NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM2442435 Query DataSets for GSM2442435
Status Public on Nov 30, 2017
Title WT25 DMM 6 WK
Sample type RNA
 
Source name subchondral bone
Organism Mus musculus
Characteristics strain: C57BL6
gender: Male
tissue: subchondral bone
time post-surgery (weeks): 6
Treatment protocol Post-traumatic OA was surgically induced in 10-12 week old male wild type C57BL6 and Jaffa mice by bilateral destabilization of the medial meniscus (DMM), as described previously. Briefly, the medial menisco-tibial ligament was exposed (by medial parapatellar arthrotomy and intrapatellar fat pad elevation, without tissue resection) and transected with curved dissecting forceps by one surgeon (CBL). Bilateral sham-operations were also performed, where the medial menisco-tibial ligament was visualised but not transected. All joints were flushed with sterile saline to remove any blood prior to separate closure of the joint capsule (simple continuous 8/0 polyglactin 910), subcutaneous tissue (mattress suture 8/0 polyglactin 910) and skin (cyanoacrylate).
Growth protocol DMM and sham were co-housed with 2-5 animals/30×20×18cm individually-ventilated-cage with filter lids, provided with sterilised bedding and environmental enrichment, maintained at 21-22°C with a 12-hour light/dark cycle, and received water and complete pelleted food ad libitum. Mice received no post-operative medication, were maintained in their pre-operative groups and were allowed unrestricted cage exercise.
Extracted molecule total RNA
Extraction protocol Mice were randomly allocated to groups/harvest time point prior to study commencement using their individual ID numbers. Animals were sacrificed at 1 and 6 weeks after surgery. For each animal, one joint was processed for histology whilst the other was used for microarray expression profiling/qPCR. Microarray experiments on cartilage samples were performed on n = 3/group/time point, each consisting of RNA pooled from 3 individual mice. qPCR validation was performed on the same 3 pooled RNA samples and 4 additional biological replicates per time point per group. Microarray experiments on SCB samples were performed on n = 4/group/time point with qPCR validation performed on a different cohort of 4 mice/group/time point. Joint dissection, laser micro-dissection and RNA extraction from mouse cartilage and SCB was performed in a similar fashion to previously described. Briefly, mice were sacrificed 1 and 6 weeks after surgery and the tibial epiphyses were isolated and placed in RNA Later (Life Technologies) containing 10% EDTA for at least 72 hrs at 4°C. After decalcification the samples were washed in DEPC-treated PBS, embedded in OCT and stored at -80°C. Serial 10 µm sagittal cryo-sections were fixed in ethanol and air-dried. Sections of the cartilage and underlying SCB of the medial tibial plateau were laser micro-dissected (Arcturus Bioscience) and collected. Total RNA was extracted from pooled laser micro-dissected sections from each individual mouse joint using TRIzol according to the manufacturer’s instructions
Label Cyanine 3-pCp
Label protocol miRNA expression profiling was performed using SurePrint mouse miRNA microarray technology, release 21 (G4859C, Agilent Technologies) at the Ramaciotti Centre for Genomics (UNSW, Sydney, Australia). Briefly, 70 ng of total RNA was labelled and hybridized using the miRNA microarray System with miRNA complete labelling and Hyb kit version 3.0 (Agilent Technologies) by following manufacturer’s instructions.
 
Hybridization protocol miRNA expression profiling was performed using SurePrint mouse miRNA microarray technology, release 21 (G4859C, Agilent Technologies) at the Ramaciotti Centre for Genomics (UNSW, Sydney, Australia). Briefly, 70 ng of total RNA was labelled and hybridized using the miRNA microarray System with miRNA complete labelling and Hyb kit version 3.0 (Agilent Technologies) by following manufacturer’s instructions.
Scan protocol The arrays were scanned on a G2565CA microarray scanner and the features were extracted using Agilent Feature Extraction 12.0.07 software.
Description microRNA
Bilateral surgeries performed. Limbs randomly allocated to either microarray or histological analysis. Knees taken from the same mouse for both histology and expression profiling. Cartilage and bones samples isolated from the same mouse for parallel expression analyses.
Data processing The raw microarray data was processed in statistical language R, using the limma package (limma_3.20.9) and background corrected with Normexp, normalized within arrays with cyclic loess. Only probes with 10% greater signal than the negative controls in at least 4 samples were maintained for differential expression analysis. Probes were summarised at the gene level and the data was adjusted for multiple testing using Benjamini-Hochberg method to control for false discovery rate.
 
Submission date Dec 29, 2016
Last update date Nov 30, 2017
Contact name John Bateman
Organization name Murdoch Childrens Research Institute
Department Skeletal Biology
Lab John Bateman
Street address Flemington Road
City Melbourne
ZIP/Postal code 3052
Country Australia
 
Platform ID GPL21265
Series (2)
GSE93008 Cartilage microRNA dysregulation during the onset and progression of mouse osteoarthritis is independent of aggrecanolysis and overlaps with candidates from end-stage human disease [miRNA]
GSE101574 Cartilage microRNA dysregulation during the onset and progression of mouse osteoarthritis is independent of aggrecanolysis and overlaps with candidates from end-stage human disease

Data table header descriptions
ID_REF
VALUE Norm Exp and Cyclic lowess normalized signal intensity

Data table
ID_REF VALUE
mmu-let-7a-5p 11.64740125
mmu-let-7b-5p 11.61546379
mmu-let-7c-5p 11.75741788
mmu-let-7d-5p 10.12171158
mmu-let-7e-5p 7.98176955
mmu-let-7f-1-3p 4.980884671
mmu-let-7f-5p 10.88177964
mmu-let-7g-5p 9.940814418
mmu-let-7i-5p 10.22584238
mmu-let-7j 6.352739066
mmu-let-7k 7.046628392
mmu-miR-100-5p 6.744679865
mmu-miR-101a-3p 5.382932663
mmu-miR-101c 5.184257705
mmu-miR-103-1-5p 5.64827529
mmu-miR-103-3p 9.136956536
mmu-miR-106a-3p 4.500978072
mmu-miR-106b-3p 5.411215997
mmu-miR-106b-5p 8.548520195
mmu-miR-107-3p 8.126725982

Total number of rows: 490

Table truncated, full table size 12 Kbytes.




Supplementary file Size Download File type/resource
GSM2442435_Ramaciotti_257015510243_S01_miRNA_1200_Jun14_2_1.txt.gz 7.9 Mb (ftp)(http) TXT
Processed data included within Sample table

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