doi: 10.1038/s41422-018-0033-7.
Epub 2018 Apr 8.
Circular RNA F-circEA produced from EML4-ALK fusion gene as a novel liquid biopsy biomarker for non-small cell lung cancer
Affiliations
- PMID: 29628502
- PMCID: PMC5993747
- DOI: 10.1038/s41422-018-0033-7
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Circular RNA F-circEA produced from EML4-ALK fusion gene as a novel liquid biopsy biomarker for non-small cell lung cancer
Cell Res.
2018 Jun.
No abstract available
Conflict of interest statement
The authors declare no competing interests.
Figures
Identification and functional analysis of F-circEA in NSCLC. a Schematic representation of F-circEA generated from EML4-ALK fusion gene. The convergent primers (F1/R1) were used to detect EML4-ALK fusion site, and the divergent primer sets (F2/R2, F3/R3) were used to detect F-circEA. Violet curve represents siRNA location. b Agarose gel electrophoresis and Sanger sequencing of RT-PCR products from H2228 cells with F1/R1 primers, the arrow indicates EML4-ALK fusion site. c Identification of F-circEA in H2228 cells by RT-PCR with F2/R2 primers and Sanger sequencing. The arrow indicates F-circEA junction site. d Detection of F-circEA and EML4-ALK mRNA by RNA solution hybridization assay using 32P-labeled oligonucleotide probes crossing junction site and the fusion site. e Cell nucleus/cytoplasm fractionation and RT-qPCR analysis revealed the cytoplasmic distribution of F-circEA in H2228 cells. GAPDH mRNA and U6 snRNA represent cytoplasmic and nuclear RNA, respectively. Western blotting confirmed the efficiency of nucleus/cytoplasm isolation. Data are shown as the mean ± SD. f Knockdown efficiency of F-circEA siRNAs in H2228 cells analyzed by RT-qPCR. g F-circEA knockdown inhibited cell migration and invasion in H2228 cells. h Schematic representation of F-circEA-expressing plasmid with the reverse repeat of cirR-7 exons plus up-stream and down-stream flanking introns to facilitate RNA circularization. i RNA solution hybridization assays for F-circEA and EML4-ALK mRNA in H2228, H1299, empty vector-transfected (Ctrl-H1299), and F-circEA-overexpressing (F-circEA-H1299) H1299 cells. j Cell nucleus/cytoplasm fractionation and RT-qPCR analysis demonstrated that F-circEA was predominantly located in the cytoplasm of F-circEA-overexpressing H1299 cells. Data are shown as the mean ± SD. k Ectopic expression of F-circEA increased the migratory and invasive ability of H1299 cells. Results of statistical analysis are shown in the right panel. l RT-qPCR analysis showed effective knockdown of F-circEA by siRNA in F-circEA-overexpressing H1299 cells. The scramble siRNA (SCR) was used as negative control. m, n F-circEA knockdown attenuated the enhanced migratory and invasive ability of F-circEA-overexpressing H1299 cells. *P < 0.05. o, p Agarose gel electrophoresis and Sanger sequencing of RT-PCR products from tumor tissues (o) or plasma (p) of NSCLC patients with or without EML4-ALK fusion gene
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