Quick search:
Gene
Anatomy
Accession ID
Function
for
Login
Feedback
Home
About GUDMAP
Goals
Projects
Publications
Contacts
Positions
Funding
Events
Links
Message Board
Citing GUDMAP
Gene Expression
Query/Browse Database
Tissue Summaries
ISH Quality Control
Resources
Submission Archive
Project Protocols
Mice/Cell Lines
3D Atlas
Ontology
UQ GUDMAP - Probe Design
Web Stats
Internal
Tutorials
Overview
Urinary Development
Reproductive Development
Disease
Help
Using Database
Website
Glossary
Clinicians
Biologists
Bioinformaticians
Public
System Requirements
Expression Database
Tissue Summaries
Analysis
Annotate
Downloads
Data Source
Collections
Expression Database
GUDMAP:13975
Theiler Stage
TS19
Images
Supplemental Data Files
CEL file:
11FlkM1.CEL
CHP file:
RPT file:
TXT file:
11FlkM1.TXT
Archive ID
234
Principal Investigator(s)
Blanche Capel,
Duke University Medical Center, Durham, NC, USA, b.capel@cellbio.duke.edu
Submitted By
Samantha A Jameson,
Duke University Medical Center, Durham, NC, USA, saj3@duke.edu
Specimen Details
Sample GEO ID:
GSM686199
Sample Description:
Gonad and mesonephros, 11.5 dpc male endothelial cells
Title:
11FlkM1
Component(s) Sampled:
developing vasculature of reproductive system (EMAP:31834)
Organism:
Mus musculus
Strain:
CD-1
Genotype:
Non-wild type Allele:
Gene
Kdr
MGI ID
MGI:4417934
MGI Symbol or lab name
Tg(Kdr-mCherry)1Medi
Type
transgenic insertion
Notes:
Provided by Mary E Dickinson (Baylor College of Medicine). Larina IV, Shen W, Kelly OG, Hadjantonakis AK, Baron MH, Dickinson ME. (2009). A membrane associated mCherry fluorescent reporter line for studying vascular remodeling and cardiac function during murine embryonic development. Anat Rec (Hoboken) 292 (3), 333-341.
PMID: 19248165
Sex:
male
Development Age:
11.5 dpc
Theiler Stage:
19
Pool Size:
one or more litters
Pooled Sample:
Yes
Dissection Method:
Dissected out the gonad and a portion of the mesonephros, trypsinized and FACS sorted. Capel protocol: FACS Protocol
Experimental Design:
Female mice were time-mated and the embryos were collected. The gonads were removed and the males and females were separately pooled. The gonads were incubated in Trypsin EDTA for 5-10 minutes. The trypsin was removed, PBS (often with DNase) was added, and the gonadal cells were dissociated by pipetting and pulling through a syringe. The samples were passed through a strainer and then FACS sorted. Capel protocol: FACS protocol.
Array Hybridization
Extracted Molecule:
Total RNA
A260:280 Ratio:
2.24 (questionable accuracy given low RNA amount)
RNA Extraction Protocol:
Capel protocol: RNA extraction and sample preparation for Affymetrix Gene 1.0 ST arrays
Target Amplification Manufacturer/kit:
Nugen WT-Ovation Pico RNA Amplification System (3300) and WT-Ovation Exon Module (2000)
Target Amplification Protocol:
Capel protocol: RNA extraction and sample preparation for Affymetrix Gene 1.0 ST arrays
Rounds of Amplification:
1
Amount Labeled Target Hybridized To Array:
Approximately 2.5 ?g into the hybridization cocktail, approximately 2.1 ?g were hybridized to the array.
Label:
Biotin
Label Protocol:
Nugen Encore Biotin Module (4200)
Array Hyb/Wash Protocol:
The arrays were washed and stained using the Affymetrix Fluidics Station 450. Fluidics Protocol FS450-0007.
Scan Protocol:
Probe arrays were scanned using an Affymetrix GeneChip Scanner 3000 7G and Affymetrix GeneChip Command Console (AGCC) Software version 3.1.1.
GCOS Tgt Value:
500
Data Analysis Method:
Partek
Reference:
Universal: P0 mouse (from Steve Potter)
Series Details
Series GEO ID:
GSE27715
Number of Samples:
91 samples
Title:
Gene expression profiles of germ cells, supporting cells, interstitial cells (including steroidogenic precursors), and endothelial cells in the developing testis and ovary at 115, 125, and 135 dpc (GUDMAP Series ID: 43)
Summary:
The goal of this study is to determine the complete gene expression profile for each cell type of the developing gonad during the critical window in which it adopts the testis or ovarian fate.
Type:
Expression profiling of FACS sorted gonadal cells by microarray.
Overall Design:
Transgenic mice with cell type specific fluorescent markers were used to isolate germ cells, supporting cells, interstitial cells (including steroidogenic precursors), and endothelial cells in the developing testis and ovary. The gonads were dissociated in trypsin, and the fluorescent cells were isolated by FACS. The RNA was collected from the isolated cells and their gene expression profiles were determined by microarray analysis.
Platform Details
Platform GEO ID:
GPL6246
Title:
Affymetrix Mouse Gene 1.0 ST Array
Distribution:
commercial
Technology:
in situ oligonucleotide
Organism:
Mus musculus
Manufacturer:
Affymetrix
Manufacturer Protocol:
N/A
Catalogue Number:
N/A
