Type 2 Diabetes Mellitus Clinical Trial
— DIAXOOfficial title:
Involvement of Reactive Oxygen Species Produced by the Xanthine Oxidase in Mitochondrial Alterations in Skeletal Muscle of Type 2 Diabetic Patients
Verified date | October 2019 |
Source | Hospices Civils de Lyon |
Contact | n/a |
Is FDA regulated | No |
Health authority | |
Study type | Interventional |
Our recent data in mice have demonstrated a key role of xanthine oxidase in hyperglycemia-induced by Reactive oxygen species production, and a preventive role of allopurinol (inhibitor of xanthine oxidase) on the keeping of mitochondria number and structure, in skeletal muscle of diabetic mice. The investigators want to initiate a clinical trial in order to evaluate the efficacy of allopurinol on the improvement of mitochondrial alterations, oxidative capacities and insulin sensitivity, in skeletal muscle of type 2 diabetic patients.
Status | Completed |
Enrollment | 31 |
Est. completion date | February 18, 2016 |
Est. primary completion date | February 2016 |
Accepts healthy volunteers | No |
Gender | All |
Age group | 30 Years to 60 Years |
Eligibility |
Inclusion Criteria: - BMI from 25 to 40 kg/m² - Type 2 diabetes known for over one year but less than 10 years, treated with Oral anti-diabetic drugs or a Glucagon-like peptide-1 (GLP1-analog) - well controlled hypertension (untreated or currently treated) with a systolic blood pressure of 95 to 140 mmHg and diastolic blood pressure of 45 to 90 mmHg and heart frequency of 40 to 100 per minute - Recent HbA1c < 9 % - Uricemia > 300 µmol/l - For women : Menopausal or contraception - Renal function as defined by glomerular filtration rate (GFR) = 80 mL/min/1.73 m2 Exclusion Criteria: - Tobacco ( more than 5 cigarettes) - Excessive drinking - Known pathology - Hypersensitivity to allopurinol - Treatment by anticoagulants, allopurinol, regular steroids or Nonsteroidal anti-inflammatory drug (NSAID), fibrate or insulin |
Country | Name | City | State |
---|---|---|---|
France | CRNH Rhône Alpes | Lyon |
Lead Sponsor | Collaborator |
---|---|
Hospices Civils de Lyon |
France,
Type | Measure | Description | Time frame | Safety issue |
---|---|---|---|---|
Primary | muscle oxidative stress in diabetic patients | muscular protein carbonylation level (unit: reactive carbonyl derivates, arbitrary unit) by Western blot (oxyblot kit from Chemicon) and pro et antioxidant genes expression (unit: mRNA levels normalized by housekeeping gene, arbitrary ratio) by real time polymerase chain reaction (RT-PCR) | At 3 months of treatment | |
Secondary | - plasmatic oxidative stress by dosing plasmaticmarkers: | Dosing plasmatic malondialdéhyde, plasmatic H2O2, protein carbonylation of plasmatic protein and urinary isoprostans, and finally antioxidants (vitamins C and E, glutathione (unit: from µM to M) | At 3 months of treatment | |
Secondary | alterations in mitochondrial structure of skeletal muscle with transmission electron microscopy | Analysis of mitochondria area (in µm2) and density (in %) | At 3 months of treatment | |
Secondary | mitochondrial density by measuring the ratio mitochondrial Deoxyribonucleic acid (mtDNA)/nuclear DNA by real-time polymerase chain reaction (PCR) in skeletal muscle | At 3 months of treatment | ||
Secondary | mitochondrial function | Expression of genes implicated in mitochondrial action (messenger Ribonucleic acid (mRNA) levels by Reverse transcription polymerase chain reaction (RT-PCR) and proteins levels by Western Blot)(unit: arbitrary ratio relative to housekeeping gene/protein). | At 3 months of treatment | |
Secondary | quantification of intramuscular lipids by histology (biopsy analysis) | Staining Oil Red O evaluate the intramuscular lipid accumulation using the software ImageJ(unit: % of labelling by field). | At 3 months of treatment | |
Secondary | sensitivity to insulin using a hyperinsulinemic euglycemic clamp | sensitivity to insulin will be expressed as the glucose infusion rate (GIR)/insulinemia ratio. | At 3 months of treatment | |
Secondary | uricemia and xanthine oxidase activity in sera and muscles(unit: mg/l for uricemia and mU/ml for XO activity) | Plasma concentrations of uric acid will be measured before and after treatment to assess patient compliance . The reduction of xanthine oxidase activity in serum and muscle protein lysates will be measured using the kit " Amplex Red xanthine / xanthine oxidase assay kit" from Molecular Probes | At 3 months of treatment | |
Secondary | Tolerance of the treatment measured by any adverse events during treatment and between each visit. | Any adverse events during treatment and between each visit. | during the 3 months of treatment |
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