Pathogenic germline variants in the APC gene result in familial adenomatous polyposis (FAP) which can escalate into colon cancer. Standard clinical testing failed to identify pathogenic variants in a 4-generation FAP family. We identified and assessed co-segregation of a 5' untranslated region (UTR) variant, NM_001127511.3 (APC) c.-40G>A (GRCh37 chr5:112043375) that creates a potential out-of-frame AUG start codon. The segregation odds of pathogenicity for the APC c.-40G>A variant are 159:1. Translation initiation confidence values for all possible AUGs in the 5' UTR created by a single nucleotide substitution were calculated using PreTIS online tool. The -40G>A variant scored the highest possible confidence value. To test -40G>A as an initiating methionine, we created reporter constructs consisting of the entire 5' UTR and first 81 bases of APC driving luciferase. When the -40G>A variant was present, luciferase activity was decreased to 14%-25% of the wild-type construct. When the premature start codon created by the -40G>A variant was in-frame with luciferase, we observed luciferase activity from this de novo false start site. Combined, our evidence supports classification of APC c.-40G>A to likely pathogenic, presumably through squelching of the canonical AUG start codon. More importantly, it underlines the feasibility and importance of clinical laboratories to screen noncoding regions.
Keywords: 5′ UTR; APC; familial polyposis; luciferase reporter; mutation; sequencing; translation initiation.
© 2025 The Author(s). American Journal of Medical Genetics Part A published by Wiley Periodicals LLC.