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Sample GSM8258931 Query DataSets for GSM8258931
Status Public on Jun 17, 2024
Title corn oil_1d_Male_STARRTYC6_RNA_replicate4
Sample type SRA
 
Source name liver
Organism Mus musculus
Characteristics tissue: liver
strain: Crl:CD1(ICR)
age at_euthanasia: 8-9 weeks
Sex: Male
treatment: corn oil, 1d
dosing regimen: Low Corn Oil
Treatment protocol In vivo transfection: Plasmid DNA to be delivered to each mouse was resuspended in TransIT-EE delivery solution (MIR 5340, Mirus, Inc, Madison, WI) in a final volume of ~3 ml, equivalent to 10% of the mouse body weight (vol/weight). Each mouse was injected with a volume corresponding to ~10% of the body weight, up a maximum of 3 ml (for mice > 30 g weight) and delivered within 5-8 seconds without appreciable resistance. Hydrodynamic injection was largely ineffective, as judged by Renilla luciferase activity assayed in liver extracts, when resistance to injection precluded delivery of the full volume or when the total time of injection exceeded 10 seconds. For STARR-seq studies, 15 ug of STARR-seq library plasmid DNA was mixed with 3 ug of Renilla reporter plasmid DNA was injected per mouse. TCPOBOP (1,4-bis(2-(3,5-dichloropyridyloxy))benzene) (Chem Cruze, cat. #SC-203291) was delivered to mice at 6 days after HDI using Low Corn Oil regimen. Low Corn Oil regimen: TCPOBOP was dissolved in DMSO at 7.5 mg/ml, and then diluted 10-fold into corn oil, followed by IP injection at 4 µl per g body weight (final dose: 3 mg TCPOBOP and 4 µl of 10% DMSO in corn oil, per kg body weight). Mice were euthanized 1 day after TCPOBOP or corn oil vehicle treatment for the groups. TCPOBOP or Vehicle injections were performed in the morning, and mice were euthanized between 10:30 AM and 12 noon under CO2 followed by cervical dislocation (Boston University animal facility light cycle: 7:30 AM to 7:30 PM). Livers were excised and flash frozen in liquid nitrogen then stored at -80° C.
Growth protocol Male and female CD1 mice (ICR strain), approx. 7 weeks old, were purchased from Charles River Laboratories (Wilmington, MA) and kept on a 12-hour light/dark cycle with food and water without restriction.
Extracted molecule polyA RNA
Extraction protocol The extraction methods, adapted from the published STARR-seq protocol (Neumayr, Pagani et al. 2019), were used in a nested PCR amplification protocol to characterize the transcriptional activity of each DHS sequence (putative regulatory region) to be assayed by HDI-STARR-seq: 1) a library prepared from DNA extracted from flash frozen liver tissue collected 7 d after in vivo transfection by HDI (primers ON8381, ON8382); and 2) a library prepared from the transcribed RNA (reporter sequences) extracted from each HDI-transfected liver (primers ON8379, ON8380; see STARR_seq_primer.txt). STARR-seq reporter plasmid DNA remaining in the liver 7 d after HDI was extracted using a commercial QIAprep spin miniprep kit (QIAgen, cat. # 27106). Liver tissue (200 mg frozen liver) was initially homogenized in 750 ul of QIAgen Buffer P1 using a rubber-tipped micropestle and passed through a 20G needle 3 times to homogenize large tissue pieces. The extracted plasmid DNA was bound to a QIAprep spin column, eluted in EB buffer and used as a PCR template in a subsequent nested PCR reaction using primers ON8381 and ON8382 (see STARR_seq_primer.txt). To extract transcribed reporter RNA, 120 ug of total liver RNA was isolated from 60-100 mg liver tissue from each mouse by TRIzol guanidinium thiocyanate-phenol-chloroform extraction then purified by polyA selection using oligo(dT) beads (New England Biolabs, cat. #E7490L). The transcribed RNA was digested with Turbo DNase I (Ambion, cat. # AM2238) at 37°C for 30 min, reverse transcribed using primer ON8731 (see STARR_seq_primer.txt) for STARR-seq RNA first strand synthesis and Superscript III first-strand synthesis supermix (Invitrogen, cat. # 18080-400) and treated with 10 mg RNase A per ml (Fermentas, cat. # EN0531) for 1 h at 37 Celsius. The cDNA obtained was purified using 1.8x SPRI beads then used as a PCR template in the nested PCR reaction.
The nested PCR reaction requires a set of primers that specifically targets DNA or RNA derived from a STARR-seq reporter, after which the sequences are amplified using Illumina dual index primers. A primer set, primers ON8381 and ON8382 (see STARR_seq_primer.txt) was designed to amplify the STARR-seq plasmid DNA libraries by specifically targeting the unspliced intron incorporated into the original plasmid and present in the plasmid and DNA libraries, but that is spliced out of the reporter RNA sequences. Another primer set, primers ON8379 and ON8380 (see STARR_seq_primer.txt) straddles the splice junction and was designed to specifically amplify only the transcribed and spliced RNA molecules. Subsequently, nested PCR was completed using NEBNext® Multiplex Oligos for Illumina (#E7600S) for all three library types (plasmid, DNA and RNA) to further amplify the material and attach Illumina i5 and i7 barcoded sequences used for multiplex sequencing on an Illumina sequencer.
 
Library strategy OTHER
Library source transcriptomic
Library selection other
Instrument model Illumina HiSeq 2500
 
Description polyA-selected RNA, stranded library
G187M08
Data processing READ MAPPING: reads were aligned to the mm9 mouse genome using Bowtie2 (Langmead et al 2009, Genome Biology) with default settings. Reads were filtered so that only uniquely-aligned reads were used for downstream analysis.
PEAK CALLING: 117,122 merged peaks were called using MACS2 (Zhang et al 2008, Genome Biology) from the associated plasmid, DNA, RNA libraries with default parameters without filtering for PCR duplicates. Peaks were filtered to remove ENCODE blacklisted regions (www.sites.google.com/site/anshulkundaje/projects/blacklists) and also regions called as peaks by MACS2 but contain only PCR duplicated reads. 50,332 MACS2 regions with more than 40 normalized squence reads in plasmid library (G170M6) were considered as qualified regions with reliable readout for in vivo STARR-seq assay.
READ COUNTING: Reads within 50,332 qualified genomic regions (>40 normalized sequence reads in plasmid library) were counted using the bedtools coverage option without filtering for PCR duplicates.
Assembly: mm9
Supplementary files format and content: G187_global_processed_dataset.xlsx. In vivo global STARR-seq assay of 50,322 qualified open chromatin (DHS) regions. These 50,322 qualified DHS sites are a subset of regions with more than 40 normalized reads from a 117,122 MACS2 peak list. Columns E-S show the raw normalized reads per 10 million mapped reads in the STARR-seq plasmid library, each DNA library extracted from each liver, and each RNA library prepared from each liver after HDI. Columns V-AA show the number of liver samples in the biological condition with at least 20 normalized RNA reads, and the averaged RNA counts in those qualified liver samples. For each biological condition (CTRL_M, CTRL_F and TCPO_M; columns AC-AE), we defined a set of active regions (regions with at least 20 sequence reads per 10 million mapped RNA reads in at least 3 out of 4 male livers, 3 out of 4 TCPOBOP-treated male livers, or 3 out of 3 female livers and a set of stringently inactive regions (regions with no more than 20 sequence reads per 10 million mapped RNA reads in 4 out of 4 male livers, 4 out of 4 TCPOBOP-treated male livers, or 3 out of 3 female livers) for the corresponding biological condition. "NA" in columns AB-AE indicate others.
Library strategy: STARR-seq
 
Submission date May 08, 2024
Last update date Jun 17, 2024
Contact name David J. Waxman
E-mail(s) djw@bu.edu
Organization name Boston University
Department Department of Biology and Bioinformatics Program
Street address 5 Cummington Mall
City Boston
State/province MA
ZIP/Postal code 02215
Country USA
 
Platform ID GPL17021
Series (2)
GSE267046 Global STARR-seq library profiling of open chromatin regions in livers of mice treated with the nuclear receptor CAR (Nr1i3) agonist ligand TCPOBOP, in livers of control male mice and in livers of control female mice. [G187_global]
GSE267205 STARR-seq reporter activity of plasmid libraries delivered to mouse liver by hydrodynamic injection: In vivo MPRA assay for enhancer activity
Relations
BioSample SAMN41271011
SRA SRX24501733

Supplementary data files not provided
SRA Run SelectorHelp
Raw data are available in SRA

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