Pathogenic mechanism and therapeutic intervention of impaired N 7 -methylguanosine (m 7 G) tRNA modification
Neurons
Taurochenodeoxycholic Acid
Mice
RNA, Transfer
Guanosine
GTP-Binding Proteins
Mutation
Animals
Humans
Apoptosis
Methyltransferases
Endoplasmic Reticulum Stress
DOI:
10.1073/pnas.2405886121
Publication Date:
2024-10-29T17:36:55Z
AUTHORS (19)
ABSTRACT
Mutations modification enzymes including the tRNA N
7
-methylguanosine (m
7
G) methyltransferase complex component WDR4 were frequently found in patients with neural disorders, while the pathogenic mechanism and therapeutic intervention strategies are poorly explored. In this study, we revealed that patient-derived
WDR4
mutation leads to temporal and cell-type-specific neural degeneration, and directly causes neural developmental disorders in mice. Mechanistically,
WDR4
point mutation disrupts the interaction between WDR4 and METTL1 and accelerates METTL1 protein degradation. We further uncovered that impaired tRNA m
7
G modification caused by
Wdr4
mutation decreases the mRNA translation of genes involved in mTOR pathway, leading to elevated endoplasmic reticulum stress markers, and increases neural cell apoptosis. Importantly, treatment with stress-attenuating drug Tauroursodeoxycholate (TUDCA) significantly decreases neural cell death and improves neural functions of the
Wdr4
mutated mice. Moreover, adeno-associated virus mediated transduction of wild-type WDR4 restores METTL1 protein level and tRNA m
7
G modification in the mouse brain, and achieves long-lasting therapeutic effect in
Wdr4
mutated mice. Most importantly, we further demonstrated that both TUDCA treatment and WDR4 restoration significantly improve the survival and functions of human iPSCs-derived neuron stem cells that harbor the patient’s
WDR4
mutation. Overall, our study uncovers molecular insights underlying
WDR4
mutation in the pathogenesis of neural diseases and develops two promising therapeutic strategies for treatment of neural diseases caused by impaired tRNA modifications.
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