Targeting nonsense-mediated mRNA decay in colorectal cancers with microsatellite instability

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作者
A’dem Bokhari
Vincent Jonchere
Anaïs Lagrange
Romane Bertrand
Magali Svrcek
Laetitia Marisa
Olivier Buhard
Malorie Greene
Anastasia Demidova
Jieshuang Jia
Eric Adriaenssens
Thierry Chassat
Denis S. Biard
Jean-François Flejou
Fabrice Lejeune
Alex Duval
Ada Collura
机构
[1] Centre de Recherche Saint Antoine,Sorbonne Université, UPMC Univ Paris 06, INSERM, UMRS 938, SIRIC CURAMUS, Equipe Instabilité des Microsatellites et Cancer, Equipe Labellisée par la Ligue Contre le Cancer
[2] Service d’Anatomie et Cytologie Pathologiques,AP
[3] Ligue Nationale Contre le Cancer,HP, Hôpital Saint
[4] UMR 8161—M3T—Mechanisms of Tumorigenesis and Target Therapies,Antoine
[5] University of Lille,Programme “Cartes d’Identité des Tumeurs”
[6] Pasteur de Lille—PLEHTA (Plateforme d’expérimentation et de Haute Technologie Animale),Univ. Lille, CNRS, Institut Pasteur de Lille
[7] Service d’Etude des Prions et des Infections Atypiques,INSERM U908, Cell Plasticity and Cancer
来源
Oncogenesis | / 7卷
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摘要
Nonsense-mediated mRNA decay (NMD) is responsible for the degradation of mRNAs with a premature termination codon (PTC). The role of this system in cancer is still quite poorly understood. In the present study, we evaluated the functional consequences of NMD activity in a subgroup of colorectal cancers (CRC) characterized by high levels of mRNAs with a PTC due to widespread instability in microsatellite sequences (MSI). In comparison to microsatellite stable (MSS) CRC, MSI CRC expressed increased levels of two critical activators of the NMD system, UPF1/2 and SMG1/6/7. Suppression of NMD activity led to the re-expression of dozens of PTC mRNAs. Amongst these, several encoded mutant proteins with putative deleterious activity against MSI tumorigenesis (e.g., HSP110DE9 chaperone mutant). Inhibition of NMD in vivo using amlexanox reduced MSI tumor growth, but not that of MSS tumors. These results suggest that inhibition of the oncogenic activity of NMD may be an effective strategy for the personalized treatment of MSI CRC.
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