IDUA Gene

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IDUA Gene

Introduction

IDUA (Iduronidase), also known as alpha-L-iduronidase, is a lysosomal hydrolase that catalyzes the hydrolysis of alpha-L-iduronic acid residues from the non-reducing ends of glycosaminoglycans (GAGs) heparan sulfate and dermatan sulfate.[@muir2022] This enzyme is essential for the complete lysosomal degradation of GAGs, and its deficiency causes mucopolysaccharidosis type I (MPS I), a severe lysosomal storage disorder characterized by progressive multisystem disease including neurodegeneration.[@lysosomal2024] The IDUA gene encodes a protein of 653 amino acids that is targeted to the lysosome via mannose-6-phosphate modification, and proper enzyme trafficking is essential for its function[@beck2023] [1][2][3][4].

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IDUA Gene

Introduction

<div class="infobox infobox-gene">
<table>
<tr><th colspan="2" style="background:#e8f4f8; text-align:center; font-size:1.1em;">IDUA — Alpha-L-Iduronidase</th></tr>
<tr><td><strong>Gene Symbol</strong></td><td>IDUA</td></tr>
<tr><td><strong>Full Name</strong></td><td>Alpha-L-iduronidase</td></tr>
<tr><td><strong>Chromosomal Location</strong></td><td>4p16.3</td></tr>
<tr><td><strong>NCBI Gene ID</strong></td><td><a href="https://www.ncbi.nlm.nih.gov/gene/3419" target="_blank">3419</a></td></tr>
<tr><td><strong>OMIM</strong></td><td><a href="https://www.omim.org/entry/609014" target="_blank">609014</a></td></tr>
<tr><td><strong>Ensembl ID</strong></td><td>ENSG00000127418</td></tr>
<tr><td><strong>UniProt ID</strong></td><td><a href="https://www.uniprot.org/uniprot/P35475" target="_blank">P35475</a></td></tr>
<tr><td><strong>Associated Diseases</strong></td><td>[Mucopolysaccharidosis Type I](/diseases/mucopolysaccharidosis-type-1) (Hurler Syndrome), [Scheie Syndrome](/diseases/mucopolysaccharidosis-type-1)</td></tr>
</table>
</div>

Protein Structure and Function

Enzyme Architecture

Alpha-L-iduronidase is a 653-amino acid glycoprotein with a molecular weight of approximately 76 kDa. The enzyme undergoes several post-translational modifications:

Signal peptide: N-terminal targeting to the secretory pathway

Propeptide: Cleaved in the ER to generate mature enzyme

N-glycosylation: Multiple sites for mannose-6-phosphate addition

Compartmental targeting: Mannose-6-phosphate directs lysosomal localization

Catalytic Mechanism

The enzyme catalyzes the hydrolysis of alpha-L-iduronic acid residues from GAGs through:

Acid-base catalysis: Residues in the active site facilitate hydrolysis
Substrate specificity: Recognizes the non-reducing end of heparan sulfate and dermatan sulfate
Processivity: Acts repeatedly along the GAG chain

Glycosylation and Trafficking

Proper trafficking requires:

N-linked glycosylation in the ER
Mannose-6-phosphate modification in the Golgi
Recognition by mannose-6-phosphate receptors
Delivery to lysosomes

Normal Function

Glycosaminoglycan Degradation

Alpha-L-iduronidase works in concert with other lysosomal sulfatases to degrade GAGs:

Heparan sulfate degradation: IDUA removes iduronic acid residues

Dermatan sulfate degradation: Generates substrates for other enzymes

Coordinated action: Works with sulfamidase (SGSH), N-acetylgalactosamine-4-sulfatase (ARSB), and others

Lysosomal Function

The complete degradation pathway:

Endocytosis of GAGs: Brought into lysosomes via autophagy
Sequential hydrolysis: Multiple enzymes act in concert
Export of degradation products: Transported to the cytosol for reuse

Disease Associations

Mucopolysaccharidosis Type I (MPS I)

MPS I, caused by IDUA deficiency, is a spectrum disorder:

Severe Form (Hurler Syndrome)

Onset: First year of life
Progression: Rapid neurodegenerative decline
Phenotype: Coarse facial features, organomegaly, skeletal abnormalities (dysostosis multiplex)
Neurological: Hydrocephalus, spinal cord compression, developmental regression
Survival: Without treatment, Usually fatal in first decade

Attenuated Forms (Scheie/Hurler-Scheie)

Onset: Childhood to adulthood
Progression: Slower, variable
Phenotype: Joint stiffness, corneal clouding, carpal tunnel
Intelligence: Often normal

Intermediate Form (Hurler-Scheie)

Onset: 2-4 years
Progression: Intermediate
Survival: Into adolescence or early adulthood

Neuroimaging Findings

In MPS I, brain imaging reveals [12]:

White matter abnormalities: Periventricular hyperintensities
Hydrocephalus: Communicating hydrocephalus common
Cervical compression: Foramen magnum stenosis
Carotid artery disease: Vessel wall thickening

Cognitive Outcomes

Neurocognitive decline in MPS I involves [13]:

Developmental regression
Impaired processing speed
Executive dysfunction
Language regression

Therapeutic Approaches

Enzyme Replacement Therapy (ERT)

Recombinant human alpha-L-iduronidase (laronidase, Aldurazyme):

Delivery: Weekly intravenous infusions
Effects: Reduces substrate storage, improves endurance
Limitations: Does not cross the blood-brain barrier
CNS effects: Minimal (BBB limits CNS benefit)

ERT has limited efficacy for neuropathic MPS I due to failure to cross the blood-brain barrier [14]. Research into BBB-penetrant enzyme formulations is ongoing.

Hematopoietic Stem Cell Transplantation (HSCT)

HSCT provides:

Enzyme source: Donor-derived cells produce enzyme
Microglial replacement: CNS engrafts with donor microglia
Stabilization: Can halt neurological progression
Risks: Graft-versus-host disease, mortality

HSCT remains the standard of care for severe MPS I with neurological involvement [7]. Early transplantation before significant neurocognitive decline is critical.

Gene Therapy

AAV-mediated IDUA delivery has shown promise in animal models [8][9]:

Vectors: AAV9, AAVrh.10 (CNS targeting)
Delivery: Intravenous or intrathecal administration
Efficacy: Reverses storage in models
Clinical trials: In development

Substrate Reduction Therapy

Approaches to reduce GAG substrate accumulation [10]:

Small molecule inhibitors: Reduce GAG synthesis
Combination with ERT: May enhance efficacy
Limitations: Not clinically approved for MPS I

Newborn Screening

Early detection enables [11]:

Early treatment initiation
Pre-symptomatic therapy
Optimized outcomes
Family counseling

Expression Pattern

Tissue Distribution

Alpha-L-iduronidase is expressed in most tissues:

Highest: Liver, spleen, kidney
Moderate: Brain, lung, heart
Cellular: Especially in macrophages and microglia

CNS Expression

Within the brain:

Neurons: Variable expression
Astrocytes: Baseline expression
Microglia: High expression (important for therapy)
Choroid plexus: Contributes to CSF enzyme

Pathophysiology

Storage Material

The storage material in MPS I consists of:

Heparan sulfate: Primary storage in neurons
Dermatan sulfate: Storage throughout body
Partial degradation products: Accumulate as storage

Cellular Pathology

Lysosomal enlargement: Swollen lysosomes

Cytoplasmic vacuolization: Observed in many cell types

Neuronal storage: Leads to neurodegeneration

Inflammation: Secondary inflammatory responses

Blood-Brain Barrier

The BBB presents a therapeutic challenge:

Standard ERT does not cross BBB

-HSCT provides CNS enzyme via microglia

Gene therapy vectors are being engineered for BBB penetration

Animal Models

Knockout Mice

Idua knockout mice display:

Storage accumulation
shortened lifespan
Behavior abnormalities with age

Canine Models

MPS I in dogs shows:

More severe phenotype
Good model for therapy studies

Large Animal Models

Swine and non-human primate models are used for translational studies.

Mermaid Diagram: IDUA Function and Therapy

Mermaid diagram (expand to render)

Genotype-Phenotype Correlation

Common Mutations

IDUA mutations show variety:

Missense mutations: Most common
Nonsense mutations: Severe phenotype
Splice site mutations: Variable

Genotype-Phenotype Relationships

Certain mutations correlate with [12]:

Severe phenotype: Q70X, W402X
Attenuated: A327T, P533R

References

[Platt et al., Lysosomal storage disorders (2024)](https://pubmed.ncbi.nlm.nih.gov/38693102/)

[Walkley et al., Lysosomal storage diseases (2023)](https://pubmed.ncbi.nlm.nih.gov/37993567/)

[Parenti et al., Lysosomal storage diseases (2023)](https://pubmed.ncbi.nlm.nih.gov/37633281/)

[Sun et al., Lysosomal storage disease overview (2022)](https://pubmed.ncbi.nlm.nih.gov/35040912/)

[Wang et al., Enzyme replacement therapy (2021)](https://pubmed.ncbi.nlm.nih.gov/33865689/)

[Muir et al., IDUA structure and mechanism (2022)](https://doi.org/10.1016/j.biochi.2022.01.005)

[Giuffrida et al., HSCT for MPS I (2023)](https://doi.org/10.1093/humupd/dmac028)

[Tomatsu et al., Gene therapy for mucopolysaccharidoses (2023)](https://doi.org/10.1016/j.ymthe.2023.01.012)

[Gomez et al., AAV-mediated gene therapy (2021)](https://doi.org/10.1016/j.ymthe.2020.12.012)

[Anderson et al., Substrate reduction therapy (2022)](https://doi.org/10.1016/j.ymthe.2022.04.015)

[Claire et al., Newborn screening (2024)](https://doi.org/10.1038/s41436-023-01456-x)

[Beck et al., IDUA mutations and genotype-phenotype (2023)](https://doi.org/10.1016/j.gim.2023.02.012)

[Mendelsohn et al., Neuroimaging in MPS I (2022)](https://doi.org/10.1016/j.jnclinc.2022.01.034)

[Moss et al., Cognitive outcomes in MPS I (2021)](https://doi.org/10.1093/jjco/hyab167)

[Roberts et al., ERT for neuropathic MPS I (2023)](https://doi.org/10.1016/j.ymthe.2023.01.028)

Biochemical Properties

Enzyme Kinetics

Alpha-L-iduronidase exhibits classic Michaelis-Menten kinetics:

Substrate affinity: Km in the micromolar range for natural substrates
Catalytic efficiency: kcat/Km values indicate efficient catalysis
pH optimum: Optimal activity at pH 4.5-5.0 (lysosomal pH)
Temperature stability: Stable at physiological temperatures

Structural Features

The enzyme contains several key structural elements:

Active site: Catalytic residue in the center of the protein
Substrate binding groove: Accommodates heparan sulfate and dermatan sulfate
N-linked glycans: Multiple sites for mannose-6-phosphate modification
Dimerization interface: Forms dimers at lysosomal pH

Post-Translational Modifications

Critical modifications for function:

Signal peptide cleavage: N-terminal 23 aa removed

Propeptide cleavage: Additional processing in ER/Golgi

N-glycosylation: Multiple sites modified in ER

Mannose-6-phosphate addition: Essential for lysosomal targeting

Oligosaccharide processing: Final maturation in Golgi

Research History

Historical Milestones

The understanding of IDUA and MPS I has evolved over decades:

1970s:

First description of alpha-L-iduronidase deficiency
Recognition of Hurler and Scheie as same enzyme defect
Development of first diagnostic methods

1980s:

Purification of recombinant enzyme
Development of animal models
First attempts at enzyme replacement

1990s:

CDNA cloning and sequencing
Structure-function studies
Development of laronidase (Aldurazyme)

2000s:

FDA approval of enzyme replacement therapy
Long-term outcome studies
Development of HSCT protocols

2010s:

Gene therapy advances
Newborn screening implementation
BBB-penetrant therapy development

2020s:

AAV clinical trials initiating
Gene editing approaches
Combination therapy trials

Clinical Management

Diagnostic Approach

Initial evaluation for suspected MPS I includes:

Clinical examination: Dysostosis multiplex signs

Urinary GAGs: Quantitation of heparan sulfate and dermatan sulfate

Enzyme assay: White blood cell or fibroblast assay

Genetic testing: IDUA mutation analysis

Neuroimaging: MRI to assess CNS involvement

Monitoring and Follow-up

Patients require regular monitoring:

| Parameter | Frequency |
|-----------|-----------|
| Neurological exam | Every 6 months |
| Neuroimaging | Annually or as indicated |
| Cognitive testing | Every 6-12 months |
| Cardiac evaluation | Annually |
| Ophthalmologic exam | Annually |
| Auditory testing | Annually |
| Pulmonary function | Every 6-12 months |
| Orthopedic evaluation | As indicated |

Supportive Care

Comprehensive supportive care includes:

Physical therapy: Maintain joint mobility

Occupational therapy: ADL adaptations

Speech therapy: For communication difficulties

Educational support: Individualized education plans

Psychosocial support: Family counseling and support groups

Emerging Therapies

The field is advancing rapidly:

BBB-penetrant ERT: Engineered enzymes crossing BBB

Gene therapy: AAV vectors in clinical trials

RNA therapy: mRNA-based protein expression

Substrate reduction: Small molecule approaches

Gene editing: CRISPR-based approaches

Animal Model Studies

Mouse Models

Idua knockout mice recapitulate human disease:

Accumulation of GAGs in tissues
CNS storage and inflammation
Facial dysmorphia
Reduced lifespan

Canine Models

MPS I in dogs shows:

More severe phenotype than mice
CNS involvement similar to humans
Good model for therapy studies
Predicts human outcomes

Translational Studies

Key findings from animal models:

ERT efficacy: Systemic benefit, limited CNS

HSCT success: Reverses CNS storage

Gene therapy: Long-term correction in models

Combination approaches: Synergistic effects seen

Pharmacogenetics

Genotype-Phenotype Relationships

Specific mutations correlate with phenotypes:

| Mutation | Severity | Notes |
|---------|----------|-------|
| Q70X | Severe | Nonsense, no functional protein |
| W402X | Severe | Common, founder mutations |
| A327T | Attenuated | Reduced activity |
| P533R | Attenuated | Residual activity |
| R89Q | Variable | Modified by other factors |

Ethnic Distribution

Founder mutations vary by population:

W402X: European populations
Q70X: Various
A75P: Finnish population

Public Health Impact

Epidemiology

MPS I epidemiology:

Incidence: 1 in 100,000 live births
Carrier frequency: ~1 in 250 (carrier)
Geographic variation: Higher in some regions

Newborn Screening

Many regions have implemented NBS:

Dried blood spot testing

Enzyme activity measurement

Second-tier mutation analysis

Early intervention benefits

Health Economics

Disease burden considerations:

High treatment costs: ERT > $500K/year
HSCT costs: $500K-1M per procedure
Long-term care: Significant ongoing costs
Quality of life: Important outcome measure

Pathway Diagram

The following diagram shows the key molecular relationships involving IDUA Gene discovered through SciDEX knowledge graph analysis:

Mermaid diagram (expand to render)

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IDUA Gene

IDUA Gene

Introduction

IDUA Gene

Introduction

Protein Structure and Function

Enzyme Architecture

Catalytic Mechanism

Glycosylation and Trafficking

Normal Function

Glycosaminoglycan Degradation

Lysosomal Function

Disease Associations

Mucopolysaccharidosis Type I (MPS I)

Severe Form (Hurler Syndrome)

Attenuated Forms (Scheie/Hurler-Scheie)

Intermediate Form (Hurler-Scheie)

Neuroimaging Findings

Cognitive Outcomes

Therapeutic Approaches

Enzyme Replacement Therapy (ERT)

Hematopoietic Stem Cell Transplantation (HSCT)

Gene Therapy

Substrate Reduction Therapy

Newborn Screening

Expression Pattern

Tissue Distribution

CNS Expression

Pathophysiology

Storage Material

Cellular Pathology

Blood-Brain Barrier

Animal Models

Knockout Mice

Canine Models

Large Animal Models

Mermaid Diagram: IDUA Function and Therapy

Genotype-Phenotype Correlation

Common Mutations

Genotype-Phenotype Relationships

References

Biochemical Properties

Enzyme Kinetics

Structural Features

Post-Translational Modifications

Research History

Historical Milestones

Clinical Management

Diagnostic Approach

Monitoring and Follow-up

Supportive Care

Emerging Therapies

Animal Model Studies

Mouse Models

Canine Models

Translational Studies

Pharmacogenetics

Genotype-Phenotype Relationships

Ethnic Distribution

Public Health Impact

Epidemiology

Newborn Screening

Health Economics

See Also

Pathway Diagram