Ptchd1 deficiency induces excitatory synaptic and cognitive dysfunctions in mouse

Ung, Dévina C.; Iacono, Giovanni; Méziane, Hamid; Blanchard, Edward; Papon, M-A; Selten, Martijn; Rhijn, J-R van; Montjean, Rodrick; Rucci, Julien; Martin, Stéphane; Fleet, Andrew; Birling, Marie‐Christine; Marouillat, Sylviane; Roepman, Ronald; Selloum, Mohammed; Lux, Aline; Thépault, R-A; Hamel, Paul A.; Mittal, Kirti; Vincent, John B.; Dorseuil, Olivier; Stunnenberg, Henk; Billuart, Pierre; Kasri, Nael Nadif; Hérault, Yann; Laumonnier, Frédéric

doi:10.1038/mp.2017.39

Cited by 68 publications

(87 citation statements)

References 47 publications

(76 reference statements)

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“…The first dataset we assessed was obtained from Ptchd1 -KO mice. Loss-of-function mutations in the PTCHD1 gene lead to X-linked intellectual disability (OMIM # 300830) ( Ung et al, 2017 ). We found that nearly 23% (185 genes) of the genes that are downregulated in the hippocampus of Ptchd1 -KO mice are amongst the genes that increase following DBS in WT mice ( Figure 7A ).…”

Section: Resultsmentioning

confidence: 99%

“…Limma ( Ritchie et al, 2015 ), a R package was used for differential expression analysis and genes with FDR < 0.05 and absolute logFC >0 were called as differentially expressed and were used for further analysis. For Intellectual Disorder, we used list of differentially expressed downregulated genes from the following studies ( Mehmood et al, 2011 ; Ung et al, 2017 ).…”

Section: Methodsmentioning

confidence: 99%

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Forniceal deep brain stimulation induces gene expression and splicing changes that promote neurogenesis and plasticity

Pohodich

Yalamanchili

Raman

et al. 2018

eLife

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Clinical trials are currently underway to assess the efficacy of forniceal deep brain stimulation (DBS) for improvement of memory in Alzheimer’s patients, and forniceal DBS has been shown to improve learning and memory in a mouse model of Rett syndrome (RTT), an intellectual disability disorder caused by loss-of-function mutations in MECP2. The mechanism of DBS benefits has been elusive, however, so we assessed changes in gene expression, splice isoforms, DNA methylation, and proteome following acute forniceal DBS in wild-type mice and mice lacking Mecp2. We found that DBS upregulates genes involved in synaptic function, cell survival, and neurogenesis and normalized expression of ~25% of the genes altered in Mecp2-null mice. Moreover, DBS induced expression of 17–24% of the genes downregulated in other intellectual disability mouse models and in post-mortem human brain tissue from patients with Major Depressive Disorder, suggesting forniceal DBS could benefit individuals with a variety of neuropsychiatric disorders.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Forniceal deep brain stimulation induces gene expression and splicing changes that promote neurogenesis and plasticity

Pohodich

Yalamanchili

Raman

et al. 2018

eLife

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“…In situ hybridization and PCR analysis. In situ hybridizations with chromogenic detection were done using digoxigenin-labeled cRNA probes and were performed as described previously (Schaeren-Wiemers and Gerfin-Moser, 1993). The DNA fragment encoding the Ptchd1 probe contained SP6 and T7 promoters flanking the 5Ј-or 3Ј-end, respectively: Ptchd1:CCGCTCTGCTCTAGGATGCTGCGGCAGGTTCTGCACAGG GGCTTGAGGACGTGTTTCTCCCGGCTTGGCCACTTCATTGCCA GTCACCCGGTCTTCTTTGCTTCGGCGCCGGTGCTCATCTCCAT CCTGCTCGGCGCCAGCTTCAGCCGCTACCAGGTCGAAGAGAGC GTGGAGCACCTGCTGGCGCCCCAGCACAGCCTAGCCAAGATCG AGCGCAACCTAGTCAACAGCCTCTTCCCGGTCAACCGCTCCAAG CACCGGCTCTACTCGGACCTGCAGACCCCTGGGCGCTACGGCC GGGTCATTGTCACCTCCTACCAGAAAGCCAACATGCTAGACC AACATCACACGGACCTGA.…”

Section: Methodsmentioning

confidence: 99%

Cellular Functions of the Autism Risk Factor PTCHD1 in Mice

et al. 2017

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The gene () is mutated in patients with autism spectrum disorders and intellectual disabilities and has been hypothesized to contribute to Sonic hedgehog (Shh) signaling and synapse formation. We identify a panel of Ptchd1-interacting proteins that include postsynaptic density proteins and the retromer complex, revealing a link to critical regulators of dendritic and postsynaptic trafficking. knock-out (KO) male mice exhibit cognitive alterations, including defects in a novel object recognition task. To test whether Ptchd1 is required for Shh-dependent signaling, we examined two Shh-dependent cell populations that express high levels of mRNA: cerebellar granule cell precursors and dentate granule cells in the hippocampus. We found that proliferation of these neuronal precursors was not altered significantly in KO male mice. We used whole-cell electrophysiology and anatomical methods to assess synaptic function in Ptchd1-deficient dentate granule cells. In the absence of Ptchd1, we observed profound disruption in excitatory/inhibitory balance despite normal dendritic spine density on dentate granule cells. These findings support a critical role of the Ptchd1 protein in the dentate gyrus, but indicate that it is not required for structural synapse formation in dentate granule cells or for Shh-dependent neuronal precursor proliferation. The mechanisms underlying neuronal and cellular alterations resulting from () gene mutations are unknown. The results from this study support an association with dendritic trafficking complexes of Ptchd1. Loss-of-function experiments do not support a role in sonic hedgehog-dependent signaling, but reveal a disruption of synaptic transmission in the mouse dentate gyrus. The findings will help to guide ongoing efforts to understand the etiology of neurodevelopmental disorders arising from Ptchd1 deficiency.

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“…PTCHD1 encodes a transmembrane protein with a patched domain, and its involvement in neurodevelopmental disorders is supported by microdeletions and frameshift mutations in individuals with neurodevelopmental delay (NDD), intellectual disability, and ASD (15)(16)(17)(18)(19)(20)(21). However, recently described Ptchd1 mutant mice had impairments in attention and cognition (22)(23)(24) but did not overtly exhibit ASD-associated behaviors. Also, many ASDassociated PTCHD1 locus microdeletions are upstream of the PTCHD1 protein-coding gene and disrupt exons of the neighboring brain-enriched long noncoding RNA (lncRNA) PTCHD1-AS (15).…”

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confidence: 99%

Synaptic Dysfunction in Human Neurons With Autism-Associated Deletions in PTCHD1-AS

Ross

Zhang

Mok

et al. 2020

Biological Psychiatry

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BACKGROUND: The Xp22.11 locus that encompasses PTCHD1, DDX53, and the long noncoding RNA PTCHD1-AS is frequently disrupted in male subjects with autism spectrum disorder (ASD), but the functional consequences of these genetic risk factors for ASD are unknown. METHODS: To evaluate the functional consequences of PTCHD1 locus deletions, we generated induced pluripotent stem cells (iPSCs) from unaffected control subjects and 3 subjects with ASD with microdeletions affecting PTCHD1-AS/PTCHD1, PTCHD1-AS/DDX53, or PTCHD1-AS alone. Function of iPSC-derived cortical neurons was assessed using molecular approaches and electrophysiology. We also compiled novel and known genetic variants of the PTCHD1 locus to explore the roles of PTCHD1 and PTCHD1-AS in genetic risk for ASD and other neurodevelopmental disorders. Finally, genome editing was used to explore the functional consequences of deleting a single conserved exon of PTCHD1-AS. RESULTS: iPSC-derived neurons from subjects with ASD exhibited reduced miniature excitatory postsynaptic current frequency and N-methyl-D-aspartate receptor hypofunction. We found that 35 ASD-associated deletions mapping to the PTCHD1 locus disrupted exons of PTCHD1-AS. We also found a novel ASD-associated deletion of PTCHD1-AS exon 3 and showed that exon 3 loss altered PTCHD1-AS splicing without affecting expression of the neighboring PTCHD1 coding gene. Finally, targeted disruption of PTCHD1-AS exon 3 recapitulated diminished miniature excitatory postsynaptic current frequency, supporting a role for the long noncoding RNA in the etiology of ASD. CONCLUSIONS: Our genetic findings provide strong evidence that PTCHD1-AS deletions are risk factors for ASD, and human iPSC-derived neurons implicate these deletions in the neurophysiology of excitatory synapses and in ASD-associated synaptic impairment.

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Ptchd1 deficiency induces excitatory synaptic and cognitive dysfunctions in mouse

Cited by 68 publications

References 47 publications

Forniceal deep brain stimulation induces gene expression and splicing changes that promote neurogenesis and plasticity

Forniceal deep brain stimulation induces gene expression and splicing changes that promote neurogenesis and plasticity

Cellular Functions of the Autism Risk Factor PTCHD1 in Mice

Synaptic Dysfunction in Human Neurons With Autism-Associated Deletions in PTCHD1-AS

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