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Sample GSM146727 Query DataSets for GSM146727
Status Public on Nov 28, 2006
Title Head Short Day Cy5 Rep1
Sample type RNA
 
Channel 1
Source name Head of pea aphid reared under 16h photoperiod: reference channel
Organism Acyrthosiphon pisum
Characteristics Strain: YR2 (red holocyclic clone)
Parthenogenetic female
10 days of 16h photoperiod
Instar stage L3
Female producing parthenogenetic females
Biomaterial provider INRA Rennes, UMR 1099 BiO3P
Treatment protocol Long Day reared pea aphids
Growth protocol The clone YR2 of the pea aphid A. pisum was reared on broad bean (Vicia fabae) at 18°C. Parthenogenetic reproduction was maintained at 16 h of light and aphids were reared at low density (one to five individuals per plant) over three generations to prevent the production of winged forms. Conditions: 16 h of light (“long-day” or LD) that maintained parthenogenesis. To initiate the experiment clonal third instar larvae (L3) were placed under LD photoperiod. This corresponds to generation G0. L3-G0 aphids reached adulthood (wingless adults or WA) and produced offspring (G1) that were transferred onto new plants and kept under LD conditions. A batch of 50 L3-G1 aphids was collected in the middle of the photophase (15:00) and immediately frozen in liquid nitrogen. As a control, few G1 aphids were maintained on plants to confirm the production of asexual forms in LD.
Extracted molecule total RNA
Extraction protocol RNAs were extracted from heads using either the RNeasy Mini kit (Qiagen, Germantown, MD, USA). This Channel 1 sample corresponds to a mixture of total RNAs taken from the three replicated samples reared under Long Day photoperiod. RNAs were amplified by using MessageAmp aRNA kit (Ambion, Austin, TX, USA), starting with 2 µg of total RNA. RNAs were checked with a Bioanalyzer 2100 (Agilent Tech. Inc., Palo Alto, CA, USA), and quantified with a Nanodrop (Agilent).
Label Cy3
Label protocol 5 µg of aRNA were labelled and purified using the CyScribe Post-labelling (anchored oligo-dT primed) and the CyScribe GFX Purification kits (Amersham Biosciences-GE, Fairfield, CT, USA)
 
Channel 2
Source name Head of pea aphid reared under 12h photoperiod
Organism Acyrthosiphon pisum
Characteristics Strain: YR2 (red holocyclic clone)
Parthenogenetic female
10 days of 12h photoperiod
Instar stage L3
Parthenogenetic female producing sexual individuals
Biomaterial provider INRA Rennes, UMR 1099 BiO3P
Treatment protocol Short Day reared pea aphids
Growth protocol The clone YR2 of the pea aphid A. pisum was reared on broad bean (Vicia fabae) at 18°C. Parthenogenetic reproduction was maintained at 16 h of light and aphids were reared at low density (one to five individuals per plant) over three generations to prevent the production of winged forms. Conditions: 12 h of light (“short-day” or SD) that induced sexual forms after two generations. To initiate the experiment clonal third instar larvae (L3) were placed at SD photoperiod. This corresponds to generation G0. L3-G0 aphids reached adulthood (wingless adults or WA) and produced offspring (G1) that were transferred onto new plants and kept under SD conditions. A batch of 50 L3-G1 aphids was collected in the middle of the photophase (15:00) and immediately frozen in liquid nitrogen. As a control, few G1 aphids were maintained on plants to confirm the production of sexual forms in SD.
Extracted molecule total RNA
Extraction protocol RNAs were extracted from heads using either the RNeasy Mini kit (Qiagen, Germantown, MD, USA). RNAs were amplified by using MessageAmp aRNA kit (Ambion, Austin, TX, USA), starting with 2 µg of total RNA. RNAs were checked with a Bioanalyzer 2100 (Agilent Tech. Inc., Palo Alto, CA, USA), and quantified with a Nanodrop (Agilent).
Label Cy5
Label protocol 5 µg of aRNA were labelled and purified using the CyScribe Post-labelling (anchored oligo-dT primed) and the CyScribe GFX Purification kits (Amersham Biosciences-GE, Fairfield, CT, USA).
 
 
Hybridization protocol Hybridizations were performed in a Discovery XT System hybridization robot using the ChipMap 80 kit (Ventana Medical Systems, Tucson, AZ, USA) at the OUEST-Genopole and Agenae transcriptomic facilities (INRA Sribe, Rennes, France). Prehybridization was performed at 42ºC for 1 h in 2 ml of ChipSpread buffer containing 4xSSC and 0.2% SDS. Target cDNAs were mixed before hybridizations at 42ºC for 6 h (protocol N°2, ALC-D60/10-H48/8, Ventana). Washes were performed manually at room temperature in 1xSSC.
Scan protocol Fluorescent images of the microarrays were generated with a Genepix 4000B scanner and Genepix Pro analysis software v5.0 (Axon Instruments, Molecular Devices Co., Sunnyvale, CA, USA).
Description none
Data processing Raw data were normalized by the MADSCAN software. After subtraction of the fluorescence background, a rank-invariant method and a spatial normalisation were performed before a scaling of the variance within each slide and between all the slides at the same rank. The normalized values were log-transformed and used to perform statistical analysis by GeneANOVA. The contribution of each experimental factor (Gene, Photoperiod, Biological replicate, Dye, Technical replicate) and the interaction between them was evaluated by a global ANOVA. Differentially expressed genes where selected by imposing stringent cut-offs on the local ANOVA graphic of the interaction “Gene-Photoperiod”
 
Submission date Nov 22, 2006
Last update date Nov 27, 2006
Contact name Denis TAGU
E-mail(s) denis.tagu@rennes.inra.fr
Organization name INRA Rennes
Department UMR 1099 BiO3P
Street address BP35327
City Le Rheu
ZIP/Postal code BP35653
Country France
 
Platform ID GPL4580
Series (1)
GSE6363 Effect of day-length shortening on gene expression on pea aphid heads

Data table header descriptions
ID_REF
VALUE Log2(Gnorm/Rnorm)
Rmed Median of Cy3 fluorescence
Rbmed Background - median of Cy3 fluorescence
Gmed Median of Cy5 fluorescence
Gbmed Background of Cy5 fluorescence
Rnorm Normalisation of Rmed
Gnorm Normalisation of Gmed
A coefficient of variation: (Log2Rnorm+Log2Gnorm)/2

Data table
ID_REF VALUE Rmed Rbmed Gmed Gbmed Rnorm Gnorm A
1a -0.28 2295 60 2430 116 2062 2504 11.15
2a 0.9 1517 57 510 121 1031 553 9.56
3a 0.71 1950 66 838 122 1484 907 10.18
4a 1.66 3688 67 1321 122 3692 1168 11.02
5a -0.98 3712 67 10026 129 4270 8422 12.55
6a 0.49 3069 66 2341 119 3051 2172 11.33
7a 0.45 3755 67 3678 123 4226 3093 11.82
8a 1.03 2295 67 880 121 1852 907 10.34
9a 0.8 1658 68 602 123 1152 662 9.77
10a -0.04 178 64 166 109 79 82 6.33
11a 0.64 9356 65 11873 117 13034 8364 13.35
12a 1.17 1737 65 513 116 1222 543 9.67
13a 1.15 1915 69 594 117 1394 628 9.87
14a -0.27 1253 66 762 112 801 965 9.78
15a 0.26 1863 59 1061 116 1428 1193 10.35
16a 0.03 1340 60 712 121 876 858 9.76
17a 0.14 1827 69 1115 122 1389 1261 10.37
18a 0.22 4937 65 6736 121 6123 5257 12.47
19a 0.87 2535 67 1184 121 2187 1197 10.66
20a 0.66 2326 69 1182 118 1951 1235 10.6

Total number of rows: 6720

Table truncated, full table size 277 Kbytes.




Supplementary data files not provided

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