User:Karmella Haynes/Notebook/PcTF Genomics/2013/01/07: Difference between revisions
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# Assign Binding Proteins to Experiments: Protein label = the appropriate binding protein (created in previous step). Click [Next >]. | # Assign Binding Proteins to Experiments: Protein label = the appropriate binding protein (created in previous step). Click [Next >]. | ||
# Setup Preprocessing: Desired preprocessing = QSeq; Normalization method = none; Sequence files against which to quantify = browse to Desktop > Human Genome Ref > select all NC...gbk files. | # Setup Preprocessing: Desired preprocessing = QSeq; Normalization method = none; Sequence files against which to quantify = browse to Desktop > Human Genome Ref > select all NC...gbk files. | ||
# Select "Use features of type(s)" and set to "gene". | ## Select "Use features of type(s)" and set to "gene". | ||
#Genome filtering = Discover peaks in the entire genome. | ## Genome filtering = Discover peaks in the entire genome. | ||
# Configure Advanced Options: under General, Graphs > Create Wiggle (.wig). Set Location to ChIPseq Wig Files on desktop. | ## Configure Advanced Options: under General, Graphs > Create Wiggle (.wig). Set Location to ChIPseq Wig Files on desktop. | ||
# Configure Advanced Options: under General, Alignment Files > Create BED Alignment (.bed). Set Location to ChIPseq BED Files on desktop. | ## Configure Advanced Options: under General, Alignment Files > Create BED Alignment (.bed). Set Location to ChIPseq BED Files on desktop. | ||
# Configure Advanced Options: under Peak Detection, is set to Qseq Peak Finder by default. Leave this as-is for now. | ## Configure Advanced Options: under Peak Detection, is set to Qseq Peak Finder by default. Leave this as-is for now. | ||
## Click [Next >]. Wait a while | |||
# Setup Attributes and Replicates: Show only grouping attributes (default). Click [Finish]. | |||
# Window with Peak Table and other tabs should appear. Finished! Explore the data. | |||
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* Set control 2_ and 7_aln_sorted as "yes" for "Is control?" | * Set control 2_ and 7_aln_sorted as "yes" for "Is control?" | ||
* Set 2_aln_sorted as control for 1_aln_sorted. Set 7_aln_sorted as control for 6_aln_sorted. | * Set 2_aln_sorted as control for 1_aln_sorted. Set 7_aln_sorted as control for 6_aln_sorted. | ||
** <font color="red">This analysis required too much disk space</font> | |||
* Started over, but only used '''chromosomes 1-3''' as reference templates (trying a few at a time). | |||
** This worked | |||
Results/ Notes: | |||
* Peak Table: shows very few hits for PcTF, many more for H3K27me3, no overlap! | |||
* Display wig file on UCSC Genome browser online - add file from "ChIPseq Wig Files" folder as a custom track; wig file shows raw data histogram | |||
** 1_aln_sorted.wig, 6_aln_sorted.wig | |||
* Display BED file on UCSC Genome browser online - add file from "ChIPseq BED Files" folder as a custom track; BED file shows | |||
** 1_aln_sorted.bed, 6_aln_sorted.bed | |||
Revision as of 13:24, 8 January 2013
Pc-TF Genomics | <html><img src="/images/9/94/Report.png" border="0" /></html> Main project page <html><img src="/images/c/c3/Resultset_previous.png" border="0" /></html>Previous entry<html> </html>Next entry<html><img src="/images/5/5c/Resultset_next.png" border="0" /></html> |
01/07/13
Array Star analysis
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