Major Depressive Episode Clinical Trial
Official title:
Major Depression and Messenger RNAs
Major Depressive Episode (MDE) affects nearly 15% of the general population. In a preliminary study, the investigators identified 12 genes whose expression was either altered between patient and control samples and/or between first patient samples and samples from the same patients obtained 8 weeks later. However, this study did not assess evolution of these alterations beyond an 8-week window and only 2 time points were considered. The investigators aim to compare gene expression difference for 21 candidate genes, of which 12 were already investigated, in 2 groups of subjects. MDE and control samples will be analyzed across a large time window to draw a better picture of the complex progression during MDE.
Rational:
Major Depressive Episode (MDE) affects nearly 15% of the general population. To date, its
pathophysiology remains unclear and treatment effects are often inconsistent. Therefore, it
is challenging to make a valid prognosis for depression and identification of biomarkers is
an important way of improving patient's treatment. Messenger RNAs (mRNAs) could be potential
biological markers. Several studies have shown quantitative variations in peripheral blood
mononuclear cells (PBMC) during MDE. These variations are state dependent and/or correlated
with clinical measures.
In a preliminary study, the investigators identified 12 genes whose expression was either
altered between patient and control samples and/or between first patient samples and samples
from the same patients obtained 8 weeks later. However, this study did not assess evolution
of these alterations beyond an 8 weeks window and only 2 time points were considered.
Objective:
the investigators aim to compare gene expression difference for 21 candidate genes, of which
12 were already investigated, in 2 groups of subjects. MDE and control samples will be
analyzed across a large time window to draw a better picture of the complex progression
during MDE.
Population and method:
This study is longitudinal and comparative. 20 subjects per group will be included and
followed during a 6 months interval which includes 4 visits (at the inclusion, 2 and 8 weeks
later and finally 6 month later). Clinical observations and psychometric scales will be used
for evaluations. Blood collections and PBMCs extraction will be operated after each
evaluation and followed by RNA extraction, reverse transcription and gene expression
quantification by real-time PCR.
Expected results:
mRNA will be either over or under-expressed in patients during MDE in correlation with the
clinical state. There will be no variation across time in control subjects. Comparison
between MDE and control will show differences during MDE but not after clinical remission.
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Allocation: Non-Randomized, Intervention Model: Parallel Assignment, Masking: Open Label, Primary Purpose: Diagnostic
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