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Sample GSM4114013 Query DataSets for GSM4114013
Status Public on May 14, 2020
Title mLN_exp2
Sample type RNA
 
Source name mLN_CD45-
Organism Mus musculus
Characteristics strain: C57BL/6NCrl
Treatment protocol For isolation of CD45- SCs, the mesenteric lymph node (mLN) or the peripheral lymph node (pLN) of wildtyp mice were removed, and LNs were digested at 37° for 30 min with 1 mg/ml Collagenase 8 in RPMI 1640/10% FCS. CD45- cells were isolated using the MACS technique following the instructions provided by Miltenyi. The mean purity of CD45- cells was 97.4% ± 2.0 for mLN cells and 97.5% ± 2.2 for pLN cells.
Extracted molecule total RNA
Extraction protocol Sorted cells from pLN and mLN were isolated and total RNA was isolated according to the manufacturer´s protocol (RNeasy Micro Kit, Qiagen, Hilden, Germany).
Label Alexa555
Label protocol 80ng of total RNA were used to prepare aminoallyl-UTP-modified (aaUTP) cRNA (Amino Allyl MessageAmp™ II Kit; #AM1753; Thermo Fisher Scientific) applying one-round of amplification as directed by the company, except for a twofold downscaling of all reaction volumes. The labeling of aaUTP-cRNA was performed by use of Alexa Fluor 555 Reactive Dye (#A32756; Thermo Fisher Scientific) as recommended in the manual of the Amino Allyl MessageAmp™ II Kit (twofold downscaled reaction volumes).
 
Hybridization protocol cRNA fragmentation, hybridisation and washing steps were carried-out as recommended in the ‘One-Color Microarray-Based Gene Expression Analysis Protocol V5.7’, except that 400ng of each fluorescently labelled cRNA population was used for hybridization.
Scan protocol Slides were scanned on the Agilent Micro Array Scanner G2505 B at two different PMT settings (100 % and 5 %) to increase the dynamic range of the measurements (extended dynamic range mode).
Data processing Data extraction and normalization were performed with the “Feature Extraction Software V9.5.3.1” by using the recommended default extraction protocol file: GE1-v5_95_Feb07.xml. Measurements of on-chip replicates were averaged using the geometric mean of processed intensity values of the green channel, ‘gProcessedSignal’ (gPS) to retrieve one resulting value per unique non-control probe. Single Features were excluded from averaging, if they i) were manually flagged, ii) were identified as Outliers by the Feature Extraction Software, iii) lay outside the interval of ‘1.42 x interquartile range‘ regarding the normalized gPS distribution of the respective on-chip replicate population, or, iv) showed a coefficient of variation of pixel intensities per Feature that exceeded 0.5. Averaged gPS values were normalized by global linear scaling: All gPS values of one sample were multiplied by an array-specific scaling factor. This factor was calculated by dividing a ‘reference 75th Percentile value’ (set as 1500 for the whole series) by the 75th Percentile value of the particular Microarray to be normalized (‘Array I’ in the formula shown below). Accordingly, normalized gPS values for all samples (microarray data sets) were calculated by the following formula: normalized gPSArray i = gPSArray i x (1500 / 75th PercentileArray i) Finally, a lower intensity threshold (surrogate value) was defined based on intensity distribution of negative control features. This value was fixed at 15 normalized gPS units. All of those measurements that fell below this intensity cutoff were substituted by the respective surrogate value of 15.
 
Submission date Oct 08, 2019
Last update date May 14, 2020
Contact name Oliver Dittrich-Breiholz
E-mail(s) dittrich.oliver@mh-hannover.de
Organization name Medical School Hannover
Department Research Core Unit Genomics
Street address Carl-Neuberg-Str. 1
City Hannover
ZIP/Postal code 30625
Country Germany
 
Platform ID GPL7202
Series (2)
GSE138593 Dietary lipids accumulate in macrophages and stromal cells and change the microarchitecture of the mesenteric lymph node I
GSE138595 Dietary lipids accumulate in macrophages and stromal cells and change the microarchitecture of the mesenteric lymph node

Data table header descriptions
ID_REF
VALUE Normalized processed signal intensity values (non logarithmic), averaged across on-chip replicate probes. Measurements of control features were removed.

Data table
ID_REF VALUE
A_51_P100021 15
A_51_P100034 6073.057398
A_51_P100052 18.25847279
A_51_P100063 209.0108284
A_51_P100084 186.3955213
A_51_P100099 5400.442741
A_51_P100155 10596.07029
A_51_P100174 245.7070718
A_51_P100181 1053.447838
A_51_P100218 15
A_51_P100227 2905.704402
A_51_P100238 15
A_51_P100246 3779.612611
A_51_P100289 3953.761865
A_51_P100298 389.2338109
A_51_P100309 15
A_51_P100327 3039.797248
A_51_P100347 15
A_51_P100379 525.6383898
A_51_P100428 15

Total number of rows: 41174

Table truncated, full table size 915 Kbytes.




Supplementary file Size Download File type/resource
GSM4114013_M2886.txt.gz 9.1 Mb (ftp)(http) TXT
Processed data included within Sample table

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