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Sample GSM1576198 Query DataSets for GSM1576198
Status Public on Mar 02, 2023
Title 13h post ICSI single zygote injected control mcherry cRNA-replicate-04
Sample type RNA
 
Source name single cell whole transcriptome amplification
Organism Mus musculus
Characteristics developmental stage: 13h post ICSI single zygote
injected: control mcherry cRNA
strain: B6D2F1
Treatment protocol ICSI using sperm from 8 to 12 weeks old B6D2F1 males was essentially as previsously described (Suzuki et al., 2010).
Growth protocol The Oocytes incubated in kalium simplex optimized medium under mineral oil in humidified 5% CO2 (v/v air) at 37°C, until required (Yoshida et al, 2007).
Extracted molecule total RNA
Extraction protocol It was based on isolation of the cellular mRNA by oligo-dT beads, cDNA synthesis using random octamer and oligo-dT primers, poly-dG tailing, and PCR amplification using a single primer under very stringent conditions adequate for CG-rich sequences. The solid-phase capturing of the mRNA enabled depleting the cDNA from free cDNA synthesis pri- mers and abundant dNTPs thus avoiding the subsequent amplification of tailed primers or inefficient tailing. Together with the introduction of random primers (resulting in a fragmentation of the cDNA to a size amplifiable by PCR) the protocol therefore allowed for optimal conditions of all enzymatic reactions such as high concentrations of dNTPs, primer and enzyme, all of which were individually shown to contribute to increased sensitivity. The highest increase of sensitivity (100-fold) over the original Brady procedure was achieved by the use of poly-G tailing instead of poly-A tailing and the subsequent use of a single poly-C-containing primer. Our methods were based on (Hartmann and Klein, 2006) and further improved to apply for extraction of total RNA from mouse single cells.
Label biotin
Label protocol Primary cDNA amplification products were labelled in the presence of 3% formamide, 2.4 mM CP2-BGL primer (TCA-GAATTCATGCCGCCCCCCCGGCCC), dNTPs (0.35 mM dATP and dGTP, 0.3 mM dTTP and dCTP) and 0.05 mM labelled nucleotides. Sample cDNA was labelled with digoxygenin-dUTP (Roche) and aminodigoxygenin-dCTP (PerkinElmer, Rodgau-Ju ̈ gesheim), reference cDNA with biotin-dUTP (Roche) and biotin-dCTP (Invitrogen).
 
Hybridization protocol Corning, Schiphol-Rijk, Netherlands) were prehybridized with 5xSSC + 0.1% SDS + 0.1% BSA at 42C and hybridized in an Arraybooster hybstation (Implen, Munich) at 42C overnight. Washing steps following hybridization were at 50C twice in 1· SSC + 0.1% SDS for 10 min, twice in 0.5x SSC + 0.1% SDS for 10 min, and twice in 0.1x SSC for 30 min. Unspecific binding of labelled proteins was blocked with 1% blocking reagent for nucleic acid hybridization (Roche) followed by a staining procedure with anti-Dig-Cy5 and Streptavidin-Cy3 (each 16 mg/ml, Jackson Laboratories). Excess antibody/streptavidin was removed with 4x SSC + 0.2% Tween-20 and slides were scanned on a Genepix 4000A scanner (Axon Instruments, Union City). Experiments shown in Table 2 were performed using human cells hybridized to Human Genome OpArrays version 4. Protocol details are available upon request.
Scan protocol Slides were scanned on GenePix 4000A scanner Axon Instruments, Union City). Numerical readout of fluorescence intensities (GPR file) was generated using GenePixPro 7 (Molecular Devices)
Description cRNA mCh-04
Data processing background correction and normalization using limma package in R
 
Submission date Jan 05, 2015
Last update date Mar 02, 2023
Contact name Xin Lu
E-mail(s) [email protected]
Organization name University of Regensburg
Street address Universitätsstraße 31
City Regensburg
ZIP/Postal code 93053
Country Germany
 
Platform ID GPL7202
Series (2)
GSE64648 Genome activity during the emergence of mouse embryonic totipotency (morpholino)
GSE64650 Genome activity during the emergence of mouse embryonic totipotency

Data table header descriptions
ID_REF
VALUE normalized signal intensities

Data table
ID_REF VALUE
A_51_P143341 0.921574408
A_52_P674309 1.780743724
A_52_P24896 1.746962824
A_51_P414948 3.332891445
A_52_P510647 2.505657486
A_51_P165408 3.029177558
A_52_P598468 1.624426056
A_51_P262325 0.76903308
A_52_P264525 1.123602159
A_51_P114616 1.285950781
A_52_P239381 1.647538821
A_51_P437289 3.574926254
A_52_P675171 3.785028139
A_52_P264918 1.995153512
A_51_P309056 0.776130288
A_51_P444502 1.115007889
A_51_P416695 0.969469311
A_52_P420715 0.935764079
A_51_P415126 1.033515043
A_52_P243658 0.782635725

Total number of rows: 41174

Table truncated, full table size 998 Kbytes.




Supplementary file Size Download File type/resource
GSM1576198_251486824598_A3.gpr.gz 4.6 Mb (ftp)(http) GPR
Processed data included within Sample table

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