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Sample GSM4090263 Query DataSets for GSM4090263
Status Public on Sep 24, 2019
Title GABA_3
Sample type SRA
 
Source name Brainstem
Organism Petromyzon marinus
Characteristics treatment: GABA
ecotype: Spain: river Ulla
age: 5-7 years
Extracted molecule polyA RNA
Extraction protocol The brainstems of control and treated larvae were dissected out and immediately put in RNAlater (Ambion Inc., TX, USA). RNA extraction was performed using the RNeasy mini kit (Qiagen) with DNase treatment following the manufacturer’s instructions. Isolated RNAs were eluted in nuclease free water.
mRNA sequencing libraries were prepared from poly dT selected mRNA using the Illumina TrueSeq Stranded mRNA Library Preparation kit according to the manufacturer’s protocol.
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina HiSeq 4000
 
Description RNA-Seq of Petromyzon marinus: GABA-treated brainstem after spinal injury
Data processing Raw paired-end FASTQ files were quality filtered using Fastp to remove leading or trailing bases with Phred quality scores < 15 (-q 15), reads with length < 30 base pairs (-l 30), polyG tails (--trim_poly_g) and trim adaptor sequences (detected by per-read overlap, default).
Genome alignment: The resulting trimmed FASTQ files were aligned against the latest lamprey genome assembly (Pmar_germline 1.0) using STAR in 2-pass mapping mode (--twopassMode Basic) with the following parameters: 10 maximum multiple alignments allowed per read (--outFilterMultimapNmax 10), 10 maximum mismatches per read pair (--outFilterMismatchNmax 10), minimum and maximum intron lengths of 20 and 1M bp respectively (--alignIntronMin 20; --alignIntronMax 1000000), maximum distance of 1 Mb between mate reads (--alignMatesGapMax 1000000) and detection of chimerica sequences with a minimum mapped length of 20 bp (--chimSegmentMin 20; --chimScoreMin 1).
Transcriptome reconstruction: StringTie with default parameters (fr-firststrand, --rf) was used to construct the lamprey transcriptome for our samples using the genome alignment files.
Generation of read counts per gene: FeatureCounts was used to quantify gene expression at the gene level with the following parameters: fragments (paired-end reads) were counted instead of individual reads ('-p'), only fragments with both ends mapper were considered ('-B'), chimeric fragments were not considered ('-C'), and strand specified as reversely stranded ('-s 2').
Genome_build: Pmar_germline 1.0
Supplementary_files_format_and_content: Tab delimited text with raw read counts for each gene in the genome-guided de novo transcriptome (TSA submission GHVE00000000). The first six columns of the file correspond to gene ID, chromosome, start and end positions, strand and length of the gene
 
Submission date Sep 23, 2019
Last update date Sep 24, 2019
Contact name Diego Robledo
E-mail(s) diego.robledo@usc.es
Organization name University of Santiago de Compostela
Department Genetics
Street address Rúa Lope Gómez de Marzoa s/n CIBUS building
City Santiago de Compostela
ZIP/Postal code 15782
Country Spain
 
Platform ID GPL27509
Series (2)
GSE137859 RNA sequencing analysis of the sea lamprey brainstem after spinal cord injury and GABA or baclofen treatments [GABA]
GSE137860 RNA sequencing analysis of the sea lamprey brainstem after spinal cord injury and GABA or baclofen treatments
Relations
BioSample SAMN12607219
SRA SRX6736552

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

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