Title: at Cambridge University
1at Cambridge University
Analysis of gene expression in the NOD mouse
2Hi!
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6Control
Chr18.A
x 3
Chr18.B
NOD
NOD.ABH(18)
Splenocyte RNA
NOD.ABH(sub18)
Sent to UK In 3 volumes ethanol _at_ 20ºC
28S
18S
7_at_Wellcome Trust, Cambridge UK
Dr Paul Lyons Laboratory
Agilent Bioanalyzer
28S
18S
Marker
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9Microarray Protocol
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1st Strand cDNA synthesis
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cDNA amplification (Clontech SMART system)
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Cy3/Cy5 Incorporation - Klenow polymerase
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G-50 Sepharose column purification
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Hybridisation at 50ºC for 18 hours
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Post-hybridisation washes (SSC/SDS)
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Dry arrays, then scanned within 24 hours
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11Experimental Design
- 4 experiments on Splenocyte RNA
- 2 dye reversal experiments
- 3 Pairwise comparisons within each Experiment
- Control vs C18A
- Control vs C18B
- C18A vs C18B
- Duplicated genes on each array
12The Sanger Centre
13Agilent TechnologiesG2505A Scanner
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16IMAGENE 4.2
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18Calculating Gene Ratios (Log2)
A
C
A
-
B
B
C
Where A is NOD B is NOD.ABH(18) C is
NOD.ABH(sub18)
19Gene Ratio Agreement
Percent of Genes
Agreement between calculated and empirical gene
ratios within each experiment Where calculated
and empirical were within 25 of each other
20Identifying Candidate Genes
- Spot present in all experiments
- Greater than 2-fold change (Log21)
- Coefficient of Variation lt 20
Absolute Mean
CoeffVar
Standard Deviation
21Differentially Expressed Genes
Control vs C18A 16 genes Control vs C18B 146
genes C18A vs C18B 191 genes
From 7500 genes
22Further Investigation
- Slides from Paul Lyons, UK
- Otago Microarray Facility
- Isolation of pancreatic lymph node RNA of high
quality
23Acknowledgements
- Paul Lyons and his research group at the MRC,
Cambridge University, UK - Gerry Morris and Sian Piper
- Tony Merriman, Marilyn Merriman, Peter Stockwell
and Jade Hollis-Moffatt - Biochemistry Department, University of Otago
- Functional Genomics, gene expression and
proteomics Research Theme - Marjorie MaCallum Travel Award in Biochemistry