Reproducible features of small RNAs in <i>C. elegans</i> reveal NU RNAs and provide insights into 22G RNAs and 26G RNAs

Blumenfeld, Andrew; Jose, Antony M.

doi:10.1261/rna.054551.115

Cited by 20 publications

(27 citation statements)

References 38 publications

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“…We next filtered for small RNA reads of 20-23 nucleotide in length ( Blumenfeld and Jose, 2016 ). Then we counted reads in antisense orientation to genes as defined by the corresponding Ensembl .gff file, using a python based script HTSeq count ( Anders et al., 2015 ): HTSeq.scripts.count–stranded = reverse–minaqual = 0–mode = intersection-nonempty input.sam GENES.gff > output.txt …”

Section: Methodsmentioning

confidence: 99%

“…Endo-siRNAs target both protein-coding and non-protein coding loci ( Gu et al., 2009 , Vasale et al., 2010 ). Endo-siRNAs align in the antisense orientation to exons, can tile the entire length of the mature mRNA transcript, and complement the target perfectly ( Blumenfeld and Jose, 2016 ). For simplicity, units of small RNAs targeting a specific gene, will be referred to here as STGs (see Rechavi et al.…”

Section: Introductionmentioning

confidence: 99%

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Neuronal Small RNAs Control Behavior Transgenerationally

Posner

Toker

Antonova

et al. 2019

Cell

149

148

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Summary It is unknown whether the activity of the nervous system can be inherited. In Caenorhabditis elegans nematodes, parental responses can transmit heritable small RNAs that regulate gene expression transgenerationally. In this study, we show that a neuronal process can impact the next generations. Neurons-specific synthesis of RDE-4-dependent small RNAs regulates germline amplified endogenous small interfering RNAs (siRNAs) and germline gene expression for multiple generations. Further, the production of small RNAs in neurons controls the chemotaxis behavior of the progeny for at least three generations via the germline Argonaute HRDE-1. Among the targets of these small RNAs, we identified the conserved gene saeg- 2, which is transgenerationally downregulated in the germline. Silencing of saeg- 2 following neuronal small RNA biogenesis is required for chemotaxis under stress. Thus, we propose a small-RNA-based mechanism for communication of neuronal processes transgenerationally.

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Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Neuronal Small RNAs Control Behavior Transgenerationally

Posner

Toker

Antonova

et al. 2019

Cell

149

148

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“…While such products arise during viral infection, they have not been observed among endo-siRNAs in wild-type C. elegans (Ruby et al 2006;Ashe et al 2013;Billi et al 2014). Rather, characterized DCR-1-dependent endo-siRNAs are 26 nt, have a 5 ′ guanosine monophosphate (26G siRNAs), and are produced by DCR-1 acting in concert with the RNA-dependent RNA polymerase (RdRP) RRF-3 (Thivierge et al 2012;Blumenfeld and Jose 2016). 26G siRNAs occur in embryos and germline tissues and exist in two classes bound to distinct Argonaute proteins.…”

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confidence: 99%

C. elegans ADARs antagonize silencing of cellular dsRNAs by the antiviral RNAi pathway

2018

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Cellular dsRNAs are edited by adenosine deaminases that act on RNA (ADARs). While editing can alter mRNA-coding potential, most editing occurs in noncoding sequences, the function of which is poorly understood. Using dsRNA immunoprecipitation (dsRIP) and RNA sequencing (RNA-seq), we identified 1523 regions of clustered A-to-I editing, termed editing-enriched regions (EERs), in four stages of development, often with highest expression in embryos. Analyses of small RNA-seq data revealed 22- to 23-nucleotide (nt) siRNAs, reminiscent of viral siRNAs, that mapped to EERs and were abundant in mutant animals. Consistent with roles for these siRNAs in silencing, EER-associated genes (EAGs) were down-regulated in embryos, and this was dependent on associated EERs and the RNAi factor RDE-4. We observed that ADARs genetically interact with the 26G endogenous siRNA (endo-siRNA) pathway, which likely competes for RNAi components; deletion of factors required for this pathway ( or ) in mutant strains caused a synthetic phenotype that was rescued by deleting antiviral RNAi factors. Poly(A) RNA-seq revealed EAG down-regulation and antiviral gene induction in embryos, and these expression changes were dependent on and Our data suggest that ADARs restrict antiviral silencing of cellular dsRNAs.

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“…We found that loss of rrf-3 or of eri-1 but not of ergo-1 eliminated inhibition of feeding RNAi by expression from a repetitive transgene within the hypodermis ( Figure 4I). Because RRF-3 and ERI-1 are not required for the production of dsRNA from repetitive transgenes (Kim et al 2005), these results suggest that silencing by feeding RNAi in the presence of expression from a repetitive transgene is enabled by loss of dsRNA production at endogenous loci (see Figure S9 in Blumenfeld and Jose 2016).…”

Section: Expression Of a Repetitive Transgene In A Tissue Can Inhibitmentioning

confidence: 97%

Each cell needs long double-stranded RNA for silencing by feeding RNAi inC. elegans

Raman

Zaghab

Traver

et al. 2016

Preprint

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Long double-stranded RNA (dsRNA) can silence genes of matching sequence upon ingestion in many invertebrates and is therefore being developed as a pesticide. Such feeding RNA interference (RNAi) is best understood in the worm C. elegans, where it is thought that derivatives of ingested dsRNA, including short dsRNAs, move between cells and cause systemic silencing. Movement of short dsRNAs has been inferred using tissue-specific rescue of the long dsRNA-binding protein RDE-4 by expressing it from repetitive transgenes. We found that the use of repetitive transgenes for the tissue-specific rescue of a gene could inhibit RNAi within that tissue and could result in misexpression of the gene in other tissues. Both inhibition and misexpression were not detectable when a singlecopy transgene was used for tissue-specific rescue. In animals with single-copy rescue of RDE-4, RNAi was restricted to the tissue with RDE-4 expression. Thus, unlike previous observations using repetitive transgenes, these results suggest that binding of long dsRNA by RDE-4 in each silenced cell is required for systemic RNAi. Taken together with the requirement for long dsRNA to trigger RNAi in insects, these results suggest that the entry of long dsRNA is a necessary first step for feeding RNAi in animal cells.

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Reproducible features of small RNAs in C. elegans reveal NU RNAs and provide insights into 22G RNAs and 26G RNAs

Cited by 20 publications

References 38 publications

Neuronal Small RNAs Control Behavior Transgenerationally

Neuronal Small RNAs Control Behavior Transgenerationally

C. elegans ADARs antagonize silencing of cellular dsRNAs by the antiviral RNAi pathway

Each cell needs long double-stranded RNA for silencing by feeding RNAi inC. elegans

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