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SRX23430828: GSM8043315: Far Right bin of Sort-seq on YFP/RFP ratio with mutational librar, replicate-1; Saccharomyces cerevisiae; OTHER
1 ILLUMINA (Illumina HiSeq 4000) run: 14.7M spots, 4.4G bases, 1.7Gb downloads

External Id: GSM8043315_r1
Submitted by: Molecular and Cell Biology, UC berkeley
Study: Defining the mechanisms and properties of post-transcriptional regulatory disordered regions by high-throughput functional profiling
show Abstracthide Abstract
Disordered regions within RNA binding proteins are required to control mRNA decay and protein synthesis. To understand how these disordered regions modulate gene expression, we surveyed regulatory activity across the entire disordered proteome using a high-throughput functional assay. We identified hundreds of regulatory sequences within intrinsically disordered regions and demonstrate how these elements cooperate with core mRNA decay machinery to promote transcript turnover. Coupling high-throughput functional profiling with mutational scanning revealed diverse molecular features, ranging from defined motifs to overall sequence composition, underlying the regulatory effects of disordered peptides. Machine learning analysis implicated aromatic residues in particular contexts as critical determinants of repressor activity, consistent with their roles in forming protein-protein interactions with downstream effectors. Our results define the molecular principles and biochemical mechanisms that govern post-transcriptional gene regulation by disordered regions and exemplify the encoding of diverse yet specific functions in the absence of well-defined structure. Overall design: We measured the post-transcriptional regulatory activity of thousands of disordered peptides using a Sort-Seq style approach in budding yeast
Sample: Far Right bin of Sort-seq on YFP/RFP ratio with mutational librar, replicate-1
SAMN39658582 • SRS20285124 • All experiments • All runs
Library:
Name: GSM8043315
Instrument: Illumina HiSeq 4000
Strategy: OTHER
Source: TRANSCRIPTOMIC
Selection: other
Layout: PAIRED
Construction protocol: After flow sorting, RNA was extract by phenol/choloroform followed by ethanol precipitation Libraries were prepared by constructing cDNA from total cellular mRNA using dT priming. Peptide constucts were amplifeid from cDNA with oJL090 and oJL109, followed by 2nd step amplification with indexing primers for illumina sequencing
Runs: 1 run, 14.7M spots, 4.4G bases, 1.7Gb
Run# of Spots# of BasesSizePublished
SRR2776595214,690,7994.4G1.7Gb2024-02-02

ID:
31661588

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