A general method for rapid and cost-efficient large-scale production of 5′ capped RNA

The promoter in HIV type 1 (HIV-1) proviral DNA contains three sequential guanosines at the U3-R boundary that have been proposed to function as sites for transcription initiation. Here we show that all three sites are used in cells infected with HIV-1 and that viral RNAs containing a single 5′ capped guanosine ( Cap 1G) are specifically selected for packaging in virions, consistent with a recent report [Masuda et al. (2015) Sci Rep 5:17680]. In addition, we now show that transcripts that begin with two or three capped guanosines ( Cap 2G or Cap 3G) are enriched on polysomes, indicating that RNAs synthesized from different transcription start sites have different functions in viral replication. Because genomes are selected for packaging as dimers, we examined the in vitro monomer-dimer equilibrium properties of Cap 1G, Cap 2G, and Cap 3G 5′-leader RNAs in the NL4-3 strain of HIV-1. Strikingly, under physiological-like ionic conditions in which the Cap 1G 5′-leader RNA adopts a dimeric structure, the Cap 2G and Cap 3G 5′-leader RNAs exist predominantly as monomers. Mutagenesis studies designed to probe for base-pairing interactions suggest that the additional guanosines of the 2G and 3G RNAs remodel the base of the PolyA hairpin, resulting in enhanced sequestration of dimerpromoting residues and stabilization of the monomer. Our studies suggest a mechanism through which the structure, function, and fate of the viral genome can be modulated by the transcriptionally controlled presence or absence of a single 5′ guanosine.HIV-1 | 5′-leader | transcription | RNA | structure

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“…1D). These RNA standards were prepared by in vitro transcription and were capped using a recombinant Vaccinia virus capping enzyme (37,38).…”

Section: Resultsmentioning

confidence: 99%

Transcriptional start site heterogeneity modulates the structure and function of the HIV-1 genome

Kharytonchyk

Monti

Smaldino

et al. 2016

Proc. Natl. Acad. Sci. U.S.A.

106

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“…To that end, we used a capped and fluorescently labeled RNA (Fuchs et al 2016), to which we added increasing amounts of Dcp1: Dcp2 RD + CD . We performed those experiments in the absence of Edc1 and in the presence of saturating amounts of Dcp1 is a dynamic hub for decapping regulators www.rnajournal.org 1367 Edc1 or Edc1 ΔYAG (Fig.…”

Section: Edc1 Interacts With Dcp1 and The Regulatory Domain Of Dcp2mentioning

confidence: 99%

“…Both RNAs were purified by denaturing anion exchange chromatography using a DNAPac PA100 column (22 × 250 mm, Dionex) at 80°C (Buffer A: 20 mM, Tris pH 8, 5 M Urea, Buffer B: as A plus 2 M NaCl). Afterward, the N7-methylguanosine cap was added to the 5 ′ end of the RNAs using vaccinia virus capping enzyme according to a recently published protocol (Fuchs et al 2016). The 30mer RNA was fluorescently labeled after capping using 5-(iodoacetamido)-fluorescein (Ramos and Varani 1998).…”

Section: Rna Preparationmentioning

confidence: 99%

The S. pombe mRNA decapping complex recruits cofactors and an Edc1-like activator through a single dynamic surface

Wurm

Overbeck

Sprangers

2016

RNA

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The removal of the 5 ′ 7-methylguanosine mRNA cap structure (decapping) is a central step in the 5 ′ -3 ′ mRNA degradation pathway and is performed by the Dcp1:Dcp2 decapping complex. The activity of this complex is tightly regulated to prevent premature degradation of the transcript. Here, we establish that the aromatic groove of the EVH1 domain of Schizosaccharomyces pombe Dcp1 can interact with proline-rich sequences in the exonuclease Xrn1, the scaffolding protein Pat1, the helicase Dhh1, and the C-terminal disordered region of Dcp2. We show that this region of Dcp1 can also recruit a previously unidentified enhancer of decapping protein (Edc1) and solved the crystal structure of the complex. NMR relaxation dispersion experiments reveal that the Dcp1 binding site can adopt multiple conformations, thus providing the plasticity that is required to accommodate different ligands. We show that the activator Edc1 makes additional contacts with the regulatory domain of Dcp2 and that an activation motif in Edc1 increases the RNA affinity of Dcp1:Dcp2. Our data support a model where Edc1 stabilizes the RNA in the active site, which results in enhanced decapping rates. In summary, we show that multiple decapping factors, including the Dcp2 C-terminal region, compete with Edc1 for Dcp1 binding. Our data thus reveal a network of interactions that can fine-tune the catalytic activity of the decapping complex.

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“…A strategy to reduce the stimulation of the immune system is the removal of the triphosphates of the 5 end of uncapped IVT mRNA by using a phosphatase [9,28]. On the other hand, there is the risk of reverse orientation of the cap analogues, which impede the binding to the CBP and the posterior translation [11,24,29]. As an alternative, an anti-reverse cap analogue (ARCA) has been developed [11,24].…”

Section: ' Capmentioning

confidence: 99%

Nanomedicines to Deliver mRNA: State of the Art and Future Perspectives

et al. 2020

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The use of messenger RNA (mRNA) in gene therapy is increasing in recent years, due to its unique features compared to plasmid DNA: Transient expression, no need to enter into the nucleus and no risk of insertional mutagenesis. Nevertheless, the clinical application of mRNA as a therapeutic tool is limited by its instability and ability to activate immune responses; hence, mRNA chemical modifications together with the design of suitable vehicles result essential. This manuscript includes a revision of the strategies employed to enhance in vitro transcribed (IVT) mRNA functionality and efficacy, including the optimization of its stability and translational efficiency, as well as the regulation of its immunostimulatory properties. An overview of the nanosystems designed to protect the mRNA and to overcome the intra and extracellular barriers for successful delivery is also included. Finally, the present and future applications of mRNA nanomedicines for immunization against infectious diseases and cancer, protein replacement, gene editing, and regenerative medicine are highlighted.

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A general method for rapid and cost-efficient large-scale production of 5′ capped RNA

Cited by 72 publications

References 68 publications

Transcriptional start site heterogeneity modulates the structure and function of the HIV-1 genome

Transcriptional start site heterogeneity modulates the structure and function of the HIV-1 genome

The S. pombe mRNA decapping complex recruits cofactors and an Edc1-like activator through a single dynamic surface

Nanomedicines to Deliver mRNA: State of the Art and Future Perspectives

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