Argonaute-based programmable RNase as a tool for cleavage of highly-structured RNA

Dayeh, Daniel M.; Cantara, William A.; Kitzrow, Jonathan; Musier‐Forsyth, Karin; Nakanishi, K.

doi:10.1093/nar/gky496

Cited by 27 publications

(30 citation statements)

References 38 publications

(55 reference statements)

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“…Previous studies of eAgos and several mesophilic pAgos showed that mismatches between the guide and target strands may have large effects on the cleavage efficiency and precision ( 25 , 32 ). To study the effect of mismatches on target cleavage, we designed a set of DNA and RNA guides, each containing a single mismatched nucleotide at a certain position ( Supplementary Table S1 ), and tested them in the cleavage reaction with KmAgo (Figure 5 and Supplementary Figure S7 ).…”

Section: Resultsmentioning

confidence: 99%

“…Dayeh et al. reported that HIV-1 ΔDIS 5′UTR is a highly structured RNA (see Supplementary Table S2 ) ( 32 ). The HIV-1 ΔDIS 5′UTR was in vitro transcribed using T7 RNA polymerase and synthetic DNA templates carrying a T7 promoter sequence.…”

Section: Methodsmentioning

confidence: 99%

“…Transcripts used for cleavage assays was DNase I-treated and gel-purified. Guide DNAs (gDNAs) for experiments targeting the HIV-1 ΔDIS 5′UTR sequence ( Supplementary Table S3 ) were designed as described in ( 32 ) with minor modifications. Briefly, Dayeh et al.…”

Section: Methodsmentioning

confidence: 99%

See 2 more Smart Citations

A programmable omnipotent Argonaute nuclease from mesophilic bacteria Kurthia massiliensis

Liu¹,

Li²,

Jiang³

et al. 2021

Nucleic Acids Research

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Argonaute (Ago) proteins are conserved nucleic acid-guided proteins present in all domains of life. Eukaryotic Argonaute proteins (eAgos) are key players in RNA interference pathways and function as RNA-guided RNA endonucleases at physiological temperatures. Although eAgos are considered to evolve from prokaryotic Argonaute proteins (pAgos), previously studied pAgos were unable to catalyze RNA-guided RNA cleavage at physiological temperatures. Here, we describe a distinctive pAgo from mesophilic bacteria Kurthia massiliensis (KmAgo). KmAgo utilizes DNA guides to cleave single-stranded DNA (ssDNA) and RNA targets with high activity. KmAgo also utilizes RNA guides to cleave ssDNA and RNA targets at moderate temperatures. We show that KmAgo can use 5′ phosphorylated DNA guides as small as 9-mers to cut ssDNA and RNA, like Clostridium butyricum Ago. Small DNA binding confers remarkable thermostability on KmAgo, and we can suppress the guide-independent plasmid processing activity of empty KmAgo by elevating the DNA guide loaded temperature. Moreover, KmAgo performs programmable cleavage of double-stranded DNA and highly structured RNA at 37°C. Therefore, KmAgo can be regarded as a DNA-guided programmable omnipotent nuclease for cleaving most types of nucleic acids efficiently. This study broadens our understanding of Ago proteins and could expand the pAgo-based DNA and RNA manipulation toolbox.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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A programmable omnipotent Argonaute nuclease from mesophilic bacteria Kurthia massiliensis

Liu¹,

Li²,

Jiang³

et al. 2021

Nucleic Acids Research

View full text Add to dashboard Cite

show abstract

“…Our work should motivate studies to test other G analogues (especially non‐azide/alkyne initiators such as 5′‐hydrazinyl‐5′‐deoxyguanosine), and determine whether a common 10‐nt leader/initiating sequence rich in A, C, or U would afford high yields of RNAs initiated with different G analogues. The use of programmable RNases (e.g., Argonautes loaded with defined DNA guides) for site‐specific cleavage of large RNAs and the generation of smaller cleavage products bearing the 5′‐G analogue initiator also merits consideration.…”

Section: Figurementioning

confidence: 99%

An RNase P‐Based Assay for Accurate Determination of the 5′‐Deoxy‐5′‐azidoguanosine‐Modified Fraction of in Vitro‐Transcribed RNAs

et al. 2018

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Chemoenzymatic approaches are important for generating site-specific, chemically modified RNAs, a cornerstone for RNA structure-function correlation studies. T7 RNA polymerase (T7RNAP)-mediated in vitro transcription (IVT) of a DNA template containing the G-initiating class III Φ6.5 promoter is typically used to generate 5'-chemically modified RNAs by including a guanosine analogue (G analogue) initiator in the IVT. However, the yield of 5'-G analogue-initiated RNA is often poor and variable due to the high ratios of G analogue:GTP used in IVT. We recently reported that a T7RNAP P266L mutant afforded an approximately three-fold increase in fluorescent 5'-thienoguanosine-initiated pre-tRNA compared to the wild type T7RNAP. We have further explored the use of T7RNAP P266L to generate 5'-deoxy-5'-azidoguanosine ( G)-initiated RNA and found that the mutant yielded approximately four times more G-initiated pre-tRNA than the wild type in an IVT containing a 10:1 ratio of G:GTP. For accurate quantitation of the 5'- G-initiated RNA fraction, we employed RNase P, an endonuclease that catalyzes the removal of the 5'-leader in pre-tRNAs. Importantly, we show herein how RNase P can be leveraged for assessing 5'-G analogue incorporation in any RNA by rendering the target RNA, upon its binding to a customized external guide sequence RNA, into an unnatural substrate of RNase P. Such an approach in conjunction with T7RNAP P266L-based IVT should aid chemoenzymatic methods that are designed to generate 5'-chemically modified RNAs.

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“…Some truncated versions of approximately half the size (short Agos) exist in nature22 . We speculate that it will be possible to truncate them further as Ago-PAINT only relies on the property of pre-forming the helix structure of the imager strand and a variant from Kluyveromyces polysporus that contains only the C-lobe was reported to retain almost all the binding properties of the untruncated version 35.…”

mentioning

confidence: 99%

High-Speed Super-Resolution Imaging Using Protein-Assisted DNA-PAINT

Filius

Cui

Ananth

et al. 2020

Preprint

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Super-resolution imaging allows for visualization of cellular structures on a nanoscale level. DNA-PAINT (DNA Point Accumulation In Nanoscale Topology) is a super-resolutionmethod that depends on the binding and unbinding of DNA imager strands. The current DNA-PAINT technique suffers from slow acquisition due to the low binding rate of the imager strands. Here we report on a method where imager strands are loaded into a protein, Argonaute (Ago), that allows for faster binding. Ago pre-orders the DNA imager strand into a helical conformation, allowing for 10 times faster target binding. Using a 2D DNA origami structure, we demonstrate that Ago-assisted DNA-PAINT (Ago-PAINT) can speed up the current DNA-PAINT technique by an order of magnitude while maintaining the high spatial resolution. We envision this tool to be useful not only for super-resolution imaging, but also for other techniques that rely on nucleic-acid interactions.

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Argonaute-based programmable RNase as a tool for cleavage of highly-structured RNA

Cited by 27 publications

References 38 publications

A programmable omnipotent Argonaute nuclease from mesophilic bacteria Kurthia massiliensis

A programmable omnipotent Argonaute nuclease from mesophilic bacteria Kurthia massiliensis

An RNase P‐Based Assay for Accurate Determination of the 5′‐Deoxy‐5′‐azidoguanosine‐Modified Fraction of in Vitro‐Transcribed RNAs

High-Speed Super-Resolution Imaging Using Protein-Assisted DNA-PAINT

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