2019
DOI: 10.1002/cpmb.105
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STARR‐seq and UMI‐STARR‐seq: Assessing Enhancer Activities for Genome‐Wide‐, High‐, and Low‐Complexity Candidate Libraries

Abstract: The identification of transcriptional enhancers and the quantitative assessment of enhancer activities is essential to understanding how regulatory information for gene expression is encoded in animal and human genomes. Further, it is key to understanding how sequence variants affect enhancer function. STARR‐seq enables the direct and quantitative assessment of enhancer activity for millions of candidate sequences of arbitrary length and origin in parallel, allowing the screening of entire genomes and the esta… Show more

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Cited by 62 publications
(88 citation statements)
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“…1A). A similar approach has been described, however in that case UMIs are introduced in a first PCR cycle after the reverse transcription step (Neumayr et al ., 2019). The introduction of UMIs allows one to distinguish between biological replicates and PCR duplicates that can dramatically distort the relative quantities of individual fragments within a library (Islam et al ., 2014).…”
Section: Resultsmentioning
confidence: 99%
See 1 more Smart Citation
“…1A). A similar approach has been described, however in that case UMIs are introduced in a first PCR cycle after the reverse transcription step (Neumayr et al ., 2019). The introduction of UMIs allows one to distinguish between biological replicates and PCR duplicates that can dramatically distort the relative quantities of individual fragments within a library (Islam et al ., 2014).…”
Section: Resultsmentioning
confidence: 99%
“…When we started our project, UMIs were not part of the STARR-seq protocol. However, in the meantime a similar approach has been proposed for low complexity libraries where UMIs are introduced in the first PCR cycle (Neumayr et al ., 2019). By applying UMIs, we could not only identify active enhancers, but also show that specific sequence features are associated with activity levels (Fig.…”
Section: Discussionmentioning
confidence: 99%
“…We observed some variability in amplicon RNA dropout across replicates, likely due to a combination of transduction efficiency variability across animals, sensitivity recapturing amplicons with low viral representation, and PCR stochasticity 52 . While not an obvious issue here, effect of PCR-based clonal amplification bias in other MPRAs has been shown to be reduced with the addition of barcodes and unique molecular identifiers to the reporter construct 53 . Amplicons in this assay were approximately ~900 bp long, representing some of the longer sequences tested in MPRAs to date.…”
Section: Discussionmentioning
confidence: 86%
“…No reuse allowed without permission. molecular identifiers to the reporter construct 53 . Amplicons in this assay were approximately ~900 bp long, representing some of the longer sequences tested in MPRAs to date.…”
Section: Discussionmentioning
confidence: 99%
See 1 more Smart Citation