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Sample GSM3582907 Query DataSets for GSM3582907
Status Public on Jun 04, 2019
Title L3 larvae brain MAPCap: male MLE9 mutant; replicate 2
Sample type SRA
 
Source name brain
Organism Drosophila melanogaster
Characteristics developmental stage: L3 larvae (3rd Instar)
genotype: MLE9 mutant
Sex: male
Growth protocol Fruit flies (Drosophila melanogaster) were reared on standard cornflour-molasses medium. at 25°C, 70% relative humidity and 12 hrs dark/12 hrs light cycle. mle9, cn, bw/CyO flies (BDSC #5873) have been ordered from the Bloomington Drosophila Stock Center (BDSC) and rebalanced with the help of w; CyO, Act5C-GFP/If to generate the w; mle9, cn, bw/CyO, Act5C-GFP flies used in this study.
Extracted molecule total RNA
Extraction protocol RNA from embryos was extracted using the Quick RNA Kit (Zymo Research). RNA from dissected brains of larvae was isolated using the DirectZol Kit (Zymo Research). RNA was eluted in 25 ul of RNase-free water.
See our manuscript for full protocol of MAPCap library construction
MAPCap: custom strategy explained in the manuscript. RNAseq: Illumina TRUseq
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection CAGE
Instrument model Illumina HiSeq 3000
 
Description MAPCap experiment performed on 3rd instar larvae
MAPCap_J-larvae_male_MLE9.deduplicated.bw
Data processing MAPCap reads were further demultiplexed using the barcodes present in R2 read. Barcodes and corresponding sample names are provided as MAPCap_embryo_barcodes.tsv and MAPCap_larvae_barcodes.tsv. No demultiplexing required for RNAseq
MAPCap: Paired-end FASTQ files were trimmed for adaptors using Trimmomatic 56 (v 0.3.7). Samples were de-multiplexed by icetea (v0.99, demultiplexFastq) using provided barcode information, and mapped to the dm6 genome using Rsubread 57 (v 1.22.3, mapping wrapper provided in icetea). For de-duplication, we consider all reads mapping to the same 5’-position and having the same random barcode as duplicates and only keep the first instance of each such alignment (using icetea - filterDuplicates). BigWigs were created using deepTools 58 (v3.0.2) bamCoverage and bamCompare, with the option `--offSet 1 --binSize 1`.
RNA-seq: data was processed using snakePipes RNA-seq pipeline 65 (v1.0.0 beta) using the options ` -m alignment,deepTools_qc --star_options --limitBAMsortRAM 60000000000 --outBAMsortingBinsN 30 dm6`. snakePipes performed alignment using STAR 66 (v2.6.1a), counting of reads on Ensembl GTF (release 79) via featureCounts 67 (v1.6.1), and quality-checks via deepTools 58 (v3.1.2). The gene-level counts obtained from featureCounts were then used for differential expression analysis via DESeq2 68 (v1.20.0).
Pipeline for processing MAPCap data is available at: https://github.com/vivekbhr/cage_pipeline
Pipeline for processing RNAseq data is available at: https://github.com/maxplanck-ie/snakepipes
Genome_build: dm6
Supplementary_files_format_and_content: bw, featureCounts, DESeq2 output
 
Submission date Jan 29, 2019
Last update date Jun 04, 2019
Contact name Asifa Akhtar
E-mail(s) [email protected]
Organization name Max Planck Institute of Immunobiology and Epigenetics
Department Chromatin Regulation
Lab Akhtar Lab
Street address Stuebeweg 51
City Freiburg
ZIP/Postal code 79108
Country Germany
 
Platform ID GPL23323
Series (1)
GSE125831 MAPCap enables high-resolution detection and differential expression analysis of transcription start sites
Relations
BioSample SAMN10840367
SRA SRX5306506

Supplementary data files not provided
SRA Run SelectorHelp
Raw data are available in SRA
Processed data are available on Series record
Processed data provided as supplementary file

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