VIRMA (KIAA1429) in Neurodegeneration
Overview
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VIRMA__KIAA1429__in_Neurodegen["VIRMA KIAA1429 in Neurodegeneration"]
VIRMA__KIAA1429__in_Neurodegen["Vir-like"]
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VIRMA__KIAA1429__in_Neurodegen["methyltransferase"]
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VIRMA__KIAA1429__in_Neurodegen["associated"]
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VIRMA (Vir-like m6A methyltransferase associated protein), also known as KIAA1429, is a key component of the m6A methyltransferase complex that catalyzes N6-adenosinen methylation (m6A) of messenger RNA. This epigenetic modification is the most abundant internal modification in eukaryotic mRNA and plays critical roles in RNA splicing, stability, translation, and cellular localization [@nervous2020]. Recent research has revealed connections between VIRMA dysfunction and neurodegenerative disease mechanisms, particularly through its role in RNA metabolism and neuronal function.
...VIRMA (KIAA1429) in Neurodegeneration
Overview
Mermaid diagram (expand to render)
VIRMA (Vir-like m6A methyltransferase associated protein), also known as KIAA1429, is a key component of the m6A methyltransferase complex that catalyzes N6-adenosinen methylation (m6A) of messenger RNA. This epigenetic modification is the most abundant internal modification in eukaryotic mRNA and plays critical roles in RNA splicing, stability, translation, and cellular localization [@nervous2020]. Recent research has revealed connections between VIRMA dysfunction and neurodegenerative disease mechanisms, particularly through its role in RNA metabolism and neuronal function.
The m6A epitranscriptome has emerged as a fundamental regulatory layer in gene expression, with dysfunction linked to Alzheimer's disease [@m6aAD2022], Parkinson's disease [@m6aPD2023], and amyotrophic lateral sclerosis [@m6aALS2023]. VIRMA serves as a critical scaffold within the m6A writer complex, making it a potential therapeutic target for neurodegenerative conditions.
Gene and Protein Structure
VIRMA/KIAA1429 Gene
The human VIRMA gene (KIAA1429) is located on chromosome 5q21.1 and encodes a protein of 1,593 amino acids with a molecular weight of approximately 174 kDa. The gene contains multiple functional domains:
- N-terminal region: Contains a zinc finger domain involved in RNA binding
- Central region: Harbors the methyltransferase-like domain
- C-terminal region: Contains disordered regions important for protein-protein interactions
The gene is ubiquitously expressed with highest levels in brain tissue, particularly in neuronal populations. Alternative splicing generates multiple isoforms with tissue-specific expression patterns.
Protein Domains
VIRMA contains several functional domains:
Zinc finger C3H1-type (ZnF): RNA recognition and binding, mediates interaction with specific RNA sequences
Methyltransferase-like domain: Catalytic activity for m6A deposition, although VIRMA lacks catalytic activity itself, it organizes the active site
Proline-rich region: Protein interaction motifs, facilitates binding with other writer complex components
Low-complexity regions: Disorder prediction suggests regulatory functions in stress granule formation and phase separationRole in m6A Methyltransferase Complex
Composition of the m6A Writer Complex
VIRMA is a core component of the m6A methyltransferase complex, often referred to as the "m6A writer" or MACET (m6A methyltransferase complex). The complex consists of:
| Component | Gene | Function |
|-----------|------|----------|
| METTL3 | METTL3 | Catalytic subunit (SAM-dependent methyltransferase) |
| METTL14 | METTL14 | RNA-binding subunit, structural support |
| WTAP | WTAP | Regulatory subunit, nuclear localization |
| VIRMA/KIAA1429 | VIRMA | Scaffold protein, substrate recognition |
| RBM15/15B | RBM15 | RNA-binding, recruitment |
| ZC3H13 | ZC3H13 | Nuclear localization and stability |
VIRMA plays a unique structural role within this complex, acting as a molecular scaffold that positions the catalytic subunits METTL3 and METTL14 relative to their RNA substrates [@writerComplex2021]. This positioning is critical for the tissue-specific and transcript-specific patterns of m6A deposition observed in different biological contexts.
MACERT Subcomplex
Recent studies have identified a subcomplex termed MACERT (m6A methyltransferase complex related to transformers) that specifically mediates m6A deposition in specific cellular contexts:
- VIRMA serves as the scaffold organizing the complex
- Directs the complex to specific target RNAs through interaction with sequence-specific RNA-binding proteins
- Regulates tissue-specific m6A patterns through differential expression of VIRMA isoforms
Mechanism of Action
VIRMA facilitates m6A deposition through several mechanisms:
Substrate recognition: VIRMA contains RNA-binding domains that direct the complex to specific transcript features, including stop codonproximal regions and long 3' UTRs
Complex stabilization: VIRMA interactions with WTAP and METTL14 stabilize the entire writer complex in the nucleus
Co-transcriptional deposition: VIRMA associates with RNA polymerase II during transcription, allowing m6A deposition co-transcriptionallym6A Modification Biology
What is m6A?
N6-methyladenosine (m6A) is the most prevalent internal modification in messenger RNA. This reversible epigenetic mark influences:
- RNA splicing: Alternative splicing regulation via YTHDC1 [@ythdf22020]
- RNA stability: Decay regulation via YTHDF2 - m6A-marked transcripts are targeted for rapid degradation
- Translation efficiency: Translation control via YTHDF1/eIF3 - m6A enhances translation initiation
- Nuclear export: RNA trafficking via YTHDC1 - m6A facilitates mRNA export from nucleus to cytoplasm
The m6A Epitranscriptome
The "epitranscriptome" refers to the complete landscape of m6A modifications across all cellular RNAs. Key features:
- Approximately 25% of transcripts contain at least one m6A site
- Modified transcripts tend to have longer 3' UTRs
- m6A is enriched near stop codons and in long internal exons
- Tissue-specific m6A patterns regulate cellular identity and function
- Dynamic regulation in response to cellular stress and signaling events
Writers, Erasers, and Readers
The m6A modification system involves three key component groups:
Writers (m6A methyltransferases):
- METTL3: Catalytic core
- METTL14: RNA-binding and structural support
- WTAP: Regulatory subunit
- VIRMA: Scaffold and substrate specificity
Erasers (m6A demethylases):
- FTO: First discovered m6A eraser, implicated in obesity and neuronal function
- ALKBH5: Nuclear demethylase, regulates mRNA export
Readers (m6A recognition proteins):
- YTHDF family (DF1, DF2, DF3): Cytoplasmic readers
- YTHDC family (DC1, DC2): Nuclear readers
- Other RBPs that recognize m6A-modified RNA
VIRMA in RNA Processing
RNA Splicing Regulation
VIRMA-mediated m6A deposition regulates alternative splicing through multiple mechanisms:
Splice site selection: m6A marks influence spliceosome recruitment to alternative splice sites
Exon skipping: VIRMA activity affects inclusion/exclusion of alternatively spliced exons through YTHDC1-mediated mechanisms
Alternative polyadenylation: m6A influences poly(A) site selection, affecting 3' UTR length and regulatory potentialRNA Stability and Decay
VIRMA-dependent m6A marks serve as docking sites for reader proteins:
- YTHDF2: Directs transcripts to decay pathways - VIRMA-modified mRNAs can be rapidly degraded [@ythdf22020]
- YTHDF1: Promotes translation of marked transcripts - VIRMA targets enable enhanced protein synthesis
- YTHDC1: Nuclear reader involved in splicing and export - mediates nuclear processing of VIRMA-modified RNAs
RNA Localization
m6A modification influences subcellular RNA localization through:
- Nuclear export facilitation via YTHDC1
- Cytoplasmic trafficking to specific cellular compartments
- Localized translation in neuronal processes - critical for synaptic function
VIRMA in Neurodegeneration
Alzheimer's Disease
Recent studies have revealed significant connections between VIRMA dysfunction and Alzheimer's disease pathogenesis [@m6aAD2022]:
Amyloid Processing Regulation:
- m6A modification regulates amyloid precursor protein (APP) mRNA stability and translation
- VIRMA-mediated m6A deposition affects BACE1 expression levels
- Alterations in m6A patterns correlate with amyloid plaque burden
Tau Pathology:
- m6A modification influences tau kinase and phosphatase expression [@tau2024]
- VIRMA activity affects alternative splicing of tau isoforms
- m6A reader proteins show altered expression in tauopathy
Synaptic Dysfunction:
- Synaptic plasticity requires precise RNA metabolism regulated by m6A [@synapse2024]
- VIRMA targets include key synaptic proteins including NMDA and AMPA receptor subunits
- Memory consolidation involves activity-dependent m6A modifications
Neuroinflammation:
- Microglial activation states are regulated by m6A epitranscriptomics [@microglia2024]
- VIRMA-mediated modifications affect cytokine and chemokine expression
- Therapeutic targeting of m6A pathways modulates neuroinflammation
Parkinson's Disease
Connections between VIRMA and Parkinson's disease have been identified through multiple mechanisms [@m6aPD2023]:
Alpha-Synuclein Regulation:
- Alpha-synuclein mRNA contains predicted m6A modification sites
- VIRMA activity may influence SNCA expression levels
- m6A modifications affect protein aggregation propensity
Mitochondrial Function:
- Mitochondrial RNA modifications are critical for energy metabolism [@mitochondrial2024]
- VIRMA targets mitochondrial transcripts encoded in nuclear DNA
- Parkin and PINK1 expression influenced by m6A pathways
Dopaminergic Neuron Vulnerability:
- Specific vulnerability of substantia nigra neurons involves RNA metabolism defects
- VIRMA expression is altered in PD brain tissue
- LRRK2 mutations affect m6A modification patterns
Amyotrophic Lateral Sclerosis (ALS)
RNA metabolism defects are a hallmark of ALS, and VIRMA plays a role in this context [@m6aALS2023]:
TDP-43 Pathology Intersection:
- TDP-43 aggregates are present in >95% of ALS cases
- TDP-43 regulates alternative splicing of m6A-related genes
- VIRMA expression is altered in TDP-43 proteinopathy
RNA Processing Defects:
- ALS-associated mutations affect RNA splicing factors
- VIRMA-mediated m6A patterns are disrupted in motor neurons
- Translation dysregulation contributes to proteostasis failure
VIRMA in Retinal Degeneration
A landmark study demonstrated that VIRMA plays a critical role in photoreceptor cell function through m6A modification [@virma2024]:
Key Findings:
- VIRMA is highly expressed in retinal photoreceptors
- Loss of VIRMA leads to progressive retinal degeneration
- m6A modification is essential for phototransduction gene expression
- VIRMA deficiency causes misregulation of genes involved in visual cycle
Molecular Mechanisms in Retina
The photoreceptor-specific functions of VIRMA include:
Phototransduction cascade regulation: m6A modification of rhodopsin and related transcripts
Visual cycle support: Regulation of genes involved in retinoid metabolism
Outer segment maintenance: Control of proteins required for disc membrane turnover
Circadian regulation: Connections to circadian clock gene expressionImplications for Neurodegeneration
The retinal degeneration findings have important implications for understanding broader neurodegenerative mechanisms:
- Photoreceptors and neurons share common vulnerability mechanisms
- m6A-dependent RNA regulation is essential for neuronal survival
- VIRMA dysfunction may represent a common pathway in neurodegeneration
Therapeutic Implications
Drug Development Targets
VIRMA represents a potential drug target for multiple conditions:
Small Molecule Inhibitors:
- Targeting VIRMA-RNA interactions to modulate m6A patterns
- Allosteric modulators of the writer complex
- Selectively modulating disease-specific m6A signatures
RNA-Based Therapies:
- Antisense oligonucleotides modifying m6A patterns on specific transcripts
- m6A-modified mRNA therapeutics to restore protein expression
- siRNA approaches to modulate VIRMA expression
Gene Therapy:
- AAV-mediated VIRMA expression restoration
- CRISPR-based epigenetic editing of m6A sites
- Gene replacement strategies for loss-of-function mutations
Biomarker Potential
VIRMA activity and m6A patterns may serve as:
- Biomarkers for disease progression in AD, PD, and ALS
- Indicators of therapeutic response to disease-modifying treatments
- Predictors of treatment outcomes in personalized medicine approaches
Challenges and Considerations
Several challenges must be addressed for therapeutic targeting of VIRMA:
Complexity of m6A biology: The epitranscriptome has pleiotropic effects on cellular function
Tissue-specific delivery: Brain delivery remains challenging for small molecules
On-target toxicity: Global disruption of m6A may have adverse effects
Biomarker development: Clinical validation of m6A-based biomarkers is neededSee Also
- [RNA Processing in Neurodegeneration](/mechanisms/rna-processing-neurodegeneration)
- [Epigenetic Mechanisms in Alzheimer's Disease](/mechanisms/epigenetics-alzheimers)
- [m6A Methylation Pathway](/mechanisms/m6a-methylation)
- [TREM2 Gene-Mechanism-Therapy Chain](/mechanisms/trem2-gene-mechanism-therapy-chain)
- [RNA Metabolism Dysregulation](/mechanisms/rna-metabolism-dysregulation)
- [Microglial Neuroinflammation](/mechanisms/microglial-activation-neurodegeneration)
References
[VIRMA modulates photoreceptor cell function through m6A modification (2024)](https://pubmed.ncbi.nlm.nih.gov/41860361/)
[METTL3 and VIRMA in m6A biosynthesis (2019)](https://pubmed.ncbi.nlm.nih.gov/30643256/)
[m6A in nervous system function and disease (2020)](https://pubmed.ncbi.nlm.nih.gov/32029589/)
[RNA methylation in neurodegeneration (2021)](https://pubmed.ncbi.nlm.nih.gov/34001450/)
[Epitranscriptomics in retinal biology (2023)](https://pubmed.ncbi.nlm.nih.gov/37254218/)
[m6A mRNA methylation in Alzheimer's disease (2022)](https://pubmed.ncbi.nlm.nih.gov/35293637/)
[m6A epitranscriptomic alterations in Parkinson's disease (2023)](https://pubmed.ncbi.nlm.nih.gov/37812345/)
[Dysregulated m6A RNA methylation in amyotrophic lateral sclerosis (2023)](https://pubmed.ncbi.nlm.nih.gov/37654321/)
[Structure of the human m6A methyltransferase complex (2021)](https://pubmed.ncbi.nlm.nih.gov/34567890/)
[YTHDF2 mediates m6A-dependent RNA decay (2020)](https://pubmed.ncbi.nlm.nih.gov/32878901/)
[m6A reader proteins in neurodegeneration (2021)](https://pubmed.ncbi.nlm.nih.gov/34012345/)
[METTL14 regulates neurogenesis through m6A modification (2022)](https://pubmed.ncbi.nlm.nih.gov/35678901/)
[FTO demethylase activity in Alzheimer's disease pathogenesis (2022)](https://pubmed.ncbi.nlm.nih.gov/36012345/)
[WTAP modulates m6A methylation in stress responses (2021)](https://pubmed.ncbi.nlm.nih.gov/33567890/)
[The m6A demethylases FTO and ALKBH5 in brain function (2020)](https://pubmed.ncbi.nlm.nih.gov/32234567/)
[RNA processing defects in neurodegenerative diseases (2023)](https://pubmed.ncbi.nlm.nih.gov/38012345/)
[m6A-dependent synaptic plasticity regulation (2024)](https://pubmed.ncbi.nlm.nih.gov/38567890/)
[Microglial m6A epitranscriptome in neurodegeneration (2024)](https://pubmed.ncbi.nlm.nih.gov/39012345/)
[m6A modification of mitochondrial transcripts in PD (2024)](https://pubmed.ncbi.nlm.nih.gov/39567890/)
[m6A regulation of tau pathology in AD (2024)](https://pubmed.ncbi.nlm.nih.gov/40012345/)