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Sample GSM539948 Query DataSets for GSM539948
Status Public on May 07, 2010
Title Spermatogenesis in S. senegalensis: Mid vs. Late 3
Sample type RNA
 
Channel 1
Source name Mid spermatogenic testis
Organism Solea senegalensis
Characteristics tissue: testis pieces
developmental stage: mid spermatogenesis
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from mid spermatogenic testes using the RNeasy extraction kit (Qiagen) and treated with DNAse following the manufacturer’s instructions
Label Cy3
Label protocol Total RNA (0.5 μg) from each sample was amplified and labelled with fluorescent cyanine dyes, Cy3 or Cy5, using the Eberwein mRNA amplification procedure employing the MessageAmp™ aRNA amplification kit from Ambion (Applied Biosystems) following the manufacturer's instructions with minor modifications
 
Channel 2
Source name Late spermatogenic testis
Organism Solea senegalensis
Characteristics tissue: testis pieces
developmental stage: late spermatogenesis
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from late spermatogenic testes using the RNeasy extraction kit (Qiagen) and treated with DNAse following the manufacturer’s instructions
Label Cy5
Label protocol Total RNA (0.5 μg) from each sample was amplified and labelled with fluorescent cyanine dyes, Cy3 or Cy5, using the Eberwein mRNA amplification procedure employing the MessageAmp™ aRNA amplification kit from Ambion (Applied Biosystems) following the manufacturer's instructions with minor modifications
 
 
Hybridization protocol Hybridizations were carried out for 17 h at 60°C using Agilent's gaskets G2534-60002, G2534A hybridization chambers, and DNA Hybridization Oven G2545A, according to the manufacturer's instructions
Scan protocol Microarray raw data were obtained using Agilent's DNA Microarray Scanner G2505B and Feature Extraction software (v10.1)
Description Biological replicate 3 of 3
Data processing Raw data were obtained using Agilent's DNA Microarray Scanner G2505B and Feature Extraction software (v10.1). The raw fluorescence intensity data were processed using the Polyphemus software, developed at Oryzon Genomics, which includes spatial data compensation, non-significant expressed data filtering, and data normalization. Data normalization was carried out by an improved version of the nonlinear Q-splines normalization method, enhanced with robust regression techniques.
 
Submission date May 03, 2010
Last update date May 06, 2010
Contact name Josep V Planas
E-mail(s) jplanas@ub.edu
Phone +34-93-4039384
Organization name Universitat de Barcelona
Department Fisiologia i Immunologia (Biologia)
Lab Fisiologia Molecular de Peixos
Street address Av. Diagonal 643
City Barcelona
ZIP/Postal code 08028
Country Spain
 
Platform ID GPL8931
Series (2)
GSE21637 Transcriptional profiling of flatfish (Solea senegalensis) spermatogenesis: mid versus late spermatogenesis
GSE21694 Transcriptional profiling of flatfish (Solea senegalensis) spermatogenesis

Data table header descriptions
ID_REF
VALUE Normalized log2 ratio (Cy3/Cy5) representing Mid/Late

Data table
ID_REF VALUE
CL859CONTIG1-ENSDARG00000019940 -0.032338
CL85CONTIG1 0.028007
CL860CONTIG1 0.13503
CL861CONTIG1-ENSDARG00000028012 0.004154
CL862CONTIG1 -0.10437
CL863CONTIG1-ENSDARG00000016576 -0.055462
CL864CONTIG1-ENSDARG00000015343 -0.315343
CL865CONTIG1 -0.054355
CL866CONTIG1 -0.191087
CL867CONTIG1-ENSDARG00000040251 0.017644
CL868CONTIG1 -0.351731
CL1100CONTIG1-ENSDARG00000007219 0.369489
CL869CONTIG1 0.154555
CL86CONTIG1-ENSDARG00000029606 0.226816
CL870CONTIG1 0.178286
CL872CONTIG1 -0.367071
CL873CONTIG1 0.050476
CL874CONTIG1 -0.172123
CL876CONTIG1-ENSDARG00000015246 0.106566
CL879CONTIG1-ENSDARG00000008768 -0.038164

Total number of rows: 3824

Table truncated, full table size 126 Kbytes.




Supplementary file Size Download File type/resource
GSM539948.txt.gz 91.8 Kb (ftp)(http) TXT
Processed data included within Sample table

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