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Sample GSM604563 Query DataSets for GSM604563
Status Public on Dec 31, 2017
Title FAMI patient N. 19 (A)
Sample type RNA
 
Source name Platelets from patient with acute MI within 6 hours of the onset of symptoms
Organism Homo sapiens
Characteristics age (years): 55
gender: female
bmi: 22.99
n. diseased vessels: 1
ck peak: 1089.00
tnl on admission (pg/ml): <0.2
crp on admission (mg/dl): 0.89
il-6 on admission (ng/dl): 1.58.
Biomaterial provider Cardio-Thoracic Unit of San Raffaele Hospital (Milan, Italy).
Treatment protocol Patients were all with the same clinical presentation: acute MI within 6 hours of the onset of symptoms, without any previous evidence of coronary disease, except for the retrospective report of possible episodes of angina in the previous week and potentially eligible for thrombolysis or other coronary reperfusion strategie.
Extracted molecule total RNA
Extraction protocol Peripheral blood (40 ml) from patients was collected in EDTA, and platelets were isolated within 1 hour by differential centrifugation. Purity of platelet preparations was checked with a Cell-Dyn Coulter counter (Abbot Diagnostics, Abbott Park). A fraction of platelets was resuspended in TRIzol reagent (Invitrogen) for total RNA isolation according to the manufacturer's guidelines. Total RNA was quantified using the ND-1000 spectrophotometer (Nanodrop, Wilmington, DE), while RNA integrity was assessed by capillary electrophoresis using the RNA 6000 Nano LabChip (Agilent Technologies, Palo Alto, CA). Platelet purification was also checked after total RNA extraction by quantitative RT-PCR on the platelet specific marker, integrin alpha 2b, and the leukocyte specific marker T cell receptor (TCR). Good samples, used for further analysis and experiments, showed < 1% TCR purity level.
Label Cy5
Label protocol We performed microarray experiments using the CodeLink Expression Bioarray System (GE Healthcare). Total RNA (1.5 µg) was amplified and biotin-labeled using the CodeLink Expression Assay Reagent Kit following the manufacturer’s protocol. Before amplification, mRNA control spikes were added to all tubes. These controls were used to verify the quality of the process. Biotin-labeled aRNA (10 µg) was fragmented and loaded into a CodeLink Human Whole Genome Bioarray, containing about 55,000 human oligonucleotide gene probes, matching more than 45,000 human genes and transcript targets
 
Hybridization protocol Arrays were hybridized for 21 hours at 37°C at 300 rpm on a Thermomixer comfort (Eppendorf) and washed according to manufacturer’s protocol. The bioarrays were stained with incubation in 3.4 mL of streptavidin-Cy5 solution for 30 minutes, washed, and dried by centrifugation at 640 rpm.
Scan protocol Images were obtained with ScanArray Lite (PerkinElmer) scanner, using the ScanArray Express software (PerkinElmer), with a 635 nm laser, maintaining constant laser power (85%) and constant photomultiplier gain (55%).
Description Images were analyzed using CodeLink expression software version 4.2, and raw data analysis was exported to GeneSpring format (tab-delimied text format).
Data processing Raw intensity signals were analyzed with the GeneSpring GX 7.3.1 software (Agilent Technologies). Normalization steps included: data transformation, setting measurements less than 0.01 to 0.01; per chip and per gene median polishing; per gene normalization to specific samples (i.e. normal controls). Before performing the statistical analysis we filtered genes with the “present” or “marginal” quality flag values (automatically assigned to each spot by the CodeLink software, according to a signal to noise computation) in 28 out of 38 conditions for platelet data.
 
Submission date Oct 05, 2010
Last update date Dec 31, 2017
Contact name Gerolamo Lanfranchi
E-mail(s) stefano.cagnin@unipd.it
Phone +39-0498276219
Organization name University of Padova
Department CRIBI - Biotechnology Center and Biology Department
Lab Functional Genomics Lab
Street address Via U. Bassi, 58/B
City Padova
ZIP/Postal code 35131
Country Italy
 
Platform ID GPL2895
Series (2)
GSE24519 Gene expression profiling of patients affected by first acute myocardial infarction (FAMI)
GSE24591 Gene and microRNA expression profiling of patients affected by first acute myocardial infarction (FAMI)

Data table header descriptions
ID_REF
VALUE Average normalized signal intensity value
Raw Raw signal intensity value

Data table
ID_REF VALUE Raw
1053 0.6442537 23.2258
1073 0.94346255 24.08197
1011 0.34058863 19.79412
1041 0.61732197 14.954544
1075 0.36418986 6.3157883
1077 0.32427356 10.678162
1013 1.309776 38.4375
1039 2.2258787 23.629631
1042 1.1058162 24
1070 0.8929381 19.419357
1086 0.24952546 3600.9167
1089 0.47594237 23.13559
1091 0.24856608 10.472221
1098 0.69344383 27.225807
1109 0.27920052 18.2967
1005 0.27282745 5.4193573
1009 0.5938411 20.73529
1010 1.1017677 948.8572
1012 0.30319494 38.837845
1040 0.8855514 886.3951

Total number of rows: 54902

Table truncated, full table size 1384 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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