Three-Component Repurposed Technology for Enhanced Expression: Highly Accumulable Transcriptional Activators via Branched Tag Arrays

Kunii, Atsushi; Hara, Yoshihiro; Takenaga, Mitsumasa; Hattori, Naoko; Fukazawa, Takuya; Yamamoto, Takashi; Sakuma, Tetsushi

doi:10.1089/crispr.2018.0009

Cited by 31 publications

(25 citation statements)

References 25 publications

(36 reference statements)

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“…While allowing efficient changes in gene expression in various cellular contexts including human, mouse, and Drosophila models, the performance of each of the above mentioned systems varies greatly depending on target loci and cell types [ 133 ]. Many more variants have been designed since, including the three-component repurposed technology for enhanced expression (TREE) system, which combines SunTag with the RNA tethering system used by SAM in a tree-resembling structure [ 134 ].…”

Section: Targeted Epigenetic Editing With Dcas9mentioning

confidence: 99%

Chromatin Manipulation and Editing: Challenges, New Technologies and Their Use in Plants

Fal

Tomkova

Vachon

et al. 2021

IJMS

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An ongoing challenge in functional epigenomics is to develop tools for precise manipulation of epigenetic marks. These tools would allow moving from correlation-based to causal-based findings, a necessary step to reach conclusions on mechanistic principles. In this review, we describe and discuss the advantages and limits of tools and technologies developed to impact epigenetic marks, and which could be employed to study their direct effect on nuclear and chromatin structure, on transcription, and their further genuine role in plant cell fate and development. On one hand, epigenome-wide approaches include drug inhibitors for chromatin modifiers or readers, nanobodies against histone marks or lines expressing modified histones or mutant chromatin effectors. On the other hand, locus-specific approaches consist in targeting precise regions on the chromatin, with engineered proteins able to modify epigenetic marks. Early systems use effectors in fusion with protein domains that recognize a specific DNA sequence (Zinc Finger or TALEs), while the more recent dCas9 approach operates through RNA-DNA interaction, thereby providing more flexibility and modularity for tool designs. Current developments of “second generation”, chimeric dCas9 systems, aiming at better targeting efficiency and modifier capacity have recently been tested in plants and provided promising results. Finally, recent proof-of-concept studies forecast even finer tools, such as inducible/switchable systems, that will allow temporal analyses of the molecular events that follow a change in a specific chromatin mark.

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Section: Targeted Epigenetic Editing With Dcas9mentioning

confidence: 99%

Chromatin Manipulation and Editing: Challenges, New Technologies and Their Use in Plants

Fal

Tomkova

Vachon

et al. 2021

IJMS

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show abstract

“…For instance, the CRISPR-Sirius system can recruit 16 effector proteins through an engineered sgRNA scaffold with eight MS2 aptamers ( Figure 1 B) [ 47 ]. The TREE system, which combines the MS2 and SunTag systems, has the ability to recruit even more effector proteins ( Figure 1 B) [ 48 ]. With more deaminases recruited to genomic regions of interest, the editing window could be enlarged.…”

Section: Limitations and Future Prospectsmentioning

confidence: 99%

Full-Spectrum Targeted Mutagenesis in Plant and Animal Cells

Iaffaldano

Reiser

2021

IJMS

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Directed evolution is a powerful approach for protein engineering and functional studies. However, directed evolution outputs from bacterial and yeast systems do not always translate to higher organisms. In situ directed evolution in plant and animal cells has previously been limited by an inability to introduce targeted DNA sequence diversity. New hypermutation tools have emerged that can generate targeted mutations in plant and animal cells, by recruiting mutagenic proteins to defined DNA loci. Progress in this field, such as the development of CRISPR-derived hypermutators, now allows for all DNA nucleotides within user-defined regions to be altered through the recruitment of error-prone DNA polymerases or highly active DNA deaminases. The further engineering of these mutagenesis systems will potentially allow for all transition and transversion substitutions to be generated within user-defined genomic windows. Such targeted full-spectrum mutagenesis tools would provide a powerful platform for evolving antibodies, enzymes, structural proteins and RNAs with specific desired properties in relevant cellular contexts. These tools are expected to benefit many aspects of biological research and, ultimately, clinical applications.

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“…Three-component repurposed technology for enhanced expression (TREE) is a strong transcriptional activation system, which combines attraction of effectors by RNA aptamers and by protein tags ( Kunii et al, 2018 ). It consists of dCas9-VP64, sgRNA with two MS2 aptamers, SunTag fused with MS2 protein, and scFv-effector.…”

Section: Second Generation Crispra Systemsmentioning

confidence: 99%

Cell Reprogramming With CRISPR/Cas9 Based Transcriptional Regulation Systems

Shakirova

Ovchinnikova

Дашинимаев

2020

Front. Bioeng. Biotechnol.

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The speed of reprogramming technologies evolution is rising dramatically in modern science. Both the scientific community and health workers depend on such developments due to the lack of safe autogenic cells and tissues for regenerative medicine, genome editing tools and reliable screening techniques. To perform experiments efficiently and to propel the fundamental science it is important to keep up with novel modifications and techniques that are being discovered almost weekly. One of them is CRISPR/Cas9 based genome and transcriptome editing. The aim of this article is to summarize currently existing CRISPR/Cas9 applications for cell reprogramming, mainly, to compare them with other non-CRISPR approaches and to highlight future perspectives and opportunities.

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Three-Component Repurposed Technology for Enhanced Expression: Highly Accumulable Transcriptional Activators via Branched Tag Arrays

Cited by 31 publications

References 25 publications

Chromatin Manipulation and Editing: Challenges, New Technologies and Their Use in Plants

Chromatin Manipulation and Editing: Challenges, New Technologies and Their Use in Plants

Full-Spectrum Targeted Mutagenesis in Plant and Animal Cells

Cell Reprogramming With CRISPR/Cas9 Based Transcriptional Regulation Systems

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