Comparative analysis of expression of mutant and wild-type alleles is essential for reliable PCR-based detection of MET exon 14 skipping

外显子 等位基因 生物 桑格测序 外显子跳跃 遗传学 外显子捕获 分子生物学 PCR变异 基因 突变体 突变 选择性拼接
作者
Natalia V. Mitiushkina,Maksim Kholmatov,Vladislav I. Tiurin,Alexandr A. Romanko,Olga S. Yatsuk,Tatiana N. Sokolova,Alexandr O. Ivantsov,Ekatherina Sh. Kuligina,Ilya A. Stepanov,Aleksey Belyaev,Alexandr V. Togo,Evgeny N. Imyanitov
出处
期刊:Biochimie [Elsevier]
卷期号:165: 267-274 被引量:11
标识
DOI:10.1016/j.biochi.2019.08.014
摘要

MET exon 14 skipping (exon 14Δ) mutations are associated with tumor sensitivity to a number of tyrosine kinase inhibitors, however clinical testing for MET gene status remains complicated. We developed a simple allele-specific PCR cDNA-based test, which allowed for the identification of MET exon 14Δ allele in 35 (2.5%) out of 1415 EGFR mutation–negative lung carcinomas (LCs). MET exon 14Δ was significantly associated with elderly age and non-smoking status of the patients. A total of 34 (97%) out of 35 tumors carrying MET exon 14Δ showed preferential expression of the mutated allele; this imbalance was attributed to the down-regulation of the expression of the wild-type gene copy. Sanger sequencing confirmed the presence of genomic exon 14 splice site mutations in 24/35 (68.6%) cases, which showed MET exon 14 skipping by PCR. In addition to LCs described above, some carcinomas demonstrated low-abundance MET exon 14Δ-specific signal. Low-level expression of MET exon 14Δ allele may potentially compromise the results of allele-specific PCR-based tests, therefore comparison of the level of expression of mutated and normal alleles is essential for the reliability of MET gene testing.
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