PT - JOURNAL ARTICLE AU - Nabeel S. Ganem AU - Noa Ben-Asher AU - Aidan C. Manning AU - Sarah N. Deffit AU - Michael C. Washburn AU - Emily C. Wheeler AU - Gene W. Yeo AU - Orna Ben-Naim Zgayer AU - Einav Mantsur AU - Heather A. Hundley AU - Ayelet T. Lamm TI - Disruption in A-to-I editing levels affects <em>C. elegans</em> development more than a complete lack of editing AID - 10.1101/273433 DP - 2018 Jan 01 TA - bioRxiv PG - 273433 4099 - http://biorxiv.org/content/early/2018/02/28/273433.short 4100 - http://biorxiv.org/content/early/2018/02/28/273433.full AB - A-to-I RNA editing is widespread in eukaryotic transcriptomes and plays an essential role in the creation of proteomic and phenotypic diversity. Loss of ADARs, the proteins responsible for A-to-I editing, results in lethality in mammals. In C. elegans, knocking out both ADARs, ADR-1 and ADR-2, results in aberrant behavior and abnormal development. Studies have shown that ADR-2 can actively deaminate dsRNA while ADR-1 cannot. However, as most studies of C. elegans ADARs were performed on worms mutated in both ADAR genes, the effects observed cannot be attributed to a single ADAR or to the interactions between ADAR genes. Therefore, we set to study the effects of each C. elegans ADAR on RNA editing, gene expression, protein levels and the contribution of each of ADAR to the phenotypes observed in worms mutated in both genes, in order to elucidate their distinct functions. We found significant differences in the phenotypes observed in worms mutated in a single ADAR gene. Worms harboring adr-1 mutations have a significant reduction in their lifespan, while worms harboring adr-2 mutations have extended lifespan. We also observed severe abnormalities in vulva formation in adr-1 mutants, and we suggest that these phenotypes are a result of an RNA editing independent function of ADR-1. Mutations in each ADAR resulted in expressional changes in hundreds of genes, and a significant downregulation of edited genes. However, very few changes in the protein levels were observed. In addition, we found that ADR-1 binds many edited genes. Our results suggest that ADR-1 plays a significant role in the RNA editing process and by altering editing levels it causes the severe phenotypes that we observed. In contrast, a complete lack of RNA editing is less harmful to the worms. Furthermore, our results indicate that the effect of RNA editing on the protein content in the cell is minor and probably the main purpose of these modifications is to antagonize or enhance other gene regulatory mechanisms that act on RNA.