Mirounga angustirostris muscle raw transcriptome assembly

Raw assembly of northern elephant seal (Mirounga angustirostris) skeletal muscle transcriptome. Experimental Design: Skeletal muscle tissue for transcriptome sequencing was collected from three anesthetized juvenile northern elephant seals at three time points during an acute stress challenge experi...

Full description

Bibliographic Details
Main Authors: Khudyakov, Jane, Likit Preeyanon, Champagne, Cory, Ortiz, Rudy, Crocker, Daniel
Format: Dataset
Language:unknown
Published: figshare 2016
Subjects:
60604 Comparative Physiology
FOS Biological sciences
Champagne
Grinder
Ortiz
Elephant Seal
Elephant Seals
Online Access:https://dx.doi.org/10.6084/m9.figshare.2062518.v3
https://figshare.com/articles/dataset/Mirounga_angustirostris_raw_muscle_transcriptome/2062518/3
Description
Summary:Raw assembly of northern elephant seal (Mirounga angustirostris) skeletal muscle transcriptome. Experimental Design: Skeletal muscle tissue for transcriptome sequencing was collected from three anesthetized juvenile northern elephant seals at three time points during an acute stress challenge experiment: before 0.25 U/kg ACTH injection (“0 hr”), 2 hours after injection (“2 hr”), and 24 hours (“24 hr”) after injection. RNA Isolation: Tissue samples were stored at −80 °C until extraction. In the laboratory, 75–165 mg of muscle tissue were minced with a scalpel on ice, transferred to a glass tissue grinder (Kimble-Chase Kontes Duall, USA), and homogenized with 1 ml of TRIzol Reagent (Life Technologies, USA). RNA was extracted according to the manufacturer’s protocol and purified with the RNeasy mini kit including a 30-minute on-column DNase I digest (Qiagen, USA). RNA was treated with TURBO DNase I (Ambion, Life Technologies, USA) for 30 minutes according to manufacturer’s protocol. Phenol:chloroform:isoamyl alcohol (Affymetrix, USA) extraction was performed to remove DNase I. RNA concentration was quantified on a Qubit fluorometer (Life Technologies, USA). Total RNA integrity was evaluated using 2100 Bioanalyzer RNA 6000 kit (Agilent, USA). All RNA samples had integrity values (RIN) of 7.6 - 9.0. Library Preparation and Sequencing: Libraries for sequencing were prepared according to TruSeq protocol (Illumina, USA). Specifically, mRNA was isolated from total RNA samples using oligo-d(T)25 magnetic beads (Dynabeads: Invitrogen, USA) and used as template for first-strand cDNA synthesis. After double-stranded (ds) cDNA synthesis, overhang fragments were end-repaired by incubation in the presence of T4 DNA polymerase and Klenow polymerase. The polished fragments were phosphorylated by T4 PNK, followed by the addition of a single ‘A’ base to the 3′ end of the blunt-ended phosphorylated fragments. This ‘A’ base prepared the cDNA fragments for ligation to proprietary adapter oligonucleotides (Illumina, USA) that have a ‘T’ base at their 3′ end. Ligation products were subjected to a final PCR amplification step (8–10 cycles) before library quantification and validation. Individual libraries were prepared with barcode and all nine samples (biological triplicates of 0 hr, 2 hr, and 24 hr samples) were pooled for sequencing on one lane. Sequencing was carried out for 100 cycles on the Illumina HiSeq 2500 platform with paired-end 100 bp reads and library insert size of approximately 500 bp. The average number of reads generated per sample was 28.5 ± 7.5 million with total reads numbering 256 million, with 25.6 billion total bases and 66.3 GB of data. Fastq files were generated using the Illumina Casava pipeline v1.8.2. Assembly: Raw sequencing data were deposited at NCBI Sequence Read Archive under study accession [SRP045540]. Transcriptome assembly was performed using the Eel Pond mRNAseq Protocol (https://​khmer-protocols.​readthedocs.​org/​). Analysis was conducted in the cloud using an Amazon EC2 x-large machine (m1.xlarge), except for assembly, for which a 2x-large machine (m2.2xlarge) was required. Downloaded reads were trimmed of sequencing adapters and poor quality sequences using Trimmomatic v0.30 with TruSeq3-PE adapter sequences. Reads with quality scores Reference: Khudyakov JI, Preeyanon L, Champagne CD, Ortiz RM, Crocker DE. (2015) Transcriptome analysis of northern elephant seal (Mirounga angustirostris) muscle tissue provides a novel molecular resource and physiological insights. BMC Genomics 16: 64.

Similar Items