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Sample GSM3072382 Query DataSets for GSM3072382
Status Public on Sep 06, 2018
Title MII 120115_01 SPIA
Sample type SRA
 
Source name MII Oocyte
Organism Macaca mulatta
Characteristics tissue: oocyte
developmental stage: MII
library processing kit: SPIA
Growth protocol Control ovarian stimulation protocol (COS) was used for the collection of oocytes. Rhesus macaques were observed daily for signs of menses. Within day 1-4 of menses, animals were administered an intramuscular injection of recombinant macaque FSH (r-mFSH; National Hormone and Peptide Program, A. F. Parlow, UCLA) twice daily for a total of 7 days. On day 8 a subset of animals was used for collection of GV oocytes and another subset of animals were administrated an intramuscular injection of 1000 IU of human chorionic gonadotropin (hCG; LaJ olla Discount Pharmacy, La Jolla, CA). On day 9, ultrasound-guided needle aspiration of follicles was used for the collection of oocytes. Oocytes were observed for maturation status for both normal GV and MII, and FTM oocytes.
Extracted molecule total RNA
Extraction protocol All cumulus cells were removed by repeatedly pipetting oocytes with a narrow-gauge pipette that was just slightly larger than the oocytes while observing oocytes with a stereomicroscope. Using the PicoPureTM RNA Extraction kit, total RNA was isolated from each sample following the manufacturer protocol, including a DNAse digestion (RNase-Free DNase Set; Qiagen, Hilden, Germany) to remove any contaminating DNA.
SPIA libraries: 100 ng of each RNA sample was processed with the Ovation RNA-Seq System v2 using Ribo-SPIATM Technology (NuGen, San Carlos, CA). After this initial processing, a Covaris-2 sonicator was used to mechanically fragment the cDNA to an average of 300 bp. This was then followed by a brief S1 nuclease digestion as previously described (Head et al., 2011). After bead purification, the cDNA was processed through the Ovation Ultralow DR Multiplex Systems 1-16 (NuGen) for end repair, adaptor ligation and final library amplification.
SoLo libraries: cDNA libraries were produced with Nugen Ovation SoLo RNA-Seq(NuGEN, San Carlos, CA). After bead purification, the cDNA was processed: end repair, adaptor ligation and first round library amplification and purification. Then 20 ng of each library was used for the remainder of library preparation, which included use of InDA-C primers for rRNA depletion, as well as 2nd round library amplification and purification steps. SoLo Custom R1 primer was used instead of a standard Illumina R1 sequencing primer for the sequencing of the libraries.
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina HiSeq 2500
 
Data processing Illumina Real Time Analysis (RTA) v1.18.64 (SPIA libraries) & v2.7.6 (SoLo libraries)
Hisat2 to the Ensembl rhesus monkey genome (Mmul build v8.1.0, genome annotation relase-91)
Removing "ExAmp" duplicates with distance threshold 2500 using in-house developed Python code
DESeq2 comparisons between groups of libraries
Genome_build: Mmul 8.1.0 (Macaca Mulatta)
Supplementary_files_format_and_content: raw counts
 
Submission date Mar 30, 2018
Last update date Sep 06, 2018
Contact name Uros Midic
E-mail(s) uros@msu.edu
Organization name Michigan State University
Department Animal Sciences
Lab Latham lab
Street address 474 S. Shaw Lane
City East Lansing
State/province MI
ZIP/Postal code 48824-1225
Country USA
 
Platform ID GPL19129
Series (3)
GSE112534 Transcriptome analysis of rhesus monkey MII oocytes
GSE112536 Transcriptome analysis of rhesus monkey germinal vesicle, failed-to-mature oocytes and MII oocytes
GSE112537 Transcriptome analysis of rhesus monkey MII oocytes and embryos
Relations
BioSample SAMN08822754
SRA SRX3867036

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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