The complex, dynamic SpliceOme of the small GTPase transcripts altered by technique, sex, genetics, tissue specificity, and RNA base editing

Akansha S Das; Emily C Sherry; Robert M Vaughan; Marian L Henderson; Jacob Zieba; Katie L Uhl; Olivia Koehn; Caleb P Bupp; Surender Rajasekaran; Xiaopeng Li; Surya B Chhetri; Sahar Nissim; Carol L Williams; Jeremy W Prokop

doi:10.3389/fcell.2022.1033695

The complex, dynamic SpliceOme of the small GTPase transcripts altered by technique, sex, genetics, tissue specificity, and RNA base editing

Front Cell Dev Biol. 2022 Nov 17:10:1033695. doi: 10.3389/fcell.2022.1033695. eCollection 2022.

Authors

Akansha S Das^{1

2}, Emily C Sherry^{1

3}, Robert M Vaughan¹, Marian L Henderson^{1

4}, Jacob Zieba^{1

5}, Katie L Uhl¹, Olivia Koehn⁶, Caleb P Bupp^{1

7}, Surender Rajasekaran^{1

8

9}, Xiaopeng Li¹, Surya B Chhetri¹⁰, Sahar Nissim^{11

12

13}, Carol L Williams⁶, Jeremy W Prokop^{1

5

14}

Affiliations

¹ Department of Pediatrics and Human Development, College of Human Medicine, Michigan State University, Grand Rapids, MI, United States.
² Department of Biology, Washington and Jefferson College, Washington, PA, United States.
³ Department of Cell and Molecular Biology, Grand Valley State University, Allendale, MI, United States.
⁴ The Department of Biology, Calvin University, Grand Rapids, MI, United States.
⁵ Genetics and Genome Sciences Program, BioMolecular Science, Michigan State University, East Lansing, MI, United States.
⁶ Department of Pharmacology and Toxicology, Medical College of Wisconsin, Milwaukee, WI, United States.
⁷ Medical Genetics, Spectrum Health and Helen DeVos Children's Hospital, Grand Rapids, MI, United States.
⁸ Department of Pediatric Critical Care Medicine, Helen DeVos Children's Hospital Spectrum Health, Grand Rapids, MI, United States.
⁹ Office of Research, Spectrum Health, Grand Rapids, MI, United States.
¹⁰ Department of Biomedical Engineering, Johns Hopkins University, Baltimore, MA, United States.
¹¹ Genetics and Gastroenterology Divisions, Brigham and Women's Hospital, Harvard Medical School, Boston, MA, United States.
¹² Dana-Farber Cancer Institute, Boston, MA, United States.
¹³ Harvard-MIT Division of Health Sciences and Technology, Cambridge, MA, United States.
¹⁴ Department of Pharmacology and Toxicology, Michigan State University, East Lansing, MI, United States.

Abstract

The small GTPase family is well-studied in cancer and cellular physiology. With 162 annotated human genes, the family has a broad expression throughout cells of the body. Members of the family have multiple exons that require splicing. Yet, the role of splicing within the family has been underexplored. We have studied the splicing dynamics of small GTPases throughout 41,671 samples by integrating Nanopore and Illumina sequencing techniques. Within this work, we have made several discoveries. 1). Using the GTEx long read data of 92 samples, each small GTPase gene averages two transcripts, with 83 genes (51%) expressing two or more isoforms. 2). Cross-tissue analysis of GTEx from 17,382 samples shows 41 genes (25%) expressing two or more protein-coding isoforms. These include protein-changing transcripts in genes such as RHOA, RAB37, RAB40C, RAB4B, RAB5C, RHOC, RAB1A, RAN, RHEB, RAC1, and KRAS. 3). The isolation and library technique of the RNAseq influences the abundance of non-sense-mediated decay and retained intron transcripts of small GTPases, which are observed more often in genes than appreciated. 4). Analysis of 16,243 samples of "Blood PAXgene" identified seven genes (3.7%; RHOA, RAB40C, RAB4B, RAB37, RAB5B, RAB5C, RHOC) with two or more transcripts expressed as the major isoform (75% of the total gene), suggesting a role of genetics in altering splicing. 5). Rare (ARL6, RAB23, ARL13B, HRAS, NRAS) and common variants (GEM, RHOC, MRAS, RAB5B, RERG, ARL16) can influence splicing and have an impact on phenotypes and diseases. 6). Multiple genes (RAB9A, RAP2C, ARL4A, RAB3A, RAB26, RAB3C, RASL10A, RAB40B, and HRAS) have sex differences in transcript expression. 7). Several exons are included or excluded for small GTPase genes (RASEF, KRAS, RAC1, RHEB, ARL4A, RHOA, RAB30, RHOBTB1, ARL16, RAP1A) in one or more forms of cancer. 8). Ten transcripts are altered in hypoxia (SAR1B, IFT27, ARL14, RAB11A, RAB10, RAB38, RAN, RIT1, RAB9A) with RHOA identified to have a transient 3'UTR RNA base editing at a conserved site found in all of its transcripts. Overall, we show a remarkable and dynamic role of splicing within the small GTPase family that requires future explorations.

Keywords: RNA modifications; cancer; expression; isoforms; protein modeling; small GTPase; splicing aberrations.

Associated data

figshare/10.6084/m9.figshare.20371842

Abstract

Associated data

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