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SRX22794545: GSM7937546: 20231012_KSA075_NCIH1048_DMSO_rep7; Homo sapiens; ATAC-seq
1 ILLUMINA (NextSeq 500) run: 53.6M spots, 4.1G bases, 1.6Gb downloads

External Id: GSM7937546_r1
Submitted by: Kadoch Lab, Pediatric Oncology, Dana Farber Cancer Institute
Study: Non-Canonical BAF and mSWI/SNF Regulates POU2F3 and are Selective Targetable Dependencies for POU2F3-Positive Small Cell Lung Cancer
show Abstracthide Abstract
~12% of SCLCs are marked by the lineage transcription factor POU2F3, which is essential in all POU2F3-positive SCLCs. Thus, approaches to directly or indirectly inhibit POU2F3 could lead to new therapeutic strategies for POU2F3-positive SCLCs. Here we use a positive selection screening strategy where endogenous POU2F3 is fused to the suicide gene DCK*. Cells that express endogenous POU2F3-DCK* are killed in the presence of the nucleoside analog BVdU and only cells that downregulate the POU2F3-DCK* fusion survive. Genome-wide CRISPR/Cas9 resistance screens with BVdU in POU2F3-DCK* cells uncovered that inactivation of SMARCD1 or BRD9, both components of the non-canonical BAF (ncBAF) complex, markedly downregulate endogenous POU2F3. We find that all POU2F3-positive SCLC cell lines relative to ASCL1-positive and NEUROD1-positive cell lines, are exquisitely sensitive to mSWI/SNF complex inhibition using SMARCA2/4 inhibitors; while pure non-neuroendocrine POU2F3-positive SCLC cell lines are highly sensitive to ncBAF complex inhibition using highly selective BRD9 degraders. Mechanistically, BRD9 binds and regulates POU2F3 target genes including POU2F3 itself. BRD9 degraders or SMARCA2/4 inhibitors robustly decrease accessibility of POU2F3 target genes effectively shutting off POU2F3 function. Moreover, BRD9 degraders or SMARCA2/4 inhibitors decrease tumor growth and increase survival of mice bearing non-neuroendocrine POU2F3 xenografts. This works shows that mSWI/SNF and ncBAF tightly regulate POU2F3 expression and activity and nominate mSWI/SNF or ncBAF inhibition as druggable therapeutic strategies to selectively target POU2F3-positive SCLCs. Overall design: To investigate the relationship between POU2F3 and mSWI/SNF activity in POU2F3+ small cell lung cancer (SCLC), we assess the gene expression and chromatin accessibility effects across 4 POU2F3+ SCLC lines treated with FHD286, which is a selective SMARCA2/4 inhibitor. We performed RNA-seq and ATAC-seq on NCIH211, CORL311, NCIH526, and NCIH1048 treated with either DMSO or 100nM FHD286 for 72 hours. To understand how non-neuroendocrine POU2F3+ SCLC are sensitive to ncBAF activity, we assessed the gene expression and chromatin accessibility effects on NCIH211 and NCIH1048 treated with either DMSO or FHD609, which is a specific bromodomain-targeting PROTAC for BRD9. We performed RNA-seq and ATAC-seq on NCIH211 and NCIH1048 treated with either DMSO or 100nM FHD609 for 72 hours. We assessed how POU2F3 binding is affected by SMARCA2/4 inhibition or BRD9 degradation. We performed POU2F3, RPB1, H3K27ac, and BRD9 ChIP-seq in NCIH1048 treated with DMSO or FHD286. We also performed POU2F3 and H3K27ac ChIP-seq in NICH1048 treated with FHD609.
Sample: 20231012_KSA075_NCIH1048_DMSO_rep7
SAMN38689221 • SRS19778559 • All experiments • All runs
Organism: Homo sapiens
Library:
Name: GSM7937546
Instrument: NextSeq 500
Strategy: ATAC-seq
Source: GENOMIC
Selection: other
Layout: PAIRED
Construction protocol: For ChIP-Seq: Cells were fixed with 2mM DSG 40min RT then 1.0% PFA 10min RT, then sonicated for 12 minutes For ATAC-Seq: 200K cells were incubated in hypotonic buffer and lysis buffer, then were resuspended in transposase reaction mixture for 30 min at 37°C with gentle shaking followed by DNA purification and 8 cycles of amplification For RNA-Seq: All RNA was collected using the RNeasy Mini Kit (Qiagen). RNA-seq libraries were prepared using the Nebnext Poly(A) mRNA Magnetic Isolation Module and the Nebnext Ultra II Directional RNA Library Prep Kit for Illumina using standard protocols ChIP-seq libraries were prepared with Illumina's NEBNext Ultra II DNA library Prep Kit using standard protocols. ChIP-seq was sequenced on Illumina NextSeq 500 using 37 bp pair-end sequencing parameters. ATAC-seq samples were sequenced on NextSeq 500 (Illumina) or NovaSeq 6000 (Illumina) using 37 bp pair-end sequencing parameters. RNA-seq libraries were prepared using the Nebnext Poly(A) mRNA Magnetic Isolation Module and the Nebnext Ultra II Directional RNA Library Prep Kit for Illumina using standard protocols. RNA was sequenced on NextSeq 6000 (Illumina) using 37 bp pair-end sequencing parameters.
Runs: 1 run, 53.6M spots, 4.1G bases, 1.6Gb
Run# of Spots# of BasesSizePublished
SRR2710535053,584,3924.1G1.6Gb2024-05-23

ID:
30832032

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