Literature DB >> 31230714

Programmable RNA-Guided RNA Effector Proteins Built from Human Parts.

Simone Rauch1, Emily He2, Michael Srienc3, Huiqing Zhou4, Zijie Zhang2, Bryan C Dickinson5.   

Abstract

Epitranscriptomic regulation controls information flow through the central dogma and provides unique opportunities for manipulating cells at the RNA level. However, both fundamental studies and potential translational applications are impeded by a lack of methods to target specific RNAs with effector proteins. Here, we present CRISPR-Cas-inspired RNA targeting system (CIRTS), a protein engineering strategy for constructing programmable RNA control elements. We show that CIRTS is a simple and generalizable approach to deliver a range of effector proteins, including nucleases, degradation machinery, translational activators, and base editors to target transcripts. We further demonstrate that CIRTS is not only smaller than naturally occurring CRISPR-Cas programmable RNA binding systems but can also be built entirely from human protein parts. CIRTS provides a platform to probe fundamental RNA regulatory processes, and the human-derived nature of CIRTS provides a potential strategy to avoid immune issues when applied to epitranscriptome-modulating therapies.
Copyright © 2019 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  RNA regulation; epitranscriptome; gene therapy; humanized CRISPR; synthetic biology

Mesh:

Substances:

Year:  2019        PMID: 31230714      PMCID: PMC6657360          DOI: 10.1016/j.cell.2019.05.049

Source DB:  PubMed          Journal:  Cell        ISSN: 0092-8674            Impact factor:   41.582


  82 in total

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3.  Tethered function assays: an adaptable approach to study RNA regulatory proteins.

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4.  Structure-activity relation of human beta-defensin 3: influence of disulfide bonds and cysteine substitution on antimicrobial activity and cytotoxicity.

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5.  A consensus epitope prediction approach identifies the breadth of murine T(CD8+)-cell responses to vaccinia virus.

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Review 6.  Precise hit: adeno-associated virus in gene targeting.

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7.  Identification of an RNA-silencing suppressor in the genome of Grapevine virus A.

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8.  Generating quantitative models describing the sequence specificity of biological processes with the stabilized matrix method.

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9.  Quantitative peptide binding motifs for 19 human and mouse MHC class I molecules derived using positional scanning combinatorial peptide libraries.

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  32 in total

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3.  Programmable C-to-U RNA editing using the human APOBEC3A deaminase.

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4.  REPAIRx, a specific yet highly efficient programmable A > I RNA base editor.

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Journal:  EMBO J       Date:  2020-10-15       Impact factor: 11.598

Review 5.  RNA N6-Methyladenosine and the Regulation of RNA Localization and Function in the Brain.

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Journal:  Trends Neurosci       Date:  2020-10-08       Impact factor: 13.837

6.  CRISPR-Cas12a exploits R-loop asymmetry to form double-strand breaks.

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Review 7.  RNA-targeting CRISPR systems from metagenomic discovery to transcriptomic engineering.

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8.  Evaluation of Engineered CRISPR-Cas-Mediated Systems for Site-Specific RNA Editing.

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Review 10.  On the functional relevance of spatiotemporally-specific patterns of experience-dependent long noncoding RNA expression in the brain.

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