User: James Ashmore
James Ashmore • 2.0k
- Reputation:
- 1,980
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- Location:
- UK/Edinburgh/MRC Centre for Regenerative Medicine
- Twitter:
- jma1991
- Last seen:
- 5 hours ago
- Joined:
- 3 years ago
- Email:
- j******@icloud.com
I am a PhD student in Simon Tomlinson's research group at the MRC Centre for Regenerative Medicine. My interests lie in the biology of reprogramming, and developing methods to analyse the reprogramming process.
Posts by James Ashmore
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... I'm trying to generate a ROC curve for different RNA-seq normalisations, using qRT-PCR data for comparison. I want to define True Positives from the RNA-seq data as genes which are measured as significantly differentially expressed (FDR < 0.05) in the same direction (logFC) from the qRT-PCR data. ...
written 11 days ago by
James Ashmore • 2.0k
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... Index your FASTA file:
samtools faidx input.fasta
Then get ids which start with "NM" and pipe them into samtools faidx to retrieve only those sequences:
cut -f 1 input.fasta.fai | egrep "^NM" | xargs samtools faidx input.fasta > result.fasta ...
written 19 days ago by
James Ashmore • 2.0k
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... As far as I know the fix mate command will check that two mates of a pair are actually in the file. Sometimes prior filtering will remove one mate of a pair, but it won't update the SAM flag which says both mates are present. Fix mate will run through the file and update the flag if it can't find th ...
written 19 days ago by
James Ashmore • 2.0k
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... Lets try with an example file (using line numbers instead of actual GFF content):
$ cat test.gff
1
2
3
4
5
6
7
8
9
##FASTA
11
12
13
14
15
Find the line number which the pattern first '##FASTA' appears (for example say line 10):
...
written 19 days ago by
James Ashmore • 2.0k
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... If you look at the "Building the results table" section of that workflow you'll see that the "results" function will give you a table of genes which are either up- or down- regulated in either group. ...
written 19 days ago by
James Ashmore • 2.0k
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... I can't find an explicit reference to a description argument in the ballgown constructor function so it must be an error from a function called within the ballgown constructor function. When you run R what is your working directory? The ballgown constructor function will look for data files in a sub ...
written 19 days ago by
James Ashmore • 2.0k
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... Okay I'm slightly confused, it sounds like you want to do a differential expression analysis (an example of which you can find in the workflow I linked). Is that correct? ...
written 19 days ago by
James Ashmore • 2.0k
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... Do you have access to the raw read counts? If so, please read https://f1000research.com/articles/4-1070/v2 ...
written 19 days ago by
James Ashmore • 2.0k
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... Download the bedClip tool from the [UCSC utilities webpage][1]. Run this on your bedGraph file and it should remove those features which are running off the end of your chromosomes
[1]: http://hgdownload.soe.ucsc.edu/admin/exe/ ...
written 20 days ago by
James Ashmore • 2.0k
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Comment:
C: Data retrieval from GEO
... I guess you could just use the grep command line tool to retrieve the GSE numbers:
grep "Series:" ...
written 20 days ago by
James Ashmore • 2.0k
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For A: Fix SAM flags on quality filtered paired-end BAM file
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For Trimmomatic not removing all Nextera adapters or N base calls
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For A: Fix SAM flags on quality filtered paired-end BAM file
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6 months ago,
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For Trimmomatic not removing all Nextera adapters or N base calls
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