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Sample GSM133628

Query DataSets for GSM133628

Status

Public on Mar 26, 2007

Title

MDA-MB-435 hg133a21

Sample type

RNA

Source name

ductal breast carcinoma

Organism

Homo sapiens

Characteristics

age: 31
cell_type: ductal breast carcinoma
disease_state: ductal breast carcinoma; metastatic site: pleural effusion; In a recent study using cDNA microarrays, the parent line (MD A-MB-435) of MDA-MB-435S clustered with cell lines of melanoma origin. Ross DT et al. Nature Genetics 24: 227-235, 2000 )
sex: female

Biomaterial provider

no institution; R. Cailleau; Cancer Res 40:3118-3129,1980

Growth protocol

NCI60Adherent; RNA harvesting protocol for adherent cells Media used: RPMI 1640 500 ml FBS 25 ml -use the DTP serum if possible, from Bio Whittaker, not heat inactivated 200 mM Glutamine 5 ml 1 flask = ~15 x 106 cells yields ~ 100 ugr RNA. Grow 10 flasks. Cells: start from growing cells from Frederick (not frozen). Started before at passage #8-12. Do not use past passage 20. Growth schedule prior to harvest: Grow cells to ~80 confluencey. Trypsinize cells with 5 ml try-EDTA per T162, 15 min., 370C. Pipet up and down several times w 10 ml pipet to get good dispersment of cells. Count cells. Pass cells to as many flasks as there are cells for. When passing cells, combine flasks into a single pool. Pass 1x106 cells into each T162 w 30 ml media. Repeat growth cycle until 10 flasks are available. Refeed Refeed cells the day prior to harvest without harvesting). Draw off media (wo cells). Add back media, 30 ml per T162. Add back to T-162âs. 37 deg C, ON Harvest Target confluency 80% # of flasks = 10 Draw off media from 1st flask. Lyse cells in 15 ml lysis buffer (w 10 ul fresh BME per ml). Scrape cells. Draw off media from 2nd flask. Pipet lysis buffer from flask 1 into flask 2. Repeat lysis with up to 4 T162âs. Pipet into 50 ml tube. Repeat w next set of 4 flasks. When done, vortex 10 sec.. Draw lysate thru a 20 guage needle 12xâs. Freeze at ö800C. Purify using Quiagen Midi Kit. Use a maximun of 100 x 106 cells per column. More will not bind to the column. Company Info ------------ Quiagen Midi Kit Cat # 75144 RLT Buffer (lysis buffer) Cat. # 79216 $60-list, $51- discounted 1-800-362-7737 Fetal Bovine Serum 500 ml, list $261- Cat #14-502F Lot # 9S083F Cambrex (old Bio Whittaker) 1-800-638-8174 1x PBS pH 7.3-7.5 Bio Whittaker cat #17-516F $5.30 per 500 ml bottle (1-11) 250 ml conical tubes Corning cat #25350-250 RPMI-1640 wo L-glutamine cat # 12-167F $13.25 per 500 ml bottle (for 1-11 bottles) Cambrex (old Bio Whittaker) Walkersville, Md. 21793 301-898-7025 1-800-638-8174 Trypsin (0.05%)-EDTA (0.1%) In phosphate buffered saline without calcium and magnesium. cat # 118-087-061 $4.20 per 100 ml bottle Quality Biological, Inc. 301-840-9331 L-glutamine 200 mM, 100x Gibco-BRL cat # 25030-149 20 ml 1-800-828-6686 162 cm2 flask cat # 3150 Costar Tissue Culture Cell Scrapper, 25 cm Sarstedt Cat. # 83.1830 Cells are received from Nick Scudiero, E-mail: SCUDIERO@dtpax2.ncifcrf.gov Also trypsin, FBS and glutamine have been coming from there as well.; Protocol Type = grow;

Extracted molecule

total RNA

Extraction protocol

NCI60 Extraction Protocol; Harvest Target confluency 80% # of flasks = 10 Draw off media from 1st flask. Lyse cells in 15 ml lysis buffer (w 10 ul fresh BME per ml). Scrape cells. Draw off media from 2nd flask. Pipet lysis buffer from flask 1 into flask 2. Repeat lysis with up to 4 T162’s. Pipet into 50 ml tube. Repeat w next set of 4 flasks. When done, vortex 10 sec.. Draw lysate thru a 20 guage needle 12x’s. Freeze at –800C. Purify using Quiagen Midi Kit. Use a maximun of 100 x 106 cells per column. More will not bind to the column. ; Protocol Type = nucleic_acid_extraction;

Label

biotin

Label protocol

Affymetrix Labeling Protocol; The exact protocol is not available. But Standard Operating Proceadure can be found at http://www.affymetrix.com/support/technical/manual/expression_manual.affx or http://www.affymetrix.com/Auth/support/downloads/manuals/expression_ever_manual.zip Manual number: 701025 Revision 6, page 2.1.3; Protocol Type = labeling;

Hybridization protocol

Scan protocol

Affymetrix CEL analysis (Percentile); Protocol Type = feature_extraction; Parameter CellMargin = 2; Parameter OutlierHigh = 1.500; Parameter OutlierLow = 1.004; Parameter Percentile = 75; Software: Affymetrix MicroArraySuite, type: feature_extraction_software;
Protocol Type = image_acquisition; Software: Affymetrix MicroArraySuite, type: image_acquisition_software; Hardware: ;

Description

Background Avg = 40.73
Background Max = 43.9
Background Min = 37.9
Background Stdev = 1.02
Central- Avg = 1429
Central- Count = 9
Corner+ Avg = 40
Corner+ Count = 32
Corner- Avg = 1735
Corner- Count = 32
Noise Avg = 1.64
Noise Max = 2.0
Noise Min = 1.4
Noise Stdev = 0.09
RawQ = 1.62
Columns = 712
Number of Cells = 506944
Rows = 712
OrganismPart: skin

Data processing

ExpressionStat; Protocol Type = bioassay_data_transformation; Parameter Alpha1 = 0.05; Parameter Alpha2 = 0.065; Parameter BG = 4; Parameter Epsilon = 0.5; Parameter Gamma1H = 0.0045; Parameter Gamma1L = 0.0045; Parameter Gamma2H = 0.006; Parameter Gamma2L = 0.006; Parameter HZ = 4; Parameter NF = 1.000000000000; Parameter Perturbation = 1.1; Parameter SF = 1.000000000000; Parameter SmoothFactorBG = 100; Parameter Tau = 0.015; Parameter VZ = 4; Software: Affymetrix GeneChip Operating Software, type: bioassay_data_transformation_software;

Submission date

Sep 01, 2006

Last update date

Sep 01, 2016

Contact name

Uma T Shankavaram

E-mail(s)

uma@mail.nih.gov

Phone

301-496-6718

Organization name

NIH

Department

NCI

Lab

Radiation Oncology Branch

Street address

9000 Rockville Pike

City

Bethesda

State/province

ZIP/Postal code

20892

Country

USA

Platform ID

GPL96

Series (1)

GSE5720

Comparison between cell lines from 9 different cancer tissue (NCI-60) (U133 platform)

Relations

Reanalyzed by

GSE86363

Data table header descriptions
ID_REF	The name of the probe set.; Type: string_datatype; Scale: unscaled
CHPPairs	The number of probe pairs in the probe set.; Type: integer; Scale: linear_scale
CHPPairsUsed	The number of probe pairs in the probe set used in the Detection call.; Type: integer; Scale: linear_scale
VALUE	A measure of the relative abundance of a transcript.; Type: float; Scale: linear_scale
CHPDetection	A measurement indicating if the transcript was detected (Present), not detected (Absent) or marginally detected (Marginal). Can be one of "A", "M", "P" or "No Call".; Type: string_datatype; Scale: unscaled
CHPDetectionPvalue	See Detection p-value; Type: float; Scale: linear_scale

Data table
ID_REF	CHPPairs	CHPPairsUsed	VALUE	CHPDetection	CHPDetectionPvalue
AFFX-BioB-5_at	20	20	721.9	Present	0.00005
AFFX-BioB-M_at	20	20	3508.7	Present	0.00004
AFFX-BioB-3_at	20	20	3395.8	Present	0.00004
AFFX-BioC-5_at	20	20	120.7	Present	0.00020
AFFX-BioC-3_at	20	20	235.6	Present	0.00004
AFFX-BioDn-5_at	20	20	0.8	Absent	0.95704
AFFX-BioDn-3_at	20	20	4015.0	Present	0.00004
AFFX-CreX-5_at	20	20	1231.8	Present	0.00005
AFFX-CreX-3_at	20	20	280.5	Present	0.00007
AFFX-DapX-5_at	20	20	82.4	Present	0.00006
AFFX-DapX-M_at	20	20	167.4	Present	0.00110
AFFX-DapX-3_at	20	20	59.5	Present	0.00180
AFFX-LysX-5_at	20	20	4.0	Absent	0.35445
AFFX-LysX-M_at	20	20	8.8	Absent	0.55935
AFFX-LysX-3_at	20	20	4.9	Absent	0.35445
AFFX-PheX-5_at	20	20	0.4	Absent	0.96034
AFFX-PheX-M_at	20	20	2.2	Absent	0.74920
AFFX-PheX-3_at	20	20	12.4	Absent	0.25080
AFFX-ThrX-5_at	20	20	0.8	Absent	0.94156
AFFX-ThrX-M_at	20	20	5.0	Absent	0.41138

Total number of rows: 22283

Table truncated, full table size 812 Kbytes.

Supplementary file	Size	Download	File type/resource
GSM133628.CEL.gz	3.2 Mb	(ftp)(http)	CEL