NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM730581 Query DataSets for GSM730581
Status Public on Jan 18, 2012
Title 96 hours after irradiation
Sample type RNA
 
Channel 1
Source name T. cruzi epimastigote cells - irradiated (RNA extract 96 hours after irradiation)
Organism Trypanosoma cruzi
Characteristics strain: CL Brener
Treatment protocol Cultures with 5×108 parasites in 20 mL of LIT medium (2x107 cells/mL) were exposed to a dose of 500 Gy (1578 Gy/h per 20 minutes) in a cobalt (60Co) irradiator located at Centro de Desenvolvimento da Tecnologia Nuclear (CDTN), Belo Horizonte, Brazil
Growth protocol Epimastigote cells were cultivated at 28 ◦C in LIT medium (Liver Infusion Tryptone - liver digest neutralized) supplemented with complement-inactivated 10% fetal bovine serum, streptomycin sulfate (0.2 g/L), and penicillin (200,000 units/L).
Extracted molecule total RNA
Extraction protocol Epimastigote cells were subjected to RNA extraction using Trizol reagent (Invitrogen Life Technologies, USA) and RNA samples were purified using RNeasy® MiniEluteTM Cleanup Kit (Qiagen, German) according to the manufacturers’ instructions. Total RNA was quantified using a Nanodrop ND-100 UV/Vis spectrophotometer (NanoDrop Technologies, USA) and the overall RNA quality was assessed by denaturing gel electrophoresis [14]. Total RNA (2 μg) was amplified using the Amino Allyl MessageAmp II kit (Ambion, USA), according to the manufacturer’s specifications.
Label Cy3,Cy5
Label protocol Aminoallyl amplified RNA was labeled with Cy3 and Cy5 according to a modified version of the AminoAllyl MessageAmp II Kit (Ambion, USA) and TIGR's standard operational procedure – SOP #M008 (ftp://ftp.jcvi.org/pub/data/PFGRC/MAIN/pdf_files/protocols/M008.pdf). Briefly, we followed the manufacturer’s instructions for the labeling step, but the initial amount of amplified RNA was changed to 8 μg. The Cy3 and Cy5 labeled samples were then combined. Labeled RNA was purified away from unincorporated dyes using YM-30 Microcon columns following manufacturer's specifications (Millipore®, USA). The final sample was dried again and resuspended in 30 µL of hybridization buffer (50% formamide, 5× SSC, 0.1% SDS, 0.1M DDT, and 6% salmon sperm as blocking agent) according to TIGR's SOP #M008. The solution was heated to 95 oC during 3 minutes and placed in ice for 30 seconds. After a brief centrifugation, the solution was dispensed onto the slide surface and covered with a coverslip.
 
Channel 2
Source name T. cruzi epimastigote cells - control (Non-irradiated - Biological replicate I)
Organism Trypanosoma cruzi
Characteristics strain: CL Brener
Treatment protocol Cultures with 5×108 parasites in 20 mL of LIT medium (2x107 cells/mL) were exposed to a dose of 500 Gy (1578 Gy/h per 20 minutes) in a cobalt (60Co) irradiator located at Centro de Desenvolvimento da Tecnologia Nuclear (CDTN), Belo Horizonte, Brazil
Growth protocol Epimastigote cells were cultivated at 28 ◦C in LIT medium (Liver Infusion Tryptone - liver digest neutralized) supplemented with complement-inactivated 10% fetal bovine serum, streptomycin sulfate (0.2 g/L), and penicillin (200,000 units/L).
Extracted molecule total RNA
Extraction protocol Epimastigote cells were subjected to RNA extraction using Trizol reagent (Invitrogen Life Technologies, USA) and RNA samples were purified using RNeasy® MiniEluteTM Cleanup Kit (Qiagen, German) according to the manufacturers’ instructions. Total RNA was quantified using a Nanodrop ND-100 UV/Vis spectrophotometer (NanoDrop Technologies, USA) and the overall RNA quality was assessed by denaturing gel electrophoresis [14]. Total RNA (2 μg) was amplified using the Amino Allyl MessageAmp II kit (Ambion, USA), according to the manufacturer’s specifications.
Label Cy5,Cy3
Label protocol Aminoallyl amplified RNA was labeled with Cy3 and Cy5 according to a modified version of the AminoAllyl MessageAmp II Kit (Ambion, USA) and TIGR's standard operational procedure – SOP #M008 (ftp://ftp.jcvi.org/pub/data/PFGRC/MAIN/pdf_files/protocols/M008.pdf). Briefly, we followed the manufacturer’s instructions for the labeling step, but the initial amount of amplified RNA was changed to 8 μg. The Cy3 and Cy5 labeled samples were then combined. Labeled RNA was purified away from unincorporated dyes using YM-30 Microcon columns following manufacturer's specifications (Millipore®, USA). The final sample was dried again and resuspended in 30 µL of hybridization buffer (50% formamide, 5× SSC, 0.1% SDS, 0.1M DDT, and 6% salmon sperm as blocking agent) according to TIGR's SOP #M008. The solution was heated to 95 oC during 3 minutes and placed in ice for 30 seconds. After a brief centrifugation, the solution was dispensed onto the slide surface and covered with a coverslip.
 
 
Hybridization protocol Slides were pre-hybridized by placing them in coupling jars containing pre-hybridization solution (5× SSC, 0.1% SDS, 1%BSA) at 42 °C for one hour. Slides were washed twice by immersing 10 times in a beaker containing MilliQ water followed by dipping three times in isoamyl alcohol, and were subsequently spun dry. The slides containing 30 µL of samples in hybridization buffer were hybridized for 14 hours in a water bath at 42° C in the dark under cover slips inside Corning® hybridization chambers (Corning, USA). Slides were then washed two times for five minutes each in a low stringency wash solution (2× SSC, 0.1% N-lauroysarcosine) at 42 °C (first wash) and RT (second wash), followed by two washes of five min in medium stringency wash (0.1× SSC, 0.1% N-lauroysarcosine) at RT and two washes for five minutes each in high stringency wash solution (0.1× SSC) at RT.
Scan protocol Slides were spun dry and scanned using a microarray dual channel laser scanner (ScanExpress Lite da PerkinElmer®, USA) at 10 μm resolution, 100% laser power and PMT levels which were adjusted in order to obtain similar distributions of red and green signal intensities.
Description Analysis used non-irradiated T. cruzi epimastigote cells as control samples for comparison to irradiated epimastigote cells with RNA extracted 96 hours after irradiation. Two biological replicates (RI and RII).
Data processing For each time point, gene expression analysis was done based on information obtained from four slides, one dye-swap pair for each biological replicate. ScanArray Express (PerkinElmer®) software was used to generate the slide images and raw intensity data which were then analyzed using specific packages from the R statistical language. Spots of good quality (positive flag value) were considered to be analyzed. Data were inspected for spatial biases on both red and green channels (background and signal), for print-tip bias, dye bias, and bias dependent of intensity using the LIMMA and marray packages. Background correction was done with normexp method. Robust spline and aquantile methods were used for normalization within and between arrays, respectively. A linear model that incorporates biological and technical replication was used for statistical analysis. A list of differentially expressed genes was generated by applying adjusted p-values for multiple tests using ‘BH’ method, which works with the expected proportion of false-positives (FDR- False Discovery Rate) among the rejected hypothesis. Graphics were drawn using GraphPad version 5.03. Heatmap and cluster graphics were created using gplots package and personal scripts (R statistical language).
 
Submission date May 24, 2011
Last update date Jan 18, 2012
Contact name Priscila Grynberg
E-mail(s) priscilag@gmail.com
Phone 553134092628
Organization name Universidade Federal de Minas Gerais
Department Departamento de Bioquímica e Imunologia
Lab Laboratório de Genética Bioquímica
Street address Avenida Antonio Carlos, 6627
City Belo Horizonte
State/province Minas Gerais
ZIP/Postal code 31270-901
Country Brazil
 
Platform ID GPL5906
Series (1)
GSE29510 Trypanosoma cruzi gene expression study in response to gamma-radiation

Data table header descriptions
ID_REF
VALUE normalized log2 Fold-change (irradiated samples/control)

Data table
ID_REF VALUE
T3AQTC00001_D_1 0.015314449
T3AQTC00003_P_13
T3AQTC00006_L_13
T3AQTC00009_H_13
T3AQTC00033_D_13
T3AQTC00014_P_1
T3AQTC00017_L_1
T3AQTC00020_H_1 -0.169334052
T3AQTC00034_D_1
T3AQTC00024_P_13
T3AQTC00027_L_13
T3AQTC00030_H_13 0.068744648
T3AQTC00001_H_1
T3AQTC00004_D_1 0.023264608
T3AQTC00006_P_13 0.246324318
T3AQTC00009_L_13
T3AQTC00033_H_13
T3AQTC00014_D_13 -0.058784587
T3AQTC00017_P_1
T3AQTC00020_L_1

Total number of rows: 12788

Table truncated, full table size 263 Kbytes.




Supplementary file Size Download File type/resource
GSM730581_96hours_Cy3XControl_Cy5_RepII.gpr.gz 1.9 Mb (ftp)(http) GPR
GSM730581_96hours_Cy3xControl_Cy5_RepI.gpr.gz 2.0 Mb (ftp)(http) GPR
GSM730581_Control_Cy3X96hours_Cy5_RepI.gpr.gz 2.0 Mb (ftp)(http) GPR
GSM730581_Control_Cy3X96hours_Cy5_RepII.gpr.gz 1.9 Mb (ftp)(http) GPR
Processed data included within Sample table

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