Coronary Artery Disease Clinical Trial
Official title:
The Association Between Plasma or Platelet microRNAs and Clopidogrel Low Response and Its Mechanism
Clopidogrel is an important anti-platelet agent.However, about 30% of the coronary artery
disease patients presented clopidogrel low response (CLR).Previous studies showed that the
cardiovascular event ratio of the CLR patients was 4.4 times of the normal responders.
It is known that the plasma and platelet miRNAs are determined by different disease status
when platelets are released from the megakaryocyte, and the platelet miRNAs can adjust the
expressions of the platelet's receptors and proteins.The purpose of this study is to find
multiple platelet miRNAs involved in the development of CLR, and platelet miRNAs cause CLR
through adjusting the expressions of the key receptors and proteins in the ADP activating
pathway and consequently reducing their responses to clopidogrel.
The CLR will be detected by light transmission aggregometry (LTA) and vasodilator-stimulated
phosphoprotein phosphorylation (VASP-P). Differential expressions of plasma and platelet
miRNAs profile in CLR patients will be screened by deep sequencing and validated to
investigate the association between plasma and platelet miRNAs profile and CLR as well as
the patients' prognosis.The study results would serve as markers for individualized
anti-platelet treatment, and supply new targets for the treatment of coronary artery
disease.
A multiphase, case-control study was designed to identify plasma and platelet miRNAs as
surrogate markers for CLR .
All patients take 300mg loading dose clopidogrel plus 100mg daily ASA and 75mg daily
clopidogrel after admission. Patients are recruited after percutaneous coronary intervention
(PCI). Light transmittancy aggregation (LTA) in response to 5μM ADP is to measured 5 days
after taking the loading dose clopidogrel.Than CLR patients were selected.
In the initial biomarker-screening stage, plasma and platelet samples from 20 CLR patients
and 20 controls underwent Solexa sequencing to identify miRNAs that showed significant
differences between the CLR cases and matched controls.
Subsequently,we performed a biomarker confirmation analysis with a hydrolysis probe-based
RT-qPCR assay to refine the number of plasma and platelet miRNAs in the CLR signature. This
analysis was carried out in 2 phases: (a) the biomarker-selection phase, in which plasma and
platelet samples from 20 CLR patients and 20 control individuals formed the training set,
and (b) the biomarker-validation phase, in which plasma and platelet samples from an
additional 80 CLR patients and 80 controls formed the validation set.
;
Allocation: Randomized, Endpoint Classification: Safety/Efficacy Study, Intervention Model: Single Group Assignment, Masking: Single Blind (Subject), Primary Purpose: Diagnostic
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