2020
DOI: 10.1021/acssynbio.0c00119
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Engineering REST-Specific Synthetic PUF Proteins to Control Neuronal Gene Expression: A Combined Experimental and Computational Study

Abstract: Regulation of gene transcription is an essential mechanism for differentiation and adaptation of organisms. A key actor in this regulation process is the repressor element 1 (RE1)-silencing transcription factor (REST), a transcriptional repressor that controls more than 2000 putative target genes, most of which are neuron-specific. With the purpose of modulating REST expression, we exploited synthetic, ad hoc designed, RNA binding proteins (RBPs) able to specifically target and dock to REST mRNA. Among the var… Show more

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Cited by 5 publications
(7 citation statements)
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“…To achieve selectivity for specific endogenous mRNAs, it is desirable to use modified PUFs that can recognize longer sequences. [64,[67][68][69] Notably, PUFs can target RNAs in mitochondria, which cannot be achieved using CRISPR-Cas. [83] Although the presence of m 6 A has been reported in plant mitochondrial transcripts, [88,89] its presence in mammalian cells has not been observed, [90] but PUF has the potential to control mitochondrial RNA modifications.…”
Section: Pumilio and Fbf Homology Proteinmentioning
confidence: 99%
See 3 more Smart Citations
“…To achieve selectivity for specific endogenous mRNAs, it is desirable to use modified PUFs that can recognize longer sequences. [64,[67][68][69] Notably, PUFs can target RNAs in mitochondria, which cannot be achieved using CRISPR-Cas. [83] Although the presence of m 6 A has been reported in plant mitochondrial transcripts, [88,89] its presence in mammalian cells has not been observed, [90] but PUF has the potential to control mitochondrial RNA modifications.…”
Section: Pumilio and Fbf Homology Proteinmentioning
confidence: 99%
“…PUFs have not been used to control RNA modification in cells. To achieve selectivity for specific endogenous mRNAs, it is desirable to use modified PUFs that can recognize longer sequences [64,67–69] . Notably, PUFs can target RNAs in mitochondria, which cannot be achieved using CRISPR‐Cas [83] .…”
Section: How To Manipulate M6a Modifications At Specific Target Sites?mentioning
confidence: 99%
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“…By changing the amino acid pairs of a PUF repeat, artificial RNA-binding domains corresponding to various 8-nucleotide (nt) RNA sequences can be designed [9,21,22]. As the length of RNA recognized by PUFs (8-nt) is not enough to specify the target RNAs within a huge transcriptome, efforts to increase the length of the RNA-binding sequences have been applied by increasing the number of PUF repeats [21,[23][24][25][26]. Previous reports also showed the assembly of two PUF proteins in adjacent regions on the RNA to image specific transcripts [27][28][29][30].…”
Section: Introductionmentioning
confidence: 99%