Question: Asking About Allignment Figure
0
Chandra Trihadi • 10 wrote:
Hello,
I am sorry, I did not know about the appropriate address (
galaxy-user@bx.psu.edu) for asking.
I tried to map with Bowtie for my illumina single-read data using the
reference genome that I uploaded to the history panel, then filter
SAM, then
did SAM-to-BAM. However, the final result did not display the
allignment
figure like on the instruction video. Would you mind to tell me how to
obtain the allignment figure or to assembly my illumina data based on
my
reference genome?
Thank you.
-Chandra-
Quoting Kelly Vincent <kpvincent@bx.psu.edu>:
[Show Quoted Text - 48 lines][Hide Quoted Text]
Hi,
Sorry for the delay in response. In the future, please do send queries
like
this to galaxy-user@bx.psu.edu<https: uamail.uark.edu="" h="" imp="" message.p="" hp?mailbox="Sent&index=486#">instead
of galaxy-bugs, since it is about using Galaxy rather than a
specific bug in the software.
One issue with our screencasts is that Galaxy changes rapidly so they
can
become slightly out of date. In this case, for Illumina data, there is
a
tool called "FASTQ Summary Statistics" under Illumina Data under NGS:
QC and
manipulation. This is like the "Compute quality statistics" tool under
AB-SOLiD Data. Then, to draw the boxplot, go to the Graph/Display Data
section (not under NGS Toolbox) and choose the "Boxplot of quality
statistics" tool.
Regarding the results of your Bowtie mapping, could you give more
details
about what was different from what you were expecting? Did you make
sure
that you mapped against the correct genome?
Regards,
Kelly
Hello Galaxy Team,
I am sorry for asking the same questions for the third time since I
haven't
gotten any respons from galaxy team about these problem.
Could you at least tell me why you do not answer my questions yet?
Should I call you?
I have illumina sequencing data (single reads), and I am trying to
analyze
it.
I listened to the video tutorial on Galaxy about mapping illumina
reads
(single end read), and tried to analyze my data based on the tutorial.
However, I found instructions that I could not find on the Galaxy
window.
- In the tutorial, after uploading the data, I should "compute quality
statistic". The "compute quality statistic" is supposed to be under
"GENERIC
FASTQ DATA". However, I found it under "AB Solid Data". Since my data
is
Illumina sequencing data, I could not simply do it.
- In the tutorial, if I am done with "compute quality statistic", I
have to
do "draw quality score boxplot" that is supposed to be under "GENERIC
FASTQ
DATA". However, it is also under "AB Solid Data".
- Then, after uploading my Illumina data, I did FASTQ Groomer, and did
mapping with Bowtie for Illumina, but the result was not like the
example on
the instruction video.
Would you mind to tell me what I should do?
Thank you very much in advance.
Yohanna Gita Chandra
University of Arkansas
Fayetteville, AR 72701
Email: ytrihadi@uark.edu<https: uamail.uark.edu="" h="" imp="" message.php?mai="" lbox="Sent&index=486#">&
chandratrihadi2@yahoo.com<https: uamail.uark.edu="" h="" imp="" message.php?ma="" ilbox="Sent&index=486#">
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modified 8.4 years ago
by
Jennifer Hillman Jackson ♦ 25k
•
written
8.4 years ago by
Chandra Trihadi • 10
