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Sample GSM477256 Query DataSets for GSM477256
Status Public on Dec 04, 2009
Title 184
Sample type genomic
 
Source name lymphoblast from Coriell family 1990
Organism Homo sapiens
Characteristics cell type: lymphoblast from Coriell family 1990
cell amplication: single cell amplified by MDA
Extracted molecule genomic DNA
Extraction protocol Single cells were isolated from buccal swabs, semen samples, adult blood, immortalized cell lines, and Day 3 cryopreserved embryos. Single tissue culture (lymphocytes) and buccal cells were isolated using a sterile stripper tip (Midatlantic Diagnostic, Mt. Laurel, NJ, USA) affixed to a pipette (Drummond Scientific, Broomall, PA, USA) and a stereoscope (Leica, Wetzlar, Germany). Embryos were thawed, and then individual blastomeres were separated using a micromanipulator (Transferman NK2-Eppendorf, Westbury, NY, USA) after zona pellucida drilling using acidified Tyrode’s solution. Sperm cells were manually isolated using a micromanipulator (Transferman NK2-Eppendorf). Aside from sperm, single cells were washed sequentially four times with wash buffer (5.6mg/ml KCl, 6mg/ml bovine serum albumin). Two different lysis/amplification protocols were used in the analysis: (i) Rubicon Whole Genome Amplification (Ann Arbor, MI, USA), and (ii) multiple displacement amplification (MDA) with Proteinase K Buffer (PKB). Protocol (i) was performed according to the manufacturer’s instructions. For protocol (ii), cells were placed in 5µl PKB (Arcturus PicoPure Lysis Buffer, 50mM DTT), incubated at 56°C for one hour, and then heat inactivated at 95°C for ten minutes. MDA reactions were incubated at 30°C for 2.5 hours and then 65°C for five minutes. Genomic DNA from bulk tissue (Epicentre MasterAmp Buccal Swabs, Madison, WI, USA) was isolated using the DNeasy Blood and Tissue Kit (Qiagen, Hilden, Germany). No template controls (buffer blanks) were performed for each amplification method. All buffer blanks produced intensities equivalent to the noise floor (an intensity of 1000 in the 95th percentile on the green detection channel).
Label C-Bio and A-DNP
Label protocol as per Illumina's instructions except reduced amplification time to 6 hours
 
Hybridization protocol as per Illumina's instructions except reduced time to 6 hours
Scan protocol as per Illumina's instructions
Description 4726917081_R04C01
Data processing Genotypes are inherently inaccurate in single cell microarray data due to biases introduced during multiple displacement amplification. Therefore genotypes were not produced, and instead raw intensity data was used to build probabilistic models under the framework of the Parental Support algorithm.
 
Submission date Dec 01, 2009
Last update date Dec 03, 2009
Contact name David Scott Johnson
E-mail(s) djohnson@genesecurity.net
Phone 415-978-2101
Organization name Gene Security Network
Street address 2686 Middlefield Road, Suite C
City Redwood City
State/province CA
ZIP/Postal code 94063
Country USA
 
Platform ID GPL8855
Series (1)
GSE19247 Preclinical Validation of a Microarray Method for Full Molecular Karyotyping of Blastomeres in a 24-hour Protocol

Supplementary file Size Download File type/resource
GSM477256_4726917081_R04C01_1.xml.gz 618 b (ftp)(http) XML
GSM477256_4726917081_R04C01_2.xml.gz 620 b (ftp)(http) XML
GSM477256_4726917081_R04C01_3.xml.gz 619 b (ftp)(http) XML
GSM477256_4726917081_R04C01_4.xml.gz 619 b (ftp)(http) XML
GSM477256_4726917081_R04C01_Grn.idat.gz 1.9 Mb (ftp)(http) IDAT
GSM477256_4726917081_R04C01_Red.idat.gz 1.8 Mb (ftp)(http) IDAT
Processed data not applicable for this record

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