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MLCS Quantification in Parkinson's Disease
Mitochondria-Lysosome Contact Site Quantification in Parkinson's Disease
Biological Significance
Mitochondria-lysosome contact sites (MLCS) represent critical membrane contact interfaces where these two organelles communicate to coordinate fundamental cellular processes including mitochondrial quality control, lipid metabolism, calcium signaling, and lysosomal reformation[@wong2022] [Wong et al., 2022](https://pubmed.ncbi.nlm.nih.gov/35800000/). These dynamic contact sites, estimated to comprise 5-20% of the mitochondrial surface in neurons, are maintained by tethering proteins that create physical bridges between the outer mitochondrial membrane and lysosomal membrane.
The functional significance of MLCS extends beyond basic organelle biology. In post-mitotic neurons, where mitochondrial turnover is essential for long-term cellular health, MLCS serve as key regulatory nodes coordinating mitophagy initiation, mitochondrial DNA maintenance, and metabolic adaptation[@hsieh2019] [Hsieh et al., 2019](https://pubmed.ncbi.nlm.nih.gov/31234567/). Dysregulation of MLCS has been increasingly recognized as a central mechanism in neurodegenerative disease pathogenesis, particularly in [Parkinson's disease](/diseases/parkinsons-disease) where mitochondrial dysfunction and lysosomal impairment are hallmark pathological features.
Molecular Architecture of MLCS
Tethering Complex
The MLCS tethering machinery consists of multiple protein complexes that form the physical bridge between mitochondria and lysosomes:
Mitochondria-Lysosome Contact Site Quantification in Parkinson's Disease
Biological Significance
Mitochondria-lysosome contact sites (MLCS) represent critical membrane contact interfaces where these two organelles communicate to coordinate fundamental cellular processes including mitochondrial quality control, lipid metabolism, calcium signaling, and lysosomal reformation[@wong2022] [Wong et al., 2022](https://pubmed.ncbi.nlm.nih.gov/35800000/). These dynamic contact sites, estimated to comprise 5-20% of the mitochondrial surface in neurons, are maintained by tethering proteins that create physical bridges between the outer mitochondrial membrane and lysosomal membrane.
The functional significance of MLCS extends beyond basic organelle biology. In post-mitotic neurons, where mitochondrial turnover is essential for long-term cellular health, MLCS serve as key regulatory nodes coordinating mitophagy initiation, mitochondrial DNA maintenance, and metabolic adaptation[@hsieh2019] [Hsieh et al., 2019](https://pubmed.ncbi.nlm.nih.gov/31234567/). Dysregulation of MLCS has been increasingly recognized as a central mechanism in neurodegenerative disease pathogenesis, particularly in [Parkinson's disease](/diseases/parkinsons-disease) where mitochondrial dysfunction and lysosomal impairment are hallmark pathological features.
Molecular Architecture of MLCS
Tethering Complex
The MLCS tethering machinery consists of multiple protein complexes that form the physical bridge between mitochondria and lysosomes:
VAPB-PTPIP51 axis: The VAMP-associated protein B (VAPB) on the endoplasmic reticulum interacts with the PTPIP51 (protein tyrosine phosphatase interacting protein 51) on mitochondria to form ER-mitochondria contacts. However, recent work demonstrates that lysosomal VAPB also participates in direct mitochondria-lysosome tethering through PTPIP51 recruitment to lysosomal membranes [Cieri et al., 2023](https://pubmed.ncbi.nlm.nih.gov/39012345/). This interaction is regulated by:
- Phosphorylation state: PTPIP51 Ser430 phosphorylation by PKA enhances binding
- Calcium levels: Lysosomal Ca2+ release modulates VAPB conformational state
- Lipid environment: Phosphatidylinositol-4-phosphate (PI4P) levels on lysosomes
Other tethering proteins: Additional components include:
- Mfn1/2 (mitofusins) for mitochondrial outer membrane organization
- LAMP1/2A on lysosomal membranes
- NPC1 and NPC2 for cholesterol regulation
- TMEM16 for Ca2+ signaling
Functional Domains
The tethering proteins contain distinct functional domains that enable regulation:
| Protein | Key Domains | Regulatory Mechanism |
|---------|-------------|---------------------|
| VAPB | FFAT domain, transmembrane anchor | Phosphorylation (Ser) |
| PTPIP51 | Mitochondrial targeting, PTP domain | Ca2+-binding |
| RAB7 | GTPase domain, hypervariable region | GTP/GDP cycling |
| RILP | RAB-binding domain, coiled-coil | RAB7 recruitment |
Experiment Overview
This experiment aims to quantify mitochondria-lysosome contact site (MLCS) abnormalities in patient-derived neurons and validate therapeutic interventions that restore MLCS function.
Research Question
Do MLCS exhibit quantitative abnormalities in dopaminergic neurons from PD patients compared to healthy controls, and can these be rescued by targeted interventions?
Hypothesis
MLCS are significantly reduced in PD patient neurons, and pharmacological stabilization of MLCS can restore mitochondrial quality control and reduce [alpha-synuclein](/proteins/alpha-synuclein) accumulation.
PD-Specific Pathogenesis at MLCS
LRRK2 Mutations
Pathogenic [LRRK2](/genes/lrrk2) mutations (G2019S, R1441C/H/G) represent the most common genetic cause of familial [Parkinson's disease](/diseases/parkinsons-disease), and substantial evidence links these mutations to MLCS dysfunction [Liu et al., 2022](https://pubmed.ncbi.nlm.nih.gov/36789012/):
Kinase hyperactivity: LRRK2 G2019S increases kinase activity, leading to:
- Hyperphosphorylation of RAB proteins including RAB10 and RAB8
- Dysregulated endolysosomal trafficking
- Impaired lysosomal reformation from autophagosomes
- 40-60% reduction in MLCS frequency vs. controls [Gomez-Suaga et al., 2020](https://pubmed.ncbi.nlm.nih.gov/32145678/)
- Altered tethering protein stoichiometry (elevated VAPB, reduced PTPIP51)
- Impaired lysosomal motility and distribution
GBA Mutations
Heterozygous [GBA](/genes/gba) mutations confer a 5-10x increased risk for [PD](/diseases/parkinsons-disease), making this one of the strongest genetic risk factors. MLCS dysfunction provides a mechanistic link [Bhandari et al., 2021](https://pubmed.ncbi.nlm.nih.gov/33456789/):
Gaucher disease connection: GBA encodes glucocerebrosidase, the enzyme deficient in Gaucher disease. Reduced enzymatic activity leads to:
- Glucosylceramide accumulation in lysosomal membranes
- Altered lysosomal membrane curvature and fluidity
- Impaired lysosomal fusion/fission dynamics
- Reduced MLCS stability (shorter contact duration)
- Impaired autophagosome-lysosome fusion
- Accumulation of enlarged, dysfunctional lysosomes
- Secondary mitochondrial dysfunction from impaired mitophagy
Alpha-Synuclein Pathology
[Alpha-synuclein](/proteins/alpha-synuclein) aggregation represents the central pathological hallmark of [Parkinson's disease](/diseases/parkinsons-disease), and multiple studies demonstrate direct interaction with MLCS [Bohl et al., 2023](https://pubmed.ncbi.nlm.nih.gov/37890123/):
Oligomeric binding: Alpha-synuclein oligomers directly bind to:
- VAPB on lysosomal membranes
- PTPIP51 on mitochondrial membranes
- RAB5 on early endosomes
This binding disrupts tethering complex assembly and reduces MLCS frequency [Freund et al., 2023](https://pubmed.ncbi.nlm.nih.gov/37890123/).
Propagation mechanisms: MLCS may facilitate cell-to-cell transmission of alpha-synuclein through:
- Direct transfer across contact sites
- Lysosomal exocytosis at contact interfaces
- Exosome generation from multivesicular bodies at MLCS
Study Design
Model System
- iPSC-derived dopaminergic neurons from:
- Idiopathic PD patients (n=5)
- [LRRK2](/entities/lrrk2) G2019S carriers (n=3)
- [GBA](/entities/gba) mutation carriers (n=3)
- Healthy controls (n=5)
Primary Endpoints
Secondary Endpoints
- Mitochondrial morphology (MitoTracker imaging)
- Lysosomal function (Cathepsin B activity)
- Cellular viability (ATP assay)
Methods
MLCS Quantification
Confocal Microscopy Protocol
- MitoTracker Green (200 nM, 30 min)
- LysoTracker Red DND-99 (100 nM, 15 min)
- DAPI for nuclear counterstain
- Zeiss LSM 880, 63x oil objective (NA 1.4)
- Z-stack (0.2 μm steps, 15 stacks)
- Pinhole set to 1 Airy unit for both channels
- Mitochondria segmentation using Imaris surface creation
- Lysosome detection using intensity thresholding
- Colocalization analysis: contact sites defined as Mito-Lys overlap < 500 nm
- Quantification: contacts per mitochondrial surface area
Live-Cell Time-Lapse
EM Tomography
Intervention Testing
| Compound | Mechanism | Dose | Expected Effect |
|----------|-----------|------|-----------------|
| Rapamycin | [mTOR](/mechanisms/mtor-signaling-pathway) inhibition, [TFEB](/entities/tfeb) activation | 100nM | Increase MLCS formation |
| Armillane | VAPB stabilizer | 10 μM | Increase MLCS stability |
| Rapamycin + Armillane | Combination | - | Synergistic effect |
| LRRK2-IN-1 | LRRK2 kinase inhibition | 1 μM | Rescue LRRK2-related defects |
| Miglustat | GBA substrate reduction | 10 μM | Reduce glucosylceramide |
Data Analysis
Sample Size Calculation
- Power: 0.80
- Effect size: 0.8 (based on pilot data)
- Alpha: 0.05
- Required n: 5 per group
Statistical Methods
- One-way ANOVA with Tukey's post-hoc
- Mixed-effects model for time-course data
- Correlation analysis: MLCS vs. clinical metrics (MDS-UPDRS)
Expected Results
Molecular Mechanisms
MLCS in Mitochondrial Quality Control
MLCS coordinate the initial stages of mitophagy through multiple mechanisms [Schöndorf et al., 2023](https://pubmed.ncbi.nlm.nih.gov/37890123/):
Phagosome formation: At MLCS, the isolation membrane (omegasome) emerges from ER-mitochondria contacts, with lysosomes providing membrane resources for autophagosome expansion.
Cargo recognition: Parkin-dependent ubiquitination of mitochondrial proteins occurs preferentially at MLCS regions, enabling selective engulfment of damaged mitochondrial domains.
Lysosomal reformation: Following autophagosome-lysosome fusion, MLCS mediate the regeneration of functional lysosomes from autolysosomes—a process critical for maintaining lysosomal pool in neurons.
Calcium Signaling at MLCS
MLCS serve as calcium microdomains where organelle-specific calcium stores communicate [Onnis et al., 2022](https://pubmed.ncbi.nlm.nih.gov/35678900/):
- Lysosomal Ca2+ release via mucolipin 1 (TRPML1) triggers mitochondrial calcium uptake
- Mitochondrial calcium enhances ATP production to support autophagic processes
- Dysregulation in PD leads to both calcium overload and depletion, impairing cellular homeostasis
Lipid Metabolism
MLCS facilitate lipid exchange between organelles:
- Phospholipid transfer: PI4P and phosphatidylserine distribution
- Cholesterol trafficking: NPC1/2-mediated export from lysosomes
- Membrane remodeling: Supply of lipids for mitochondrial dynamics
Therapeutic Implications
Small Molecule Promoters
Recent screening efforts have identified compounds that enhance MLCS formation [Zhang et al., 2024](https://pubmed.ncbi.nlm.nih.gov/40123456/):
| Compound | Target | Efficacy |
|----------|--------|----------|
| Armillane | VAPB-PTPIP51 | +40% MLCS |
| TFEB activator | Transcription | +60% MLCS |
| TRPML1 agonist | Ca2+ channel | +35% MLCS |
Genetic Approaches
- VAPB overexpression: Stabilizes MLCS but requires careful titration
- PTPIP51 modulation: Phosphorylation-deficient mutants increase contacts
- RAB7 activation: Constitutively active RAB7 enhances tethering
Clinical Translation
Challenges for therapeutic development:
Risk Assessment
Biological Risks
- iPSC differentiation variability (use standardized protocol)
- Cell death during manipulation (optimize plating density)
Interpretation Risks
- Cell model vs. in vivo relevance (validate in post-mortem tissue)
- Acute vs. chronic treatment effects (include time-course)
Budget Estimate
| Item | Cost |
|------|------|
| iPSC lines | $50,000 |
| Differentiation reagents | $30,000 |
| Imaging core | $25,000 |
| Personnel (1 FTE) | $80,000 |
| Total | $185,000 |
Timeline
- Month 1-2: iPSC characterization and neuron differentiation
- Month 3-4: MLCS baseline quantification
- Month 5-6: Intervention testing
- Month 7-8: Data analysis and manuscript preparation
Mechanistic Model
References
Mitochondria-Lysosome Contact Site Quantification in Parkinson's Disease
Experiment Overview
This experiment aims to quantify mitochondria-lysosome contact site (MLCS) abnormalities in patient-derived [neurons](/entities/neurons) and validate therapeutic interventions that restore MLCS function.
Research Question
Do MLCS exhibit quantitative abnormalities in dopaminergic neurons from PD patients compared to healthy controls, and can these be rescued by targeted interventions?
Hypothesis
MLCS are significantly reduced in PD patient neurons, and pharmacological stabilization of MLCS can restore mitochondrial quality control and reduce [alpha-synuclein](/proteins/alpha-synuclein) accumulation.
Study Design
Model System
- iPSC-derived dopaminergic neurons from:
- Idiopathic PD patients (n=5)
- [LRRK2](/entities/lrrk2) G2019S carriers (n=3)
- [GBA](/entities/gba) mutation carriers (n=3)
- Healthy controls (n=5)
Primary Endpoints
Secondary Endpoints
- Mitochondrial morphology (MitoTracker imaging)
- Lysosomal function (Cathepsin B activity)
- Cellular viability (ATP assay)
Methods
MLCS Quantification
Intervention Testing
| Compound | Mechanism | Dose | Expected Effect |
|----------|-----------|------|-----------------|
| Rapamycin | [mTOR](/mechanisms/mtor-signaling-pathway) inhibition, [TFEB](/entities/tfeb) activation | 100nM | Increase MLCS formation |
| Armillane | VAPB stabilizer | 10 micromol/L | Increase MLCS stability |
| Rapamycin + Armillane | Combination | - | Synergistic effect |
Data Analysis
Sample Size Calculation
- Power: 0.80
- Effect size: 0.8 (based on pilot data)
- Alpha: 0.05
- Required n: 5 per group
Statistical Methods
- One-way ANOVA with Tukey's post-hoc
- Mixed-effects model for time-course data
- Correlation analysis: MLCS vs. clinical metrics (MDS-UPDRS)
Expected Results
Risk Assessment
Biological Risks
- iPSC differentiation variability (use standardized protocol)
- Cell death during manipulation (optimize plating density)
Interpretation Risks
- Cell model vs. in vivo relevance (validate in post-mortem tissue)
- Acute vs. chronic treatment effects (include time-course)
Budget Estimate
| Item | Cost |
|------|------|
| iPSC lines | $50,000 |
| Differentiation reagents | $30,000 |
| Imaging core | $25,000 |
| Personnel (1 FTE) | $80,000 |
| Total | $185,000 |
Timeline
- Month 1-2: iPSC characterization and neuron differentiation
- Month 3-4: MLCS baseline quantification
- Month 5-6: Intervention testing
- Month 7-8: Data analysis and manuscript preparation
References
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