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Sample GSM5195794 Query DataSets for GSM5195794
Status Public on May 23, 2021
Title Photoreceptor_H3K4me3_Rep4[CUT&Tag]
Sample type SRA
 
Source name Retina
Organism Drosophila melanogaster
Characteristics cell-type: Photoreceptor neuron
age: day 10 post eclosion
Sex: male
genotype: w;;P{w[+mC]=[UAS-GFP-Msp3 00KASH}attP2, P{ry[+t7.2]=rh1-GAL4}3, ry[506]
antibody: H3K4me3
Growth protocol Flies (genotype: w;;P{w[+mC]=[UAS-GFP-Msp300KASH}attP2, P{ry[+t7.2]=rh1-GAL4}3, ry[506]) were raised at 12:12 light:dark cycle at 25 degrees C on standard fly food. Following eclosion (day 1), they were aged for 10 with transfer to new food every other day.
Extracted molecule genomic DNA
Extraction protocol Male flies were harvested at indicated time point and heads were removed by freezing the flies in liquid nitrogen followed by five rounds of vortexing and freezing. RNA was extracted from isolated GFP-tagged photoreceptor nuclei using the method described in this manuscript
ChIP-seq libraries were made with Nugen Ovation Ultralow V2 using 2 ng of DNA as starting material. CUT&Tag librares were made following Epicypher protocol, including the IDT adapters, RNA-seq libraries were made with Nugen SoLo RNAseq system using 10 ng RNA as starting material. ATAC-seq libraries were made using IDT for Illumina primers Set A
 
Library strategy OTHER
Library source genomic
Library selection other
Instrument model Illumina NovaSeq 6000
 
Data processing Library strategy: CUT&Tag
Sanger/Illumina 1.9 used for base calling
Raw reads were trimmed to discard adapter reads and low quality reads (Q<30) using Trimmomatic settings: ILLUMINACLIP:TruSeq3-PE-2.fa:2:30:10 SLIDINGWINDOW:4:20 MINLEN:75. Additionally, Omni-ATAC and CUT&Tag reads included HEADCROP:10, and CROP:50 only for Omni-ATAC
For RNA-seq, cleaned reads were mapped to Drosophila melanogaster genome version dm6 using STAR with settings: --outSAMtype BAM SortedByCoordinate --quantMode GeneCounts
For Omni-ATAC, ChIP-seq and CUT&Tag, cleaned reads were mapped to Drosophila melanogaster genome version dm6 using Bowtie2 with settings: --sensitive
Samtools was used to convert SAM to BAM, sort and index corresponding BAM files.
Bigwig files were generated using deepTools subpackage bamCoverage, and bigwig files were analyzed using multiBigwigSummary, computeMatrix, plotCorrelation, plotProfile and plotHeatmap. Dm6 refGene GTF file was used for all analysis, available at UCSC
Differential expression analysis was performed using DESeq2. Peak calling was performed with MACS2 and peak annotation was performed using HOMER.
Genome_build: UCSC Aug. 2014 - BDGP Release 6 + ISO1 MT/dm6
 
Submission date Mar 22, 2021
Last update date May 23, 2021
Contact name Vikki M Weake
E-mail(s) vweake@purdue.edu
Organization name Purdue University
Department Biochemistry
Lab Weake lab
Street address 175 S University St
City West Lafayette
State/province Indiana
ZIP/Postal code 47907
Country USA
 
Platform ID GPL25244
Series (1)
GSE169328 In vivo tissue-specific chromatin profiling in Drosophila melanogaster using GFP-tagged nuclei
Relations
BioSample SAMN18422841
SRA SRX10412046

Supplementary file Size Download File type/resource
GSM5195794_CUTandTag_H3K4me3_R4.bw 29.1 Mb (ftp)(http) BW
SRA Run SelectorHelp
Processed data provided as supplementary file
Raw data are available in SRA

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