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Detection of ALK rearrangements in lung cancer patients using a homebrew PCR assay.


ABSTRACT: Lung cancer patients with anaplastic lymphoma kinase (ALK) rearrangements are candidates for targeted therapeutics. However, patients must be tested with a companion diagnostic assay to realize their ALK rearrangement status. We analyzed the publicly available E-GEOD-31210 microarray dataset and identified a non-coding RNA, sweyjawbu, which is strongly associated with ALK rearrangements. We validated these results using quantitative real-time PCR in an independent cohort consisting of 4 cell lines and 83 clinical samples. We could differentiate between ALK rearrangement-positive and -negative lung cancer samples by comparing sweyjawbu expression. Additionally, ALK rearrangement status was determined by comparing the expression of the 5' and 3' regions of the ALK transcript or by detecting known ALK hybrid subtypes. Thus, using our homebrew PCR assay, we were able to accurately detect ALK rearrangements, which could be used for diagnostic screening of lung cancer patients. The prototype could potentially be transferred to an automatic multiplex PCR platform (FilmArray) to differentiate between ALK rearrangement-positive and -negative patients in point-of-care settings.

SUBMITTER: Yu H 

PROVIDER: S-EPMC5352355 | biostudies-literature | 2017 Jan

REPOSITORIES: biostudies-literature

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Detection of ALK rearrangements in lung cancer patients using a homebrew PCR assay.

Yu Hui H   Chang JianHua J   Liu Fang F   Wang Qifeng Q   Lu YongMing Y   Zhang ZhuanXu Z   Shen Jiabing J   Zhai Qing Q   Meng Xia X   Wang Jialei J   Ye Xun X  

Oncotarget 20170101 5


Lung cancer patients with anaplastic lymphoma kinase (ALK) rearrangements are candidates for targeted therapeutics. However, patients must be tested with a companion diagnostic assay to realize their ALK rearrangement status. We analyzed the publicly available E-GEOD-31210 microarray dataset and identified a non-coding RNA, sweyjawbu, which is strongly associated with ALK rearrangements. We validated these results using quantitative real-time PCR in an independent cohort consisting of 4 cell lin  ...[more]

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