Type 2 Diabetes Mellitus Clinical Trial
Official title:
Type 2 Diabetes Mellitus: Role of Inflammation and Innate Immunity in The Pathogenesis of Endothelial Dysfunction and Atherosclerosis
In individuals with Type 2 Diabetes (T2D) it has been obtained an outstanding improvement in
the management of hyperglycemia, but it has not been achieved a similar result in the
reduction of the atherosclerotic syndrome. The comprehension of the mechanisms that link
over nutrition to inflammation and innate immune response can be important to understand the
relationship between insulin resistance, diabetes mellitus and endothelial dysfunction. It
will be investigated: 1) the role of Toll Like Receptors (TLR)s in the pathophysiology of
T2D and associated atherosclerosis; 2) the role of aspirin and nicotinamide adenine
dinucleotide phosphate (NADPH) oxidase inhibitor/s in the production of TxA2 and
F2-isoprostanes in T2D patients; 3)new biomarkers associated to Diabetes and atherosclerosis
including markers of endothelial dysfunction and cytokines.
It will be analyzed in isolated platelets from normal controls and/or diabetic patients the
production of TxA2, isoprostanes and pro-inflammatory/thrombotic cytokines using aspirin and
NADPHoxidase inhibitors.
Study design: prospective, controlled, randomized study. All eligible patients will be
randomly assigned in a 1:1 manner to receive aspirin or placebo.
In each recruited subjects we will do:
1. Anamnestic clinical information and Anthropometric measurements
2. Electrocardiogram, echocardiogram and ultrasound assessment of carotid intima-media
thickness (IMT) and flow-mediated dilatation (FMD)
3. Ankle-Brachial Index measurement (ABI)
4. blood samples from an antecubital vein after an overnight fast and urine samples at
baseline, after 3 days and after 30 days of aspirin (100 mg/day) administration.
Laboratory Methods: Blood samples will be immediately centrifuged at 2,000 rpm for 20 min at
4°C, and the supernatant was collected and stored at -80°C until measurement. All
measurements will be done blinded. Samples will be tested in duplicate, and those showing
values above the standard curve will be re-tested with appropriate dilutions.Analysis of
urinary and platelet isoprostane:Urinary PGF2α-III was measured by a previously described
and validated EIA assay method. Ten millilitre urine were extracted on a C-18 SPE column;
the purification was tested for recovery by adding a radioactive tracer (tritiated
PGF2α-III) (Cayman chemical). The eluates were dried under nitrogen, recovered with 1ml of
buffer, and assayed in a PGF2α-III specific EIA kit (Cayman chemical). Urinary PGF2α-III
concentration was corrected for recovery and creatinine excretion and expressed as pg/mg of
creatinine. PRP was then centrifuged 20 min at 800 g to concentrate platelets and the pellet
was suspended in Tyrode buffer to obtain a final platelet concentration of 5x108/mL.
PGF2α-III content was measured by a validated EIA assay method as previously described and
expressed as pg/mg platelet protein.
;
Allocation: Randomized, Endpoint Classification: Pharmacokinetics/Dynamics Study, Intervention Model: Parallel Assignment, Masking: Open Label, Primary Purpose: Treatment
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