NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM1493601 Query DataSets for GSM1493601
Status Public on May 15, 2015
Title S1_ebv03_mda
Sample type genomic
 
Source name EBV-transformed lymphoblast
Organism Homo sapiens
Characteristics cell type: EBV-transformed lymphoblast
dna sample: Single cell
wga: MDA
hybridization protocol: Conventional
Treatment protocol The embryos that were not suitable for transfer on day 4 were dissociated and single blastomeres were collected for further analysis. The zona pellucida was removed by incubation in a droplet of Tyrode's solution (Sigma-Aldrich, USA). The acid was and consequently washed away and the embryos were dissociated in a droplet of Ca2+/Mg2+ free medium (Life Global, Canada).
Growth protocol The embryos were in vitro cultured in Life Global medium (Life Global, Canada) or Quinns Advantage Protein Plus Medium (Cooper Surgical, USA). On day 2 and 3 after fertilization, embryo development was evaluated for the number of blastomeres, the percentage of fragmentation and the symmetry of the blastomeres. All ≥ 6 cell stage embryos that had less than 25% fragmentation on day 3 after fertilization were biopsied using a non-contact, 1.48 µm diode laser system (Fertilase®; MTG, Germany) coupled to an inverted microscope, after first being incubated in Ca2+/Mg2+ free medium. One or two blastomeres were gently aspirated from each embryo for the conventional FISH- or PCR-based PGD. The embryos were immediately transferred to fresh medium; while the aspirated blastomeres were separately washed twice with Ca2+/Mg2+ free medium to remove possible oil remnants.
Extracted molecule genomic DNA
Extraction protocol Single cells were washed in 1xPBS and transferred into a 200 µl PCR tube containing 1.5 µl alkaline lysis buffer (ALB; 200 mM KOH and 50 mM DTT) by mouth controlled pipetting using 75 µm stripper tips (Origio, Denmark). The samples were stored at -20°C for at least 30 min and were further incubated for 10 min at 65°C prior to the multiple displacement amplification (MDA) reaction. Single cell DNA was amplified following an MDA-approach with GenomiPhiV2 (GE Healthcare, USA). The MDA products were purified using the High Pure PCR Product Purification Kit (Roche, Switzerland) and resuspended in 70 µl of elution buffer. All amplification products were quantified with a spectrophotometer (Nanodrop ND-1000 spectrophotometer). Single-cell amplifications yielding less than 2 µg DNA were not further used.
Label Cy5/Cy3
Label protocol The samples were not labelled before the hybridization. The staining is based on post-hybridization Cy5/Cy3 labelling by extension, according to the manual of Infinium II Assay (Illumina, USA).
 
Hybridization protocol According to the manual of Infinium II Assay (Illumina, USA), with the exception that the fragmentation step was shortened from 20-24h to 7h and the hybridization step was shortened from 16-20h to 6h for the rapid protocol.
Scan protocol The scanning of the bead-chips was performed on an iScan, using the iScan Control software (Illumina, USA)
Description Single cell from an Epstein-Barr virus transformed lymphoblastoid cell line derived from sibling S1. EBV-transformed lymphoblastoid cells were cultured in 75-cm2 plastic flasks (BD Falcon, USA) in Dulbecco's Modified Eagle Medium/Nutrient Mixture F-12 (DMEM/F12) (Gibco, USA) medium supplemented with 10% Fetal Bovine Serum (FBS) (Thermo Scientific, USA) at 37oC, 5% CO2. The sample was processed according to the manual of Infinium II assay (Illumina, USA).
Data processing The genotypes, B allele frequencies and LogR values were extracted by the Genotyping module of GenomeStudio software. The discrete genotypes were determined using a threshold of 0,75 in GenCall.
 
Submission date Aug 28, 2014
Last update date May 15, 2015
Contact name Masoud Zamani Esteki
E-mail(s) [email protected]
Phone +31 43 38 75306
Organization name Maastricht University Medical Center
Department Clinical Genetics
Lab Cellular Genomic Medicine
Street address P. Debyelaan 25
City Maastricht
State/province Limburg
ZIP/Postal code 6229 HX
Country Netherlands
 
Platform ID GPL13829
Series (2)
GSE60909 Concurrent whole-genome haplotyping and copy number profiling of single cells (Illumina)
GSE60910 Concurrent whole-genome haplotyping and copy number profiling of single cells

Data table header descriptions
ID_REF
VALUE genotype call
GC_SCORE
Theta
R
B_Allele_Freq
Log_R_Ratio

Data table
ID_REF VALUE GC_SCORE Theta R B_Allele_Freq Log_R_Ratio
cnvi0111185 NC 0.00 0.973978 1.364939 0.9970433 0.09201703
cnvi0111186 NC 0.00 0.5813564 0.06072427 0.5842035 -3.088691
cnvi0111187 NC 0.00 0.9631019 0.9871892 0.977654 -0.6024423
cnvi0111188 NC 0.00 0.1403396 0.06725644 0.1329738 -4.296443
cnvi0111189 NC 0.00 0.5613407 0.06778111 0.5653059 -4.443614
cnvi0111190 NC 0.00 0.01559093 0.5439705 0.00 0.3064459
cnvi0111191 NC 0.00 0.7170346 0.08199155 0.7244472 -3.473142
cnvi0111192 NC 0.00 0.4597906 0.05842134 0.4594623 -4.293331
cnvi0111193 NC 0.00 0.04548478 0.5427896 0.03569242 -1.090652
cnvi0111194 NC 0.00 0.5929474 0.03665001 0.5905815 -5.098046
cnvi0111195 NC 0.00 0.04859821 1.808979 0.02003851 -0.2439781
cnvi0111196 NC 0.00 0.991096 1.318949 1 0.09359213
cnvi0111197 NC 0.00 0.04724853 0.5783825 0.03039575 -0.5618532
cnvi0111198 NC 0.00 0.9728547 0.8253373 1 -0.7040436
cnvi0111199 NC 0.00 0.0341562 0.9635684 0.02370668 -0.5155604
cnvi0111200 NC 0.00 0.5219184 0.06129529 0.5167446 -3.771616
cnvi0111201 NC 0.00 0.1117456 0.5129281 0.08747991 -0.7714785
cnvi0111202 NC 0.00 0.4984905 0.05992621 0.5157499 -4.485473
cnvi0111203 NC 0.00 0.05231706 0.316678 0.01131924 -2.544647
cnvi0111204 NC 0.00 0.7157981 0.03725861 0.7169617 -4.946731

Total number of rows: 298563

Table truncated, full table size 17837 Kbytes.




Supplementary data files not provided
Processed data included within Sample table
Processed data are available on Series record

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap