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Sample GSM2672079 Query DataSets for GSM2672079
Status Public on Sep 21, 2017
Title C16.10 (RNA-Seq)
Sample type SRA
 
Source name Human Embryo
Organism Homo sapiens
Characteristics developmental stage: Blastocyst
embryo number: CRISPR 16
sample type: Single cell
Treatment protocol Human embryo microinjections were performed in Global Total media with HEPES under mineral oil on a heated stage with a holding pipet (Research Instruments) and a Femtojet 4i microinjection manipulator set at approximately 40 injection pressure and 20 constant pressure. Embryos were microinjected with a mixture of Cas9 protein plus sgRNA back-filled into microfilament glass capillary injection needles (World Precision Instruments #TW100F-6) pulled using a pipet puller (Suter P-97 micropipette puller). Control embryos were injected with Cas9 protein. Human embryos were cultured in drops of pre-equilibrated Global media (LifeGlobal # LGGG-20) supplemented with 5 mg/mL protein supplement (LifeGlobal # LGPS-605) and overlaid with mineral oil (Origio #ART-4008-5P). Pre-implantation embryos were incubated at 37oC and 5.5% CO2 in an EmbryoScope+ (Vitrolife) time-lapse incubator for 5-6 days (human).
Extracted molecule polyA RNA
Extraction protocol Single cells were isolated from blastocyst stage embryos (6-7 days post fertilisation) for subsequent analysis by micromanipulation, with a duration of less than 20 minutes. Embryos were placed in drops of G-MOPS solution (Vitrolife) on a petri dish overlaid with mineral oil. The plate was placed on a microscope stage (Olympus IX70) and the embryos were held with an opposing holding pipette and blastomere biopsy pipette (Research Instruments) using Narishige micromanipulators (Narishige, Japan). The biopsy mode of a Saturn 5 laser (Research Instruments) was used to separate the majority of the mural TE from the ICM and polar TE. The ICM and polar TE were washed quickly in PBS without Ca2+ and Mg2+ (Invitrogen) then placed in 0.05% trypsin/EDTA (Invitrogen) for 5 minutes at room temperature. Trypsin was quenched using Global Media supplemented with 5 mg/mL LifeGlobal Protein Supplement. After quenching, the cell clump was placed back on the stage in a drop of G-MOPS solution and pipetted up and down several times using the blastomere biopsy pipette.Single cells were picked using 100 μm inner diameter Stripper pipette (Origio) and transferred to individual low bind RNAse-free tubes containing 2.5 µl RLP plus buffer.
Samples were processed using a previously published protocol that was adapted where indicated (Macaulay et al. 2016).To separate RNA from gDNA 50 µl of Dynabeads were washed and incubated with 100 uM biotinylated poly-dT oligonucleotide (IDT). 10 µl of oligo-dT beads were added to each tube containing the single cell. Samples were incubated in a thermomixer for 20 min at room temperature at 2000 rpm. Tubes were put on a magnet until the beads collected into a pellet and the supernatant went clear. The supernatant containing the gDNA was transferred to a new collection tube. Beads were washed three times to collect any residual gDNA.cDNA was generated from the RNA captured on the bead using the SMARTer v4 Ultra Low Input kit. First strand cDNA was synthesised by adding 2 µl 5X Ultra low First strand buffer, 0.5 ul SMART-Seq v4 Oligo, 0.25 µl RNase Inhibitor, 6.25 µl Nuclease free water and 1 µl SMARTScribe Reverse Transcriptase to each sample. Reverse transcription was performed on the thermomixer using the settings 2 min at 42oC at 2000 rpm, 60 min at 42oC at 1500 rpm, 30 min at 50oCat 1500 rpm and 10 min at 60oCat 1500 rpm. cDNA was amplified by adding 12.5 μl 2X SeqAmp PCR buffer, 0.5 μl PCR Primer II A (12µM), 0.5 µl SeqAmp DNA polymerase, 1.5 μl Nuclease free water. Beads were mixed on thermomixer for 60 sec at room temperature at 2000 rpm and then were incubated on a PCR machine using the following settings: 95oC for 1 min, 24 cycles of 98oC for 10 sec, 65oC for 30 sec and 68oC for 3 min, before a final extension for 10 min at 72oC. Amplified cDNA was purified by adding 25 μl SPRI Ampure XP beads, mixing well and incubating at room temperature for 8 min to allow amplified cDNA to bind to the beads. Sample tubes were placed on the magnet and allowed to stand until all beads had been immobilised. Supernatant was removed and discarded and beads were washed twice by adding 200 µl freshly prepared 80% ethanol and leaving for 30 sec before discarding the supernatant. Tubes were spun briefly to collect residual liquid. The bead pellet was allowed to air dry. 12 µl of purification buffer was added to rehydrate the pellet and incubated for 2 min at room temperature. cDNA was eluted by pipetting up and down 10 times before returning the tube to the magnet. The clear supernatant containing the cDNA was removed from the immobilised beads and transferred to a new low-bind tube. cDNA was stored at -80°C until library preparation. cDNA quality was assessed by High Sensitivity DNA assay on an Agilent 2100 Bioanalyser with good quality cDNA showing a broad peak from 300 to 9000 bp. cDNA concentration was measured using QuBit dsDNA HS kit (Life Technologies UK Ltd.).Libraries with a molar concentration greater than 2nM were submitted for 100-bp paired-end sequencing on Illumina HiSeq 2000.
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina HiSeq 2000
 
Data processing TopHat2
Samtools
Htseq-count
Genome_build: GRCh38
Supplementary_files_format_and_content: RPKM values in csv document
 
Submission date Jun 19, 2017
Last update date May 15, 2019
Contact name Kathy Niakan
E-mail(s) [email protected]
Organization name The Francis Crick Institute
Street address Mill Hill
City London
ZIP/Postal code NW7 1AA
Country United Kingdom
 
Platform ID GPL11154
Series (2)
GSE100118 Uncovering mechanisms of early human lineage specification by CRISPR/Cas9-mediated genome editing [RNA-seq]
GSE100120 Uncovering mechanisms of early human lineage specification by CRISPR/Cas9-mediated genome editing
Relations
BioSample SAMN07252100
SRA SRX2931002

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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