A toxic gain-of-function variant in MAPK8IP3 provides insights into JIP3 cellular roles
Wei Zhang, … , Konstantina Skourti-Stathaki, Stanley T. Crooke
Wei Zhang, … , Konstantina Skourti-Stathaki, Stanley T. Crooke
Published March 20, 2025
Citation Information: JCI Insight. 2025;10(8):e187199. https://doi.org/10.1172/jci.insight.187199.
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Research Article Cell biology Genetics Therapeutics

A toxic gain-of-function variant in MAPK8IP3 provides insights into JIP3 cellular roles

Abstract

Mitogen-activated protein kinase 8 interacting protein 3 (MAPK8IP3) gene encoding a protein called JIP3 is an adaption protein of the kinesin-1 complex known to play a role in axonal transport of cargo. Mutations in the gene have been linked to severe neurodevelopmental disorders, resulting in developmental delay, intellectual disability, ataxia, tremor, autism, seizures, and visual impairment. A patient who has a missense mutation in the MAPK8IP3 gene (c. 1714 C>T, Arg578Cys) (R578C) manifests dystonia, gross motor delay, and developmental delay. Here, we showed that the mutation was a toxic gain-of-function mutation that altered the interactome of JIP3; disrupted axonal transport of late endosomes; increased signaling via c-Jun N-terminal kinase, resulting in apoptosis; and disrupted dopamine receptor 1 signaling while not affecting dopamine receptor 2 signaling. Furthermore, in the presence of the mutant protein, we showed that an 80% reduction of mutant JIP3 and a 60% reduction of WT JIP3 by non-allele-selective phosphorothioate-modified antisense oligonucleotides was well tolerated by several types of cells in vitro. Our study identifies what we believe to be several important new roles for JIP3 and provides important insights for therapeutic approaches, including antisense oligonucleotide reduction of JIP3.

Authors

Wei Zhang, Swapnil Mittal, Ria Thomas, Anahid Foroughishafiei, Ricardo Nunes Bastos, Wendy K. Chung, Konstantina Skourti-Stathaki, Stanley T. Crooke

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Figure 5

Dopamine signaling was uncoupled in patient iPSC–derived neurons.

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Dopamine signaling was uncoupled in patient iPSC–derived neurons. (A) mR...
(A) mRNA levels of MAPK8IP3 (JIP3), DRD1, and DRD2 either in CRISPR control or patient iPSC–derived neurons were measured by qPCR. n = 3. *P < 0.05. (B) iPSC-derived neurons were treated with 1 μM D1-selective agonist SKF 81297, D2-selective agonist ropinirole, and 1 μM D2 selective antagonist domperidone for 30 minutes. cAMP levels were measured by cAMP-Glo Assay (Promega). Data were normalized to UTC of cells. n = 3. *P < 0.05. (C) iPSC-derived neurons were treated with 1 μM D2-selective antagonist domperidone and/or pan–β-AR antagonist timolol and/or pan–α-AR antagonist dapiprazole for 5 minutes before addition of 1 μM D1-selective agonist SKF 81297 or D2-selective agonist ropinirole for 30 minutes. cAMP levels were measured by cAMP-Glo Assay (Promega). Data were normalized to UTC of cells. n = 3. *P < 0.05. (D) The interaction of JIP3 and D1 was detected by co-IP. Briefly, JIP3 antibody was used for pulling down cell lysates and D1 and JIP3 proteins were measured by Western blot with D1 and JIP3 antibodies, respectively.