# High-throughput functional characterization of human enhancers

> **NIH NIH UM1** · CORNELL UNIVERSITY · 2020 · $750,521

## Abstract

PROJECT SUMMARY/ABSTRACT
Specific enhancers interact with promoters to specify the cellular pattern, timing, and levels of gene
expression. Enhancers can reside up to megabases away from their target gene promoters and strongly
activate transcription. Aim 1 will characterize active enhancer elements and their relationship to promoter
elements in vivo in human K562 (a tier 1 ENCODE cell line) by testing a broad array of Transcription
Regulatory Elements (TREs) for their enhancer activity using eSTARR-seq, our modified element-clone-
compatible STARR-seq assay. This collection of TREs will be selected based on a variety of criteria
established by ENCODE and others. Large numbers of selected TREs can be handled using our new Clone-
seq method, and then tested for enhancer activity by eSTARR-seq. For the TREs that have significant
enhancer activity, ~10,000 synthetic mutations will be generated that are designed to destroy distinct TF
binding motifs found within each enhancer. We will generate mutant clones using our en masse Clone-seq2
method and examine their impact on enhancer activity using eSTARR-seq. These data will be used to
understand the underlying molecular architecture and function of enhancers and promoters. Aim 2 generates
K562 cell lines using CRISPR/Cas9 that contain critical synthetic enhancer mutations identified in Aim 1. PRO-
seq assays can then be used to measure with high sensitivity and resolution the transcription at the variant
enhancers as well as all TREs and transcription units genome-wide. This will reveal the role of DNA sequence
motifs within native enhancer loci in the regulatory crosstalk with distal gene promoters and enhancers.
Circularized Chromosome Conformation Capture (4C) experiments with particular enhancers as the anchor
site will provide an unbiased analysis of distal interactions, while targeted ChIP-qPCR experiments will test
effects of these mutant enhancers on transcription factor binding and local histone marks at these genomic
points of enhancer interaction. Thus, Aim 2 rigorously characterizes mutated enhancers from Aim 1 in their
native chromatin environment. Aim 3 characterizes the de novo activation of enhancers, which are known to
be triggered by the heat shock activation of HSF1, a master regulator. Because the sequence motif, HSE, to
which HSF1 binds is well defined, targeted HSE mutations that cripple the enhancer activity will be made
immediately using CRISPR at native loci and the effects on transcription genome-wide can be analyzed
directly by PRO-seq. Additional critical motifs in these inducible enhancers will be identified in a less biased
way by the more laborious, but high-throughput, eSTARR-seq approach described in Aim 1. Finally, tracking
the kinetics with which the structural characteristics of these enhancers form in the minutes following heat
shock relative to the induced transcriptional activity as measured by PRO-seq allows assessment of which
characteristics (DNase I hypersensi...

## Key facts

- **NIH application ID:** 9904754
- **Project number:** 5UM1HG009393-04
- **Recipient organization:** CORNELL UNIVERSITY
- **Principal Investigator:** JOHN T LIS
- **Activity code:** UM1 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $750,521
- **Award type:** 5
- **Project period:** 2017-02-01 → 2023-01-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9904754

## Citation

> US National Institutes of Health, RePORTER application 9904754, High-throughput functional characterization of human enhancers (5UM1HG009393-04). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/9904754. Licensed CC0.

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