Abstract
Recent research shows that short RNA molecules act as mobile signals that direct mRNA cleavage and DNA methylation in recipient cells.
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RNA silencing is a nucleotide-sequence-specific gene regulation mechanism that controls development, maintains heterochromatin and defends many eukaryotic organisms against viruses. It is a non-cell-autonomous process in flowering plants and in nematodes. In plants, RNA silencing generates a signal that spreads from the site of initiation to neighboring cells through channels called plasmodesmata that allow direct communication of molecules between adjacent plant cells. RNA silencing also spreads systemically over long distances through the phloem tissue, which translocates metabolites. Mobile silencing operates in a nucleotide-sequence-specific manner, which is consistent with the signal including an RNA component. However, until recently the identity of the mobile RNA species that silences gene expression was unknown. Recent research has conclusively shown that small non-coding RNA molecules (sRNA, which are 21 to 24 nucleotides (nt) in length) are components of mobile silencing. Here we review the genes and RNA molecules associated with mobile RNA silencing and discuss the implications and future directions of this recently discovered phenomenon.
RNA silencing in plants
sRNAs are generated from partially or perfectly double-stranded RNA (dsRNA) precursors by an RNase III-like nuclease called Dicer or Dicer-like (DCL). They are incorporated into another nuclease named Argonaute (AGO) and they use Watson-Crick base-pairing to guide the AGO complex to target nucleic acids. The targeting mechanism involves transcriptional regulation (DNA/histone methylation) or post-transcriptional regulation (mRNA cleavage/destabilization or translational inhibition) of the target sequence [1]. In some eukaryotes, including plants, RNA-dependent RNA polymerases (RDRs) can convert the targeted mRNAs into dsRNAs. As this process generates further substrates for DCL processing, RDRs have a vital role in the amplification of silencing RNAs and the production of secondary sRNAs [2].
In eukaryotic lineages the gene families encoding the core components of RNA silencing (DCLs, AGOs and RDRs) have expanded so that there are diversified silencing pathways that control the expression of endogenous genes, repeated sequences, transgenes and viruses [3]. The model plant Arabidopsis thaliana (thale cress) has four DCL proteins and ten AGO paralogs, which have distinct roles in a broad spectrum of endogenous RNA silencing pathways [4, 5].
The diversity of RNA silencing pathways in plants is illustrated by functions of the DCL family members. DCL1 produces 21-nt sRNAs called microRNAs (miRNAs) from a partly double-stranded region of imperfectly matched foldback RNAs [6, 7] to regulate the expression of mRNAs with complementary target sites (Figure 1a). DCL2 generates 22-nt small interfering RNAs (siRNAs) from double-stranded viral RNAs and transgenes [8, 9] (Figure 1c). DCL3 produces repeat-associated, transposon-specific and transgene-derived 24-nt siRNAs to induce changes in heterochromatin using precursor dsRNAs that are generated by the coordinated action of the plant-specific DNA-dependant RNA polymerase IV (POL IV) and RDR2 [10, 11] (Figure 1d). Finally, DCL4 produces 21-nt trans-acting siRNAs (tasiRNAs) from the non-coding transcripts of TAS genes that have been converted after a miRNA-mediated cleavage into dsRNAs by RDR6 [12, 13] (Figure 1b). These tasiRNAs act via AGO1 or AGO7 to control hormone response and leaf polarity [14]. DCL4 also produces siRNAs from viruses and transgenes [8, 15] (Figure 1c).
In some instances there is a crosstalk between the different RNA silencing pathways. For example, 22-nt miRNAs can initiate the production of tasiRNAs [16, 17]. In addition, siRNAs derived from perfect dsRNA can trigger secondary 24-nt siRNA production via the POL IV-RDR2-DCL3 pathway (Figure 1) [18].
Spreading of RNA silencing
Almost a century ago, Wingard [19] described a phenomenon in virus-infected plants that can now be explained through movement of the silencing signal. He found that lower leaves of tobacco plants infected with the tobacco ringspot virus showed strong symptoms of infection but the upper leaves remained asymptomatic and became resistant to subsequent infection with the same virus [19]. We now understand that this effect probably occurs because a mobile signal can move from the site of virus infection to distant tissues and can confer nucleotide-sequence-specific resistance.
Experiments in the 1990s showed that spatial spreading of RNA silencing occurs in plants expressing chitinase [20, 21], SAM synthase [22], nitrate reductase and nitrite reductase [23] transgenes. Systemic (long-distance) transmission of post-transcriptional gene silencing was revealed by a grafting experiment in which silencing of a nitrate reductase or nitrite reductase and/or a transgene encoding glucuronidase was transmitted from silenced rootstocks to non-silenced scions [24]. A similar phenomenon occurred when localized silencing of a green fluorescent protein (GFP) transgene initiated systemic silencing of GFP in transgenic plants [25, 26].
Research in the past decade indicated that movement of silencing over short distances (such as over 10 to 15 cells) [15, 27, 28] is distinct from long-distance transmission between tissues and organs through the phloem [24, 25, 27], because these processes can be selectively inhibited by viral silencing suppressors [27, 28] and by cadmium [29]. These findings suggest that the silencing signal might not be a single molecule and that the production, spread and perception of RNA silencing signal(s) may rely on multiple silencing pathways.
Identifying genes associated with mobile RNA silencing
Several genes associated with mobile RNA silencing have been identified by two groups, ours [30] and that of Olivier Voinnet [15, 28, 31], using independent genetic screens. Both groups expressed an inverted-repeat construct using the phloem-specific promoter from the SUC2 gene, which encodes a plasma-membrane sucrose-H+ symporter, to target the SULPHUR/CH42 (SUC-SUL) [28] or the PHYTOENE DESATURASE 3 (SUC-PDS) [30] (Figure 2) endogenous mRNAs. Expression of the construct produced a chlorotic or photobleaching phenotype that spread 10 to 15 cells beyond the vasculature in transgenic Arabidopsis plants. Using forward and reverse genetic approaches, both groups found that multiple silencing pathways control the production and spread of RNA silencing. A subset of the mutants recovered from the SUC-SUL silencing-signal screen [15, 28, 31] implicated a tasiRNA-like silencing process, and they indicate the potential crosstalk between the tasiRNA pathway and the production of a mobile silencing signal [15]. These tasiRNA mutants had a defective DCL4 protein, and the Voinnet group concluded that 21-nt siRNAs might be the mobile RNA signal [15]. However, this analysis did not rule out DCL4 acting on a mobile RNA intermediate or a long precursor in cells that receive the signal to produce 21-nt secondary siRNAs.
The SUC-SUL genetic screen [15, 28, 31] also recovered several mutants in the miRNA pathway that showed reduced silencing spread due to the loss or reduced activity of AGO1, DCL1, HEN1 (an sRNA methyltransferase [32]) and HYL1 (a nuclear dsRNA binding protein [33]). Intriguingly, the spreading phenotype was sensitive to mutations in RDR2 and NRPD1 (which encodes the largest subunit of POL IV), indicating an unexpected link between the RNA silencing mechanisms associated with spreading and heterochromatin silencing [31].
Our parallel SUC-PDS mutant screen [30] also revealed roles for a similar panel of genes in miRNA, tasiRNA and POL-IV-dependent siRNA pathways. In addition, this genetic screen [30] identified an SNF2-domain-containing protein (CLSY1) implicated in DNA methylation in the POL IV pathway, a THO/TREX complex protein likely to be involved in mRNA export in the tasiRNA pathway and a JmjC-domain-containing histone H3 lysine 4 demethylase (JMJ14) [30, 34, 35]. These proteins were not identified in the SUC-SUL screen [28]. More extensive screening will be needed to analyze the role of CLSY1, THO/TREX complex proteins and JMJ14 in the SUC-SUL system.
However, mutations of DCL3 and AGO4 have revealed an important difference between the SUC-SUL [15, 28, 31] and the SUC-PDS [30] system. Mutations of these genes in SUC-PDS have an enhanced silencing phenotype [30], whereas those in SUC-SUL have no effect [31]. This difference can be explained if the SUC-PDS transgene differs from SUC-SUL such that it is subject to self-silencing that is dependent on DCL3 and AGO4. Mutation of these genes would relieve the self-silencing so that greater transcription of the transgene would generate a more abundant dsRNA and silencing signal. This difference in self-silencing between the two transgene systems might be associated with the molecular architecture of the inverted repeat T-DNA constructs (a recombinant transgene cassette used to create transgenic Arabidopsis lines via Agrobacterium-mediated gene transfer). Alternatively, the chromosomal context of the transgene DNA could influence the likelihood of self silencing [36].
The main conclusion from these genetic screens [15, 28, 30, 31] is that multiple silencing pathways are associated with the mobile silencing phenotypes. These pathways or modules (a set of interacting proteins in the same pathway) might act either in parallel, sequentially or in opposition. The self-silencing pathway in SUC-PDS, for example, acts oppositely to the other modules. The POL IV module (Figure 1d and 2b,c) is likely to act sequentially to other components of the silencing pathways and to be involved in an amplification step. However, the screens do not provide spatial information and the different modules could function in various subcellular compartments or in the cells that either produce or receive the silencing signal. Thus, the POL IV module containing CLSY1, RDR2 and NRPD1 might operate in the nucleus to generate a dsRNA substrate for DCL [30].
Brosnan et al. [37] and our group [38] overcame the lack of spatial information by using grafted plants in which the tissue generating the signal was genetically distinct and physically separated from the recipient tissue. These studies monitored the movement of the signal using a GFP transgene as a reporter of RNA silencing [37, 38]. The results of Brosnan et al. [37] are partially consistent with the genetic screens showing that the POL IV(NRPD1)-RDR2-DCL3-AGO4 chromatin silencing pathway is required for the reception of long-distance silencing in the scion but not for the transmission of the silencing signal from the rootstock. However, unlike the SUC-SUL and SUC-PDS systems [15, 28, 30, 31], the grafting experiments [37, 38] revealed a requirement for RDR6 in cells that receive the silencing signal, probably as part of an amplification system. The different results from the SUC promoter systems and the grafting approach might be associated with the distinct mechanisms in long- and short-distance silencing signaling referred to earlier. The grafting systems are inevitably dependent on long-distance movement of the silencing signal, whereas the SUC-SUL and SUC-PDS systems might be dependent on short-distance cell-to-cell movement.
The sequential action of the silencing pathway modules in these mobile silencing systems resembles the involvement of multiple Dicers in antiviral defense [8, 39]. A likely scenario is that the antiviral defense also involves the mobile silencing signal, as in Wingard's early experiments [19], and perhaps that the different Dicers are in silencing modules acting sequentially in different cell types.
RNA species associated with the mobile silencing signal
Mobile RNA silencing is likely to have an RNA component because its effects are nucleotide-sequence-specific. In principle this mobile RNA could be the single-stranded sRNAs (21 to 24 nt), the immediate 21- to 24-nt sRNA precursors that exist in a double-stranded form, the longer dsRNAs that are processed into double-stranded sRNA by DCL, or long single-stranded RNA, but until recently the data were ambiguous.
In the Brosnan et al. GFP system [37], the long-distance spread of silencing was unaffected by mutations in individual Dicer genes in the silencing source, consistent with long RNAs being the mobile signal. However, Dicer family members are functionally redundant [8] and, formally, this analysis did not rule out conclusively that sRNAs are the mobile species.
An alternative system that we have recently set up [40] was based on grafting of wild-type shoots and mutant roots of A. thaliana plants. However, it differed from Brosnan and colleagues' approach [37] in that it used high-throughput sequencing (a sensitive and direct method) to detect mobile sRNA molecules. Using silencing pathway mutants with defective DCL2, DCL3 and DCL4, the enzymes required for the biogenesis of 22-nt and 24-nt siRNAs, as donor and recipient tissue, we demonstrated that transgene-derived and endogenous 22- to 24-nt siRNAs had moved across the graft union from the wild-type shoot to the mutant root [40]. Most of these mobile sRNAs were of the 24-nt size class that is associated with DNA methylation of targeted loci [40].
The identification of mobile 24-nt sRNA [40] is consistent with the analysis of viral suppressors on systemic silencing in Nicotiana benthamiana (a wild tobacco species) [27] and the presence of 24-nt sRNA in the phloem sap of oilseed rape [41] and pumpkin [42]. However, this result contrasts with the findings of the Voinnet group [43], who used the SUC-SUL transgenic system and concluded that 21-nt siRNAs are mobile. Their approach [43] was based on phloem-cell-specific rescue of DCL4 function and cell-specific inhibition of siRNA movement using the viral silencing suppressor P19, which sequesters 21-bp siRNA duplexes but not their longer dsRNA precursors. They also showed that the mechanically delivered, fluorescently labeled 21-nt and 24-nt siRNAs move from cell to cell and over long distances [43, 44]. Furthermore, the spreading of target gene silencing was associated with the movement of 21-nt siRNAs [43].
Other evidence is also consistent with movement of 21-nt sRNAs of various types. For example, artificial miRNAs (amiRNAs) can move short distances in leaves [45] or between the pollen vegetative cell cytoplasm and the sperm cells [46]. Endogenous 21-nt miRNAs could also be mobile between shoots and roots (miR399 [47]) and within the roots (miR165a and miR166b [48]). Endogenous 21-nt tasiRNAs can move from the adaxial (upper) to abaxial (lower) side of the leaf to influence leaf polarity and development [49, 50]. In addition, grafting experiments revealed that endogenous inverted repeat (IR71)-specific siRNAs of 21 nt, 22 nt and 24 nt are also mobile in Arabidopsis [44], although these experiments did not conclusively rule out that the sRNA precursors are the mobile form of RNA (Figure 3).
To reconcile these various results, we propose that in addition to multiple size classes of sRNA, sRNA precursors may be mobile and may contribute to the accumulation of newly processed sRNAs in the recipient tissues. Supporting this idea, in grafting experiments using a GFP silenced scion and a root deficient in GFP, we observed an increased abundance of 21-nt GFP sRNAs in wild-type root compared with a triple dcl2,dcl3,dcl4 mutant root that is unable to produce 22- to 24-nt sRNAs and certain 21-nt sRNAs [40]. This observation is consistent with a precursor GFP RNA moving to the root and being acted on by DCL4 in wild-type tissue.
What are the consequences of mobile silencing?
It is likely that the mobile forms of sRNA can direct the same diverse targeting mechanisms as do the non-mobile equivalents. Thus, the mobile 21-nt and 22-nt sRNAs are likely to regulate target gene expression post-transcriptionally via target mRNA cleavage [51]. Consistent with that idea, the physical movement of 21-nt siRNA coincided with the spread of target mRNA (GFP) silencing [43]. The mobile 22-nt sRNAs could induce mRNA cleavage or they could initiate the production of secondary siRNAs in an analogous manner to 22-nt miRNAs [16, 17].
Similarly, the 24-nt sRNAs can direct epigenetic modifications (DNA methylation) in the genome of the recipient cells [40], as do the non-mobile forms of this RNA [52–55]. However, there is evidence that the movement process is selective. Approximately 35% of sRNA loci produce mobile sRNA in our experimental system, and features of the genomic locus or the precursor molecule from which the sRNA is generated could perhaps determine whether the sRNA is mobile. Indeed, we found [40] a strong correlation between DNA methylation and the production of mobile sRNAs, consistent with an effect related to the epigenetic status of the locus. At the phosphoribosylanthranilate isomerase (PAI) locus (a natural inverted repeat) there was preferential movement of POL-IV-dependent over POL-IV-independent sRNAs. Features of the different sRNA precursors from loci producing mobile sRNAs or the cell type in which the sRNAs are generated could perhaps determine mobility [40]. Expression of sRNAs in the phloem, for example, is more likely to result in movement than epidermal expression. Channeling of sRNAs into cellular compartments from which extracellular movement might take place could also influence mobility. It is tempting to speculate that the recently discovered 24-nt miRNAs that are processed from miRNA precursors by DCL3 and direct the methylation of complementary DNA sequences [56] might be mobile and might follow similar spreading characteristics to those associated with mobile 24-nt siRNAs.
The size exclusion limit of plasmodesmata is probably high enough for sRNAs to spread from cell to cell [57]. However, the sensitivity of sRNA molecules to endogenous RNases might suggest that sRNAs move as part of a larger complex that protects them from degradation. We found a strong bias in mobility or stability of the sRNAs towards the coding strand of transgene sRNA and, to a lesser extent, of the mobile PAI sRNAs [40]. There was the same strand bias in the source and recipient tissue. The simplest interpretation of these observations is that the sRNAs move in single-stranded form, potentially associated with AGO or other proteins. By contrast, 21-nt siRNAs were found to move independently of AGO1 in dsRNA form in the SUC-SUL system [43].
Two independent sets of grafting experiments revealed that mobile sRNAs follow photosynthetic source-sink relationships, that is, that movement is more efficient from the shoot to the root than reciprocally [40, 44]. It is striking that the transgene-derived mobile sRNAs were very rare - as low as 10 parts per million - in the recipient tissues, but that they nevertheless have easily detectable effects [40]. To explain the potency of this effect in the GFP transgene systems, we propose that the mobile sRNA could initiate an amplification process involving RDRs and secondary RNA production in the recipient tissue [38]. Consistent with this idea, wild-type roots containing GFP mRNA accumulated 100-fold more GFP-specific sRNAs than the non-transformed roots deficient in DCL2, DCL3 and DCL4 [40]. Mobile sRNA might also initiate amplification via an epigenetic mark in the meristems (the initiating tissue for new organs in plants, consisting of undifferentiated cells) of recipient roots. Consistent with this idea, silencing of the GFP reporter gene appears first in the lateral roots, which emerge after silencing is initiated by grafting, rather than in the cells immediately adjacent to the graft junction [40].
Perspectives
Both 21-nt and 24-nt silencing RNAs have the potential to move from cell to cell and over long distances and they can direct mRNA cleavage and DNA methylation in recipient cells. The mobile 24-nt siRNAs associated with epigenetic modifications could have roles in genome defense and in the response to external stimuli as proposed previously for this size class of sRNAs associated with a transposon (Mu) [58, 59] and an inverted repeat (IR71) [44]. For example, these RNAs could be involved in transmitting signals to meristematic tissue to reinforce the epigenetic silencing of transposons, direct- and inverted-repeat DNA sequences. They might also mediate defense against DNA and RNA viruses in a similar manner to that in which RNA signals mediate suppression and meristem exclusion of RNA viruses [38, 60]. In responses to external stimuli, the mobile RNAs could transmit signals to the meristem to initiate epigenetic changes associated with adaptation to these stimuli. Epigenetic marks directed by sRNAs could, for example, be associated with competency to flower or responses to stress, two processes that have been linked to silencing RNAs [61–63]. It is also possible that the RNA silencing signal moves into the developing seed or pollen [46, 64] to induce epigenetic changes that ultimately initiate transgenerational effects to better adapt progeny to future stress [65]. Finally, mobile sRNAs might contribute to copying epigenetic marks from one allele to another.
The mobile sRNA loci identified so far could be used to develop new genetic screens to identify both the function of mobile sRNAs and the genetic factors involved in the mobility and induction of epigenetic changes. Combined with very sensitive high-throughput sequencing of RNA and DNA, this approach could help us to further understand the mobility and biological role of sRNAs and their precursor molecules.
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Acknowledgements
We thank Andrew Bassett for critically reading the manuscript. DCB is a Royal Society Research Professor. CWM is supported by the Natural Sciences and Engineering Research Council of Canada and the Cambridge Commonwealth Trust.
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Molnar, A., Melnyk, C. & Baulcombe, D.C. Silencing signals in plants: a long journey for small RNAs. Genome Biol 12, 215 (2011). https://doi.org/10.1186/gb-2010-11-12-219
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DOI: https://doi.org/10.1186/gb-2010-11-12-219