NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM88827 Query DataSets for GSM88827
Status Public on Dec 24, 2005
Title 58
Sample type RNA
 
Channel 1
Source name BS3
Organism Zea mays
Characteristics Zea mays, Leaf, Development
Treatment protocol Bundle sheath prep
Growth protocol 10 days, 16h Light:8h Dark, 500umol m-2 s-1 light, 28C
Extracted molecule total RNA
Label Cy3
 
Channel 2
Source name ME3
Organism Zea mays
Characteristics Zea mays, Leaf, Development
Treatment protocol Mesophyll prep
Growth protocol 10 days, 16h Light:8h Dark, 500umol m-2 s-1 light, 28C
Extracted molecule total RNA
Label Cy5
 
 
Description A number of taxa utilize C4 photosynthesis, to limit the impact of photorespiration upon photosynthetic performance. In order to achieve a local elevation of CO2 concentration, maize plants possess two photosynthetic cell types. Rubisco accumulation is restricted to bundle sheath (BS) cells that surround the leaf veins. Carbon fixation occurs initially in adjacent mesophyll (ME) cells. C4 compounds are transported into the BS cells where they are subsequently decarboxylated, releasing CO2. Although the major components of the C4 pathway have been well characterized, less is known about further metabolic partitioning in the maize leaf. Microarray hybridizations have been performed in order to further investigate metabolic differences between BS and ME cell types. BS strands and ME protoplasts were isolated from the leaves of 10 day old maize seedlings by mechanical disruption and enzymatic digestion respectively. To control for differences arising from these different protocols, total leaf (TO) and total leaf stress (ST) samples were also isolated. The ST sample was subjected to the same treatments as the ME sample, with the omission of cell-wall degrading enzymes. Leaves for the TO sample were harvested as for the BS strand sample. An interwoven loop design was used to compare the four treatment groups. A biological group consisted of a growth of plants from which pooled individuals were taken for the four treatments. Six biological replicates (groups) were used. Labeling was performed using the Genisphere Array 900-MPX kit according to the manufacturer's protocol. Post hybridization washes were performed according to the recommendations of the Maize Oligo Array Project. Scan settings were used for detection of moderate to high expression signals (gain ~ 60%. power 90%). Following hybridization with TO cDNA, ~1/3 of features provided signal above twice background and below saturation.
Data processing The TIFF images were quantified using Genepix 5.0. Local background was subtracted from the signal value and the data was normalized using the quantile method in the limma package of bioconductor.
 
Submission date Dec 21, 2005
Last update date Dec 21, 2005
Contact name Ruairidh J Sawers
E-mail(s) rjs47@cornell.edu
Organization name Boyce Thompson Institute
Lab Bruntell
Street address Tower Rd
City Ithaca
State/province NY
ZIP/Postal code 14850
Country USA
 
Platform ID GPL1991
Series (1)
GSE3890 Gene expression profiling of bundle sheath and mesophyll cell types of wild-type maize seedlings.

Data table header descriptions
ID_REF Spot identifier for each feature
VALUE Normalized log2 ratio of normalized intensities defined by CH2/CH1. This value is set to null if it is flagged with "M" or "X"
CH1_NORMALIZED Normalized background subtracted CH1 intensity (RED channel)
CH1_RAW Background (CH1_BACKGROUND) subtracted raw intensity (F635 Mean - B635 Media)
CH1_BACKGROUND CH1 background median intensity (B635 Media)
CH2_NORMALIZED Normalized background subtracted CH2 intensity (GREEN channel)
CH2_RAW Background (CH2_BACKGROUND) subtracted raw intensity (F532 Mean - B532 Media)
CH2_BACKGROUND CH2 background median intensity (B532 Media)
FLAG B: no flag, good spot; X: undetectable spot; M: flagged for diameter < 70 microns, the percentage of saturated pixels > 30% or not validated PCR product

Data table
ID_REF VALUE CH1_NORMALIZED CH1_RAW CH1_BACKGROUND CH2_NORMALIZED CH2_RAW CH2_BACKGROUND FLAG
102435 null 0 65 393 0 348 552 M
102436 -0.167 21645 26496 361 19317 15780 520 B
102437 null 0 92 358 0 98 492 X
102438 null 0 73 333 0 143 488 X
102439 0.585 285 277 329 427 440 487 B
102440 null 0 98 335 0 85 499 X
102441 0.799 256 248 339 446 461 487 B
102442 null 0 277 322 0 314 448 M
102443 -0.233 3143 3321 329 2679 2536 474 B
102444 0.595 1751 1832 325 2651 2533 462 B
102445 1.531 2911 3190 320 8408 7673 458 B
102446 0.856 304 301 314 551 556 464 B
102447 0.163 389 386 318 434 438 428 B
102448 null 0 2124 322 0 3234 431 M
102449 null 0 59 315 0 131 414 X
102450 null 0 79 307 0 107 417 X
102451 null 0 63 306 0 63 410 X
102452 0.356 151 106 304 194 277 416 B
102453 null 0 52 311 0 133 402 X
102454 -0.339 4329 4650 318 3402 3167 407 B

Total number of rows: 32448

Table truncated, full table size 1147 Kbytes.




Supplementary data files not provided

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