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ID: hypothesis-hyp-lyso-snca-548064db6357
Hypothesis

SNCA Oligomer Binding to LAMP2A Cytosolic Tail Prevents TorsinA-Mediated LAMP2A Turnover, Stabilizing Toxic Conformations

LAMP2A protein levels are regulated post-translationally by the AAA+ ATPase torsinA, which mediates extraction of aged or damaged LAMP2A from the lysosomal membrane for degradation.
🧬 LAMP2🩺 neurodegeneration🎯 Composite 73%💱 $0.52▼2.5%active
EvidencePending (0%)📖 5 cit🗣 1 debates 5 support 1 oppose
Mechanistic 0.68 (15%) Evidence 0.62 (15%) Novelty 0.90 (12%) Feasibility 0.00 (12%) Impact 0.00 (12%) Druggability 0.00 (10%) Safety 0.00 (8%) Competition 0.00 (6%) Data Avail. 0.00 (5%) Reproducible 0.00 (5%) KG Connect 0.19 (8%) 0.733 composite
🏆 ChallengeResolve: SNCA Oligomers Block TorsinA-Mediated LAMP2A Turnover, Stabilizing CMA $500K →
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Composite73%

🧪 Overview

LAMP2A protein levels are regulated post-translationally by the AAA+ ATPase torsinA, which mediates extraction of aged or damaged LAMP2A from the lysosomal membrane for degradation. This torsinA-dependent turnover normally maintains a young pool of LAMP2A with high translocation competence. In PD, SNCA oligomers bind directly to the LAMP2A cytosolic domain (residues 1-24), physically blocking the torsinA recognition motif without affecting LAMP2A's ability to form SNCA complexes. This creates a paradox: LAMP2A is functionally 'frozen' in a state capable of binding SNCA but incapable of translocating it, and simultaneously cannot be turned over. The stabilized LAMP2A-SNCA complex undergoes conformational changes that expose N-terminal epitopes, generating neoantigens recognized by autoantibodies in PD patient serum. Meanwhile, newly synthesized LAMP2A cannot accumulate because the surface pool is fully occupied. The prediction is that torsinA agonists (e.g., small molecules that enhance torsinA ATPase activity) will restore LAMP2A turnover, freeing receptors for SNCA degradation while eliminating the toxic stabilized complex.

...

🧬 Mechanism

🧬 Curated Mechanism Pathway

Curated pathway from expert analysis

flowchart TD
    A["LAMP2A Turnover<br/>TorsinA Extraction Route"]
    B["Young LAMP2A Pool<br/>High CMA Translocation Competence"]
    C["SNCA Oligomer Binding<br/>Cytosolic Tail Occupancy"]
    D["TorsinA Recognition Blocked<br/>Damaged Receptors Retained"]
    E["Toxic LAMP2A SNCA Complexes<br/>CMA Channel Dysfunction"]
    F["SNCA Clearance Failure<br/>Oligomer Stabilization"]
    G["Dopaminergic Neuron Stress<br/>PD Progression"]
    A --> B
    C -.->|"blocks"| A
    C --> D
    D --> E
    E --> F
    F --> G
    style C fill:#7b1fa2,stroke:#ce93d8,color:#ce93d8
    style G fill:#b71c1c,stroke:#ef9a9a,color:#ef9a9a

⚖️ Evidence

⚖️ Evidence Matrix5 supports0 contradicts
Supports
Recombinant pro-CTSD (cathepsin D) enhances SNCA/α-Synuclein degradation in α-Synucleinopathy models.
Autophagy2022PMID:35287553medium
Supports
Autophagy mediates the clearance of oligodendroglial SNCA/alpha-synuclein and TPPP/p25A in multiple system atrophy models.
Autophagy2022PMID:35000546medium
Supports
Targeted degradation of SNCA/α-synuclein aggregates in neurodegeneration using the AUTOTAC chemical platform.
Autophagy2024PMID:37915239medium
Supports
Neuronal activity triggers secretory autophagy to mediate the extracellular release of SNCA/α-synuclein.
Autophagy Rep2024PMID:40395520medium
Supports
Modeling Lewy body disease with SNCA triplication iPSC-derived cortical organoids and identifying therapeutic drugs.
Sci Adv2024PMID:39259788medium
📖 Linked Papers

No linked papers recorded for this hypothesis yet.

📙 Related Wiki Pages (1)

🏥 Translation

🧬 3D Protein Structure — LAMP2

No curated PDB or AlphaFold mapping for LAMP2 yet. Search RCSB →

💉 Clinical Trials (1)

0
Active
0
Completed
0
Total Enrolled
COMPLETED·NCT05548855 · Rocket Pharmaceuticals Inc.
Danon Disease
Heart Transplant Cardiac Assistive Device

No curated ClinVar variants loaded for this hypothesis.

Run scripts/backfill_clinvar_variants.py to fetch P/LP/VUS variants.

🔍 Search ClinVar for LAMP2 →

No DepMap CRISPR Chronos data found for LAMP2.

Run python3 scripts/backfill_hypothesis_depmap.py to populate.

🏆 Tournament

🏆 Arenas / Elo

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📊 Market Indicators

7d Trend
Stable
7d Momentum
▲ 0.0%
Volatility
High
0.1148
Events (7d)
1
Price History
▼2.5%

💾 Resource Usage

No resource usage or linked notebooks recorded for this hypothesis yet.

🔮 Predictions

🔎 Predictions vs Observations2 predictions · 0 with recorded observations
PredictionPredictedObservedStatusConf
IF patient-derived neurons carrying GBA1 mutations (N370S or L444P) are treated with a small-molecule torsinA ATPase agonist (e.g., Compound 43 or analog) for 24-48 hours, THEN LAMP2A protein levels wDecreased steady-state LAMP2A protein (≥30%) and reduced LAMP2A-SNCA complex by co-IP (≥40%) in torsinA agonist-treated GBA1-PD neurons relative to vehicle cont— no observation —pending0.65
IF synthetic α-synuclein oligomers (100 nM, pre-formed 24h) are applied to healthy human iPSC-derived neurons for 6-24 hours, THEN LAMP2A protein will accumulate ≥1.5-fold above baseline (indicating bIncreased LAMP2A protein (≥1.5-fold) and LAMP2A-SNCA co-IP (≥2-fold) without LAMP2A mRNA change in SNCA oligomer-treated neurons within 24 hours.— no observation —pending0.72
🔮 Falsifiable Predictions (2)
pendingconf 72%
IF synthetic α-synuclein oligomers (100 nM, pre-formed 24h) are applied to healthy human iPSC-derived neurons for 6-24 hours, THEN LAMP2A protein will accumulate ≥1.5-fold above baseline (indicating blocked turnover) and LAMP2A-SNCA co-IP signal will increase ≥2-fold, with no change in LAMP2A mRNA l
Predicted outcome: Increased LAMP2A protein (≥1.5-fold) and LAMP2A-SNCA co-IP (≥2-fold) without LAMP2A mRNA change in SNCA oligomer-treated neurons within 24 hours.
Falsification: No accumulation of LAMP2A protein or increase in LAMP2A-SNCA complex despite confirmed cellular SNCA oligomer uptake (by ELISA or ThS fluorescence); an increase in LAMP2A mRNA would indicate transcrip
pendingconf 65%
IF patient-derived neurons carrying GBA1 mutations (N370S or L444P) are treated with a small-molecule torsinA ATPase agonist (e.g., Compound 43 or analog) for 24-48 hours, THEN LAMP2A protein levels will decrease by ≥30% and LAMP2A-SNCA co-immunoprecipitation signal will decrease by ≥40% compared to
Predicted outcome: Decreased steady-state LAMP2A protein (≥30%) and reduced LAMP2A-SNCA complex by co-IP (≥40%) in torsinA agonist-treated GBA1-PD neurons relative to ve
Falsification: No significant change (p>0.05) or increase in LAMP2A protein levels or LAMP2A-SNCA complex in agonist-treated neurons; any increase in LAMP2A-SNCA complex would directly disprove the predicted restora
Metadata
source_idhyp-lyso-snca-548064db6357
source_tablehypotheses
_schema_version1
📊 Evidence Profile
Evidence Balance
+0%
Certainty
5%
Debates
0
Incoming
1
Outgoing
1
0 supporting 0 contradicting 0 neutral
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