CircFISH: A Novel Method for the Simultaneous Imaging of Linear and Circular RNAs

Aakash Koppula; Ahmed Abdelgawad; Jlenia Guarnerio; Mona Batish; Vijay Parashar

doi:10.3390/cancers14020428

CircFISH: A Novel Method for the Simultaneous Imaging of Linear and Circular RNAs

Cancers (Basel). 2022 Jan 15;14(2):428. doi: 10.3390/cancers14020428.

Authors

Aakash Koppula^{1

2}, Ahmed Abdelgawad^{1

2}, Jlenia Guarnerio³, Mona Batish^{1

2}, Vijay Parashar^{1

2}

Affiliations

¹ Department of Biological Sciences, University of Delaware, Newark, DE 19716, USA.
² Department of Medical and Molecular Sciences, University of Delaware, Newark, DE 19716, USA.
³ Samuel Oschin Comprehensive Cancer Institute, Division of Cancer Biology and Therapeutics, Cedars-Sinai Medical Center, Los Angeles, CA 90048, USA.

Abstract

Circular RNAs (circRNAs) are regulatory RNAs which have recently been shown to have clinical significance in several diseases, including, but not limited to, various cancers, neurological diseases and cardiovascular diseases. The function of such regulatory RNAs is largely dependent on their subcellular localization. Several circRNAs have been shown to conduct antagonistic roles compared to the products of the linear isoforms, and thus need to be characterized distinctly from the linear RNAs. However, conventional fluorescent in situ hybridization (FISH) techniques cannot be employed directly to distinguish the signals from linear and circular isoforms because most circRNAs share the same sequence with the linear RNAs. In order to address this unmet need, we adapted the well-established method of single-molecule FISH by designing two sets of probes to differentiate the linear and circular RNA isoforms by virtue of signal colocalization. We call this method 'circular fluorescent in situ hybridization' (circFISH). Linear and circular RNAs were successfully visualized and quantified at a single-molecule resolution in fixed cells. RNase R treatment during the circFISH reduced the levels of linear RNAs while the circRNA levels remain unaltered. Furthermore, cells with shRNAs specific to circRNA showed the loss of circRNA levels, whereas the linear RNA levels were unaffected. The optimization of the in-situ RNase R treatment allowed the multiplexing of circFISH to combine it with organelle staining. CircFISH was found to be compatible with multiple sample types, including cultured cells and fresh-frozen and formalin-fixed tissue sections. Thus, we present circFISH as a versatile method for the simultaneous visualization and quantification of the distribution and localization of linear and circular RNA in fixed cells and tissue samples.

Keywords: FFPE; RNase R; circular RNAs; fixed cells; frozen tissues; immunofluorescence; multiplex RNA imaging; non-coding RNAs; nucleic acid probes; single-molecule RNA imaging; subcellular RNA localization.

Abstract

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