Colorectal Cancer Clinical Trial
Official title:
Comparison of KRAS/BRAF Mutational Status Between Tumor Tissue Section Analysis With Conventional Techniques and Plasma Samples Analysis (KPLEX2)
The goal of this multicenter prospective study is to validate, and ultimately translate in routine clinical practice, the use of plasma analysis of ccfDNA for the determination of KRAS mutation status in mCRC patients.
Analyzing qualitatively and quantitatively genetic alterations with an efficient, simple and
cost-effective test from blood samples could optimize therapeutic decision-making and
personalized cancer care. Cell-free DNA (ccfDNA) levels in the plasma of CRC patients are
significantly higher than in healthy patients. These levels decrease progressively in
tumor-free patients during the follow-up period and increase in patients with recurrence or
metastasis. In the near future, the detection of circulating DNA (ccfDNA) could therefore
represent a technology breakthrough for diagnosis, prognosis, detection of tumor growth and
cancer patient follow up.
We designed a refined and innovative method which simultaneously allows the determination of
three parameters: the specific quantification of tumor-derived ccfDNA, the ccfDNA
fragmentation index, and SNP (Single Nucleotide Polymorphism) or point mutation detection.
In addition to its unprecedented sensitivity and specificity, this qPCR based-method (termed
IntPlex®), recently patented by the CNRS, is easy and rapid, and the first multiplexed test
for ccfDNA.
Evaluation and validation of the IntPlex® test was examined in response to the pressing need
to determine the KRAS/BRAF mutational status before anti-EGFR therapy in CRC patients. As a
consequence, the method was adapted to detect the six more frequent KRAS mutations in CRC
(G12D, G12V, G13D, G12S, G12C, G12A) and the BRAF V600E. We then carried out the first
blinded prospective study to compare KRAS and BRAF mutational status data obtained from the
analysis of tumor tissue by routine gold standard methods and of plasma DNA using our
original method (ASCO oral communication). The mutational status was determined by both
methods in 70 patient samples. Our results clearly showed for the first time that ccfDNA
analysis for KRAS mutation could replace advantageously tumor-section analysis. CcfDNA
analysis showed 100% specificity and sensitivity for the BRAF V600E mutation. For the six
tested KRAS point mutations, the method exhibited 100% specificity and 87% sensitivity with
a concordance value of 96%.
The goal of this multicenter prospective study is to validate, and ultimately translate in
routine clinical practice, the use of plasma analysis of ccfDNA for the determination of
KRAS mutation status in mCRC patients.
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