TY - JOUR
T1 - High MET Overexpression Does Not Predict the presence of MET exon 14 Splice Mutations in NSCLC
T2 - Results From the IFCT PREDICT.amm study
AU - Baldacci, Simon
AU - Figeac, Martin
AU - Antoine, Martine
AU - Descarpentries, Clotilde
AU - Kherrouche, Zoulika
AU - Jamme, Philippe
AU - Copin, Marie Christine
AU - Tulasne, David
AU - Nanni, Isabelle
AU - Beau-Faller, Michèle
AU - Melaabi, Samia
AU - Levallet, Guénaëlle
AU - Quoix, Elisabeth
AU - Moro-Sibilot, Denis
AU - Friard, Sylvie
AU - Missy, Pascale
AU - Barlesi, Fabrice
AU - Cadranel, Jacques
AU - Cortot, Alexis B.
N1 - Publisher Copyright:
© 2019 International Association for the Study of Lung Cancer
PY - 2020/1/1
Y1 - 2020/1/1
N2 - Introduction: MET proto-oncogene (MET) exon 14 splice site (METex14) mutations were recently described in NSCLC and has been reported to correlate with efficacy of MET tyrosine kinase inhibitors. High diversity of these alterations makes them hard to detect by DNA sequencing in clinical practice. Because METex14 mutations induce increased stabilization of the MET receptor, it is anticipated that these mutations are associated with MET overexpression. We aim to determine whether NSCLC with high MET overexpression could define a subset of patients with a high rate of METex14 mutations. Methods: From The French Cooperative Thoracic Intergroup PREDICT.amm cohort of 843 consecutive patients with a treatment-naive advanced NSCLC who were eligible for a first-line therapy, 108 NSCLC samples with high MET overexpression defined by an immunochemistry score 3+ were tested for METex14 mutations using fragment length analysis combined with optimized targeted next-generation sequencing. MET copy number analysis was also derived from the sequencing data. Results: METex14 mutations were detected in two patients (2.2%) who also displayed a TP53 mutation and a PIK3CA mutation, respectively. An MET gene copy number increase was observed in seven additional patients (7.7%). Next-generation sequencing analysis revealed inactivating mutations in TP53 (52.7%) and PTEN (1.1%), and oncogenic mutations in KRAS (28.6%), EGFR (7.7%), PIK3CA (4.4%), BRAF (4.4%), NRAS (2.2%), GNAS (1.1%), and IDH1 (1.1%). Conclusions: The rate of METex14 mutations in NSCLC with high MET overexpression was similar to that found in unselected NSCLC. Moreover, we observed a high frequency of driver alterations in other oncogenes. Consequently these findings do not support the use of MET immunohistochemistry as a surrogate marker for METex14 mutations.
AB - Introduction: MET proto-oncogene (MET) exon 14 splice site (METex14) mutations were recently described in NSCLC and has been reported to correlate with efficacy of MET tyrosine kinase inhibitors. High diversity of these alterations makes them hard to detect by DNA sequencing in clinical practice. Because METex14 mutations induce increased stabilization of the MET receptor, it is anticipated that these mutations are associated with MET overexpression. We aim to determine whether NSCLC with high MET overexpression could define a subset of patients with a high rate of METex14 mutations. Methods: From The French Cooperative Thoracic Intergroup PREDICT.amm cohort of 843 consecutive patients with a treatment-naive advanced NSCLC who were eligible for a first-line therapy, 108 NSCLC samples with high MET overexpression defined by an immunochemistry score 3+ were tested for METex14 mutations using fragment length analysis combined with optimized targeted next-generation sequencing. MET copy number analysis was also derived from the sequencing data. Results: METex14 mutations were detected in two patients (2.2%) who also displayed a TP53 mutation and a PIK3CA mutation, respectively. An MET gene copy number increase was observed in seven additional patients (7.7%). Next-generation sequencing analysis revealed inactivating mutations in TP53 (52.7%) and PTEN (1.1%), and oncogenic mutations in KRAS (28.6%), EGFR (7.7%), PIK3CA (4.4%), BRAF (4.4%), NRAS (2.2%), GNAS (1.1%), and IDH1 (1.1%). Conclusions: The rate of METex14 mutations in NSCLC with high MET overexpression was similar to that found in unselected NSCLC. Moreover, we observed a high frequency of driver alterations in other oncogenes. Consequently these findings do not support the use of MET immunohistochemistry as a surrogate marker for METex14 mutations.
KW - Immunohistochemistry
KW - MET
KW - NSCLC
KW - Next-generation sequencing
KW - Receptor tyrosine kinase
UR - http://www.scopus.com/inward/record.url?scp=85076479869&partnerID=8YFLogxK
U2 - 10.1016/j.jtho.2019.09.196
DO - 10.1016/j.jtho.2019.09.196
M3 - Article
C2 - 31605799
AN - SCOPUS:85076479869
SN - 1556-0864
VL - 15
SP - 120
EP - 124
JO - Journal of Thoracic Oncology
JF - Journal of Thoracic Oncology
IS - 1
ER -