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Sample GSM7889866 Query DataSets for GSM7889866
Status Public on Nov 09, 2023
Title 10nM FOXA1, Free Band, Rep 1
Sample type SRA
 
Source name FOXA1-unbound (free) synthetic oligonucleotide library at 10 nM FOXA1
Organism synthetic construct
Characteristics cell type: not applicable
treatment: 10 nM FOXA1
emsa band: Free Band
Extracted molecule other
Extraction protocol Synthetic oligonucleotide library was designed to include 3,203 different sequences, each 229bp in length with 193bp variable regions and 18bp primer-binding regions on the two sides. The synthetic oligo library was ordered from Agilent (Product #G7220A).
To amplify the synthetic oligonucleotide library sequences, we performed two rounds of PCR amplification with a BbsI digestion step in between. The primer pairs for the first round of PCR contain regions annealing to the CCND1e (outside the 193bp library sequence) at the 3’-ends, partial Illumina TruSeq adaptor sequences at the 5’-end and 0-3 random nucleotide spacers in between to increase sequence complexity. Primers with different numbers of spacers are mixed in equimolar ratio for the first round of PCR. Preliminary PCR tests were performed to decide the optimal cycle number that keeps the PCR reactions in exponential phase. We used 23-25 cycles for our first round of PCR. For the first round of PCR, 30 μl of ChIP DNA was amplified in a 100 μl PCR reaction using NEBNext Ultra II Q5 master mix. The PCR products were purified with AMPure XP beads with a beads to DNA ratio of 0.9. 15 μL of the purified PCR product was digested with 20 U of BbsI in a 30 μL reaction at 37°C for two hours. The digestion products were purified with AMPure XP beads with a beads to DNA ratio of 0.9, followed by the second round of PCR. The primer pairs for the second round of PCR contain the rest of the Illumina TruSeq adaptor sequences and sample indexes. For the second round of PCR, 2 μl of purified digestion product was amplified in a 50 μl PCR reaction for 8 cycles using NEBNext Ultra II Q5 master mix. The PCR products were purified with AMPure XP beads with a beads to DNA ratio of 0.8. Quality control was conducted with TapeStation (Agilent). 30 million paired-end 150bp reads were obtained for each sample using a NextSeq 2000 (Illumina) instrument.
 
Library strategy OTHER
Library source other
Library selection other
Instrument model NextSeq 2000
 
Data processing Basecalls were performed using DRAGEN BCL Convert (v3.8.4).
Paired-end reads were filtered using fastp (Version 0.23.2) according to default settings.
First three nucleotides were trimmed from each read using cutadapt to remove the 0-3 random nucleotides introduced by the amplicon primers.
Paired-end reads were aligned to a FASTA file containing all EMSA-seq library sequences in their forward and reverse orientation using BWA-MEM2
BAM alignments containing at least 2 mismatched nucleotides were filtered out using BAMtools
Number of sequences (counts) aligning to each library sequence were determined using the "count occurences of each record" tool in Galaxy
Assembly: hg38
Supplementary files format and content: Raw counts files including sequence ID (column 1), nucleotide sequence (column 2), and number of aligned reads or "counts" (column 3) in tabular format.
Library strategy: EMSA-seq
 
Submission date Nov 09, 2023
Last update date Nov 09, 2023
Contact name Lu Bai
E-mail(s) [email protected]
Organization name Penn State University
Street address 406 South Frear Building
City University Park
State/province PA
ZIP/Postal code 16802
Country USA
 
Platform ID GPL32628
Series (2)
GSE247431 Systematic Dissection of Sequence Features Affecting the Binding Specificity of a Pioneer Factor Reveals Binding Synergy Between FOXA1 and AP-1 [EMSA-seq]
GSE247432 Systematic Dissection of Sequence Features Affecting the Binding Specificity of a Pioneer Factor Reveals Binding Synergy Between FOXA1 and AP-1
Relations
BioSample SAMN38190523
SRA SRX22470839

Supplementary file Size Download File type/resource
GSM7889866_rawCounts_10nM_Free_Rep1.tabular.txt.gz 401.9 Kb (ftp)(http) TXT
SRA Run SelectorHelp
Raw data are available in SRA

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