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Platform GPL4564

Query DataSets for GPL4564

Status

Public on Nov 16, 2007

Title

Stanford Human cDNA SHEW

Technology type

spotted DNA/cDNA

Distribution

commercial

Organism

Homo sapiens

Manufacturer

Stanford Functional Genomics Facility

Manufacture protocol

Preparation of Slides to be used to make microarrays.
Last updated: October 6, 1999
Materials
Qty
Order info
Notes
Glass microscope slides
60
Gold Seal #3010
Slide rack
2
Shandon Lipshaw #121 (800-245-6212)
Each rack holds 30 slides
Slide chamber
6
Shandon Lipshaw #121
Each chamber holds 350 mL
ddH2O
~5 L
NaOH
70 g
95% Ethanol
420 mL
Poly-L-lysine
70 mL
Sigma #P 8920
Tissue culture PBS
70 mL
Vacuum oven (45C)
Slide box (plastic only)
1
VWR #48443-806
1. Place slides in slide racks. Place racks in chambers.
2. Prepare CLEANING SOLUTION:
a. Dissolve 70 g NaOH in 280 mL ddH2O.
b. Add 420 mL 95% ethanol. Total volume is 700 mL (= 2 X 350 mL); stir until completely mixed.
c. If solution remains cloudy, add ddH2O until clear.
3. Pour solution into chambers with slides; cover chambers with glass lids. Mix on orbital shaker for 2 hr. Once slides are clean, they should be exposed to air as little as possible. Dust particles will interfere with coating and printing.
4. Quickly transfer racks to fresh chambers filled with ddH2O. Rinse vigorously by plunging racks up and down. Repeat rinses 4X with fresh ddH2O each time. It is critical to remove all traces of NaOH-ethanol.
5. Prepare POLYLYSINE SOLUTION:
a. 70 mL poly-L-lysine + 70 mL tissue culture PBS in 560 mL water.
b. Use plastic graduated cylinder and beaker.
6. Transfer slides to polylysine solution and shake 15 min. - 1 hr.
7. Transfer rack to fresh chambers filled with ddH2O. Plunge up and down 5X to rinse.
8. Centrifuge slides on microtiter plate carriers (place paper towels below rack to absorb liquid) for 5 min. @ 500 rpm. Transfer slide racks to empty chambers with covers for transport to vacuum oven.
9. Dry slide racks in 45C vacuum oven for 10 min. (Vacuum is optional.)
10. Store slides in closed slide box (plastic only, without rubber mat bottom)
11. BEFORE PRINTING ARRAYS:
a. Check that polylysine coating is not opaque.

Submission date

Nov 16, 2006

Last update date

Jan 18, 2013

Contact name

Bao Jian Fan

E-mail(s)

baojian_fan@meei.harvard.edu

Phone

617-573-6448

Fax

617-573-6439

Organization name

Harvard Medical School

Department

Ophthalmology

Lab

Howe/Wiggs Lab

Street address

MEEI, 243 Charles Street

City

Boston

State/province

ZIP/Postal code

02114

Country

USA

Samples (9)

More...

GSM144696, GSM144701, GSM144702, GSM144703, GSM144704, GSM144705

Series (1)

GSE6298

Comparison of gene expression profile of human trabecular meshwork cells induced by triamcinolone with dexamethasone

Data table header descriptions
ID
Array_Block	Block on the array
Array_Row	Row on the array
Array_Column	Column on the array
Spot_Row	Row on each block
Spot_Column	Column on each block
ORF	Gene symbol
CLONE_ID	IMAGE Clone ID for each spot
SPOT_ID

Data table
ID	Array_Block	Array_Row	Array_Column	Spot_Row	Spot_Column	ORF	CLONE_ID	SPOT_ID
1	1	1	1	1	1	ITGB2	IMAGE:342721
2	1	1	1	1	2	IGFBP2	IMAGE:233721
3	1	1	1	1	3	MTIF2	IMAGE:50754
4	1	1	1	1	4	HMBS	IMAGE:126243
5	1	1	1	1	5	GATA6	IMAGE:234736
6	1	1	1	1	6	ICAM5	IMAGE:180864
7	1	1	1	1	7	SEMA3B	IMAGE:809892
8	1	1	1	1	8	RIN2	IMAGE:187147
9	1	1	1	1	9	WT1	IMAGE:503338
10	1	1	1	1	10	UNG2	IMAGE:769600
11	1	1	1	1	11	TIMP3	IMAGE:489519
12	1	1	1	1	12	TEGT	IMAGE:884766
13	1	1	1	1	13	SMPD1	IMAGE:729964
14	1	1	1	1	14	SLC6A1	IMAGE:177967
15	1	1	1	1	15	S100A8	IMAGE:562729
16	1	1	1	1	16	RPL36AL	IMAGE:884842
17	1	1	1	1	17	KLF6	IMAGE:510381
18	1	1	1	1	18		IMAGE:140574
19	1	1	1	1	19	PIP5K1A	IMAGE:293950
20	1	1	1	1	20	PPP1R8	IMAGE:278650

Total number of rows: 43200

Table truncated, full table size 1573 Kbytes.

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