KO model using zebrafish. Methods: We identified a patient with a mutation in the DYRK1A gene using microarray analysis. Circumventing the barrier of murine model studies, we generated a dyrk1aa KO zebrafish using transcription activator-like effector nuclease (TALEN)-mediated genome editing. For social behavioral tests, we have established a social interaction test, shoaling assay, and group behavior assay. For molecular analysis, we examined the neuronal activity in specific brain regions of dyrk1aa KO zebrafish through in situ hybridization with various probes including c-fos and crh which are the molecular markers for stress response. Results: Microarray detected an intragenic microdeletion of DYRK1A in an individual with microcephaly and autism. From behavioral tests of social interaction and group behavior, dyrk1aa KO zebrafish exhibited social impairments that reproduce human phenotypes of autism in a vertebrate animal model. Social impairment in dyrk1aa KO zebrafish was further confirmed by molecular analysis of c-fos and crh expression. Transcriptional expression of c-fos and crh was lower than that of wild type fish in specific hypothalamic regions, suggesting that KO fish brains are less activated by social context. Conclusions: In this study, we established a zebrafish model to validate a candidate gene for autism in a vertebrate animal. These results illustrate the functional deficiency of DYRK1A as an underlying disease mechanism for autism. We also propose simple social behavioral assays as a tool for the broader study of autism candidate genes.

AB - Background: DYRK1A maps to the Down syndrome critical region at 21q22. Mutations in this kinase-encoding gene have been reported to cause microcephaly associated with either intellectual disability or autism in humans. Intellectual disability accompanied by microcephaly was recapitulated in a murine model by overexpressing Dyrk1a which mimicked Down syndrome phenotypes. However, given embryonic lethality in homozygous knockout (KO) mice, no murine model studies could present sufficient evidence to link Dyrk1a dysfunction with autism. To understand the molecular mechanisms underlying microcephaly and autism spectrum disorders (ASD), we established an in vivo dyrk1aa KO model using zebrafish. Methods: We identified a patient with a mutation in the DYRK1A gene using microarray analysis. Circumventing the barrier of murine model studies, we generated a dyrk1aa KO zebrafish using transcription activator-like effector nuclease (TALEN)-mediated genome editing. For social behavioral tests, we have established a social interaction test, shoaling assay, and group behavior assay. For molecular analysis, we examined the neuronal activity in specific brain regions of dyrk1aa KO zebrafish through in situ hybridization with various probes including c-fos and crh which are the molecular markers for stress response. Results: Microarray detected an intragenic microdeletion of DYRK1A in an individual with microcephaly and autism. From behavioral tests of social interaction and group behavior, dyrk1aa KO zebrafish exhibited social impairments that reproduce human phenotypes of autism in a vertebrate animal model. Social impairment in dyrk1aa KO zebrafish was further confirmed by molecular analysis of c-fos and crh expression. Transcriptional expression of c-fos and crh was lower than that of wild type fish in specific hypothalamic regions, suggesting that KO fish brains are less activated by social context. Conclusions: In this study, we established a zebrafish model to validate a candidate gene for autism in a vertebrate animal. These results illustrate the functional deficiency of DYRK1A as an underlying disease mechanism for autism. We also propose simple social behavioral assays as a tool for the broader study of autism candidate genes.

KW - Autism

KW - DYRK1A

KW - Down syndrome

KW - Group behavior

KW - Knockout

KW - Shoaling

KW - Social interaction

KW - Zebrafish

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Zebrafish knockout of Down syndrome gene, DYRK1A, shows social impairments relevant to autism

Abstract

Keywords

ASJC Scopus subject areas

UN SDGs

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