Determination of in vivo RNA structure in low-abundance transcripts

Kwok, Chun Kit; Ding, Yiliang; Tang, Yin; Assmann, Sarah M.; Bevilacqua, Philip C.

doi:10.1038/ncomms3971

Cited by 117 publications

(146 citation statements)

References 45 publications

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“…In some cases, the resulting models have disagreed with accepted structures (Quarrier et al 2010;Kladwang et al 2011c;Hajdin et al 2013;Sükösd et al 2013;Rice et al 2014), motivating efforts to estimate uncertainty (Kladwang et al 2011c;Ramachandran et al 2013), to incorporate alternative mapping strategies (Cordero et al 2012a;Kwok et al 2013), and to integrate mapping with systematic mutagenesis (mutate-and-map [M 2 ]) (Kladwang and Das 2010;Kladwang et al 2011a,b;Cordero et al 2014). Even these improvements do not provide routes to validation through independent experiments, and structure inferences remain under question (Wenger et al 2011).…”

Section: Introductionmentioning

confidence: 99%

High-throughput mutate-map-rescue evaluates SHAPE-directed RNA structure and uncovers excited states

Tian

Cordero

Kladwang

et al. 2014

RNA

101

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The three-dimensional conformations of noncoding RNAs underpin their biochemical functions but have largely eluded experimental characterization. Here, we report that integrating a classic mutation/rescue strategy with high-throughput chemical mapping enables rapid RNA structure inference with unusually strong validation. We revisit a 16S rRNA domain for which SHAPE (selective 2 ′ -hydroxyl acylation with primer extension) and limited mutational analysis suggested a conformational change between apo-and holo-ribosome conformations. Computational support estimates, data from alternative chemical probes, and mutate-and-map (M 2 ) experiments highlight issues of prior methodology and instead give a nearcrystallographic secondary structure. Systematic interrogation of single base pairs via a high-throughput mutation/rescue approach then permits incisive validation and refinement of the M 2 -based secondary structure. The data further uncover the functional conformation as an excited state (20 ± 10% population) accessible via a single-nucleotide register shift. These results correct an erroneous SHAPE inference of a ribosomal conformational change, expose critical limitations of conventional structure mapping methods, and illustrate practical steps for more incisively dissecting RNA dynamic structure landscapes.

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Section: Introductionmentioning

confidence: 99%

High-throughput mutate-map-rescue evaluates SHAPE-directed RNA structure and uncovers excited states

Tian

Cordero

Kladwang

et al. 2014

RNA

101

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“…DMS has been used both inside and outside the cell to study RNA structure, RNA-protein interactions, and even RNA structure changes that result in ligand binding (Kwok et al 2013;Rouskin et al 2014;Fang et al 2015). Although very useful, DMS suffers from the drawback of having nucleotide specificities, limiting its resolution as a general RNA structure probe.…”

Section: Introductionmentioning

confidence: 99%

Comparison of SHAPE reagents for mapping RNA structures inside living cells

Lee

Flynn

Kadina

et al. 2016

RNA

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Recent advances in SHAPE technology have converted the classic primer extension method to next-generation sequencing platforms, allowing transcriptome-level analysis of RNA secondary structure. In particular, icSHAPE and SHAPE-MaP, using NAI-N 3 and 1M7 reagents, respectively, are methods that claim to measure in vivo structure with high-throughput sequencing. However, these compounds have not been compared on an unbiased, raw-signal level. Here, we directly compare several in vivo SHAPE acylation reagents using the simple primer extension assay. We conclude that while multiple SHAPE technologies are effective at measuring purified RNAs in vitro, acylimidazole reagents NAI and NAI-N 3 give markedly greater signals with lower background than 1M7 for in vivo measurement of the RNA structurome.

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“…3a). Importantly, essentially the same conformation was obtained when NMIA was replaced by NAI, the alternative acylating reagent used for in vivo SHAPE [26,40,41] (Fig. 3b).…”

Section: Resultsmentioning

confidence: 81%

“…Between the remaining two members of Avsunviroidae, the eggplant latent viroid (ELVd) [35] and ASBVd [11], we chose the latter because despite its natural host being a woody plant, the isolate of this viroid, which we have been working with over the years (GenBank accession number J02020 with the substitution C213fiU), accumulates in vivo to levels comparable to the 5S ribosomal RNA [12,21], much higher than those reached by ELVd in eggplant. There are modifications more sensitive than conventional SHAPE [40,46], but some entail additional steps, particularly single-stranded adapter ligation, which limit the reliability of the results. These approaches, however, particularly SHAPE-MaP [46], may become indispensable with viroids reaching low titres in vivo.…”

Section: Discussionmentioning

confidence: 99%

“…Moreover, this reagent has been previously applied to determine the structure in planta of a chloroplast mRNA of Arabidopsis thaliana [40], thus indicating that NAI can traverse the membrane of this organelle. In vivo SHAPE of the mc ASBVd (+) form showed that it accumulates in chloroplasts as a free RNA uncovered by tightly bound host protein(s) which, like viral coat proteins, might exert a protecting role.…”

Section: Discussionmentioning

confidence: 99%

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The predominant circular form of avocado sunblotch viroid accumulates in planta as a free RNA adopting a rod-shaped secondary structure unprotected by tightly bound host proteins

López-Carrasco

Flores

2017

Journal of General Virology

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Avocado sunblotch viroid (ASBVd), the type member of the family Avsunviroidae, replicates and accumulates in chloroplasts. Whether this minimal non-protein-coding circular RNA of 246-250 nt exists in vivo as a free nucleic acid or closely associated with host proteins remains unknown. To tackle this issue, the secondary structures of the monomeric circular (mc) (+) and (À) strands of ASBVd have been examined in silico by searching those of minimal free energy, and in vitro at single-nucleotide resolution by selective 2¢-hydroxyl acylation analysed by primer extension (SHAPE). Both approaches resulted in predominant rod-like secondary structures without tertiary interactions, with the mc (+) RNA being more compact than its (À) counterpart as revealed by non-denaturing polyacryamide gel electrophoresis. Moreover, in vivo SHAPE showed that the mc ASBVd (+) form accumulates in avocado leaves as a free RNA adopting a similar rod-shaped conformation unprotected by tightly bound host proteins. Hence, the mc ASBVd (+) RNA behaves in planta like the previously studied mc (+) RNA of potato spindle tuber viroid, the type member of nuclear viroids (family Pospiviroidae), indicating that two different viroids replicating and accumulating in distinct subcellular compartments, have converged into a common structural solution. Circularity and compact secondary structures confer to these RNAs, and probably to all viroids, the intrinsic stability needed to survive in their natural habitats. However, in vivo SHAPE has not revealed the (possibly transient or loose) interactions of the mc ASBVd (+) RNA with two host proteins observed previously by UV irradiation of infected avocado leaves.

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Determination of in vivo RNA structure in low-abundance transcripts

Cited by 117 publications

References 45 publications

High-throughput mutate-map-rescue evaluates SHAPE-directed RNA structure and uncovers excited states

High-throughput mutate-map-rescue evaluates SHAPE-directed RNA structure and uncovers excited states

Comparison of SHAPE reagents for mapping RNA structures inside living cells

The predominant circular form of avocado sunblotch viroid accumulates in planta as a free RNA adopting a rod-shaped secondary structure unprotected by tightly bound host proteins

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