| Literature DB >> 35693072 |
Ming-Szu Hung1,2,3, Yu-Ching Lin1,2,3, Fen-Fen Chen4, Yuan-Yuan Jiang1, Yu-Hung Fang1, Ming-Shian Lu5, Chin-Kuo Lin2, Tsung-Ming Yang2, Jrhau Lung6, Chih-Cheng Chen2,7, Kuan-Der Lee8, Ying-Huang Tsai9,10.
Abstract
ROS1 fusion genes are rare but important driver genes in lung cancer. Owing to their rarity, many clinicopathological features and treatment responses for each ROS1 fusion variant are still largely unknown and require further investigation. RNA is the preferable template for the ROS1 fusion gene screening, but deterioration of RNA in FFPE often makes the detection challenging. To resolve the difficulty, a targeted chromosomal breakpoint sequencing method was developed for searching the ROS1 fusion gene, and was compared with fluorescence in situ hybridization, immunohistochemistry, RT-qPCR using 260 lung cancer samples of Southern Taiwan. The results showed that ROS1-altered cases were present at low frequencies, did not share distinct clinicopathological features, and often carried other driver mutations. The performance of the targeted sequencing assay was superior to the RT-qPCR in ROS1 fusion gene identification when the cDNAs were from FFPE samples, but long-read DNA sequencing and fresh-frozen samples would be better to revolve all fusion genes. Precise determination of all ROS1 fusion variants and concomitant driver mutations using both genomic DNA and RNA would be required to help improve the treatment of patients with ROS1 alterations. AJCREntities:
Keywords: FISH; IHC; Lung cancer; ROS1 fusion gene; RT-qPCR; targeted chromosomal breakpoint sequencing
Year: 2022 PMID: 35693072 PMCID: PMC9185620
Source DB: PubMed Journal: Am J Cancer Res ISSN: 2156-6976 Impact factor: 5.942