I second the finding that >1Gb files work best when uploading from a URL, and also best if gzip'd beforehand. Best, Dan On Thu, Apr 8, 2010 at 8:31 AM, Ian Donaldson < Ian.Donaldson@manchester.ac.uk> wrote:
I find the only reliable way to upload files >1Gb is via a URL.
Ian
Quoting Peter Andrews <Peter.Andrews@dartmouth.edu>:
I also find that uploading a file rarely works -- it just displays the
loading up blue arrow forever.
On 4/7/2010 9:23 PM, galaxy-user-request@lists.bx.psu.edu wrote:
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Today's Topics:
1. Re: Upload file (Daniel Blankenberg) 2. Re: Upload file (Yanwei Tan) 3. Re: Upload file (Daniel Blankenberg) 4. Problem w/Cheetah, repeating dataset input (Jesse Erdmann) 5. Re: Quality based trimming (Florent Angly)
----------------------------------------------------------------------
Message: 1 Date: Wed, 7 Apr 2010 09:53:19 -0400 From: Daniel Blankenberg<dan@bx.psu.edu> To: Yanwei Tan<Tan@nbio.uni-heidelberg.de> Cc:galaxy-user@lists.bx.psu.edu <Cc%3Agalaxy-user@lists.bx.psu.edu> Subject: Re: [galaxy-user] Upload file Message-ID:<37031484-8E2E-4A9C-A027-D0D75F8D0799@bx.psu.edu> Content-Type: text/plain; charset=us-ascii
Hi Wei,
3Gb is not that large of a file and should upload without issue. How are you uploading the file? - May I suggest that you try placing the file in a web-accessable location and provide the url to the upload tool in the paste box.
Galaxy does accept the upload of individual gzipped files which can greatly reduce the time required for the transfer.
Thanks,
Dan
On Apr 6, 2010, at 6:04 PM, Yanwei Tan wrote:
Hi Dan,
Here I met a problem regarding the speed of upload file into Galaxy. Since my data is around 3G fastq file, I uploaded two days ago, the uploading still did not finish yet. I was wondering if I should try the zip compressed file.
Many thanks! Wei
On 4/6/10 5:00 PM, Daniel Blankenberg wrote:
Hi Florent,
Thanks very much for the comments. A sliding window sounds like an excellent approach: allow users to specify the window size, step size, an aggregation action to perform on the window (min, max, sum, mean, etc ), a comparison method (<,<=, ==, etc) and a threshold quality value; allowing users to specify the ends (both or only one or the other) to trim would also likely be useful. Would it also be desirable to allow specifying a number of quality scores that can be excluded from the aggregation action (the zero low quality base pairs in your example)? A window size of 1 would handle the simple case of only trimming the very ends while allowing the user to configure more complex windowing schemes. Thoughts?
Thanks,
Dan
On Apr 6, 2010, at 4:00 AM, Florent Angly wrote:
Thanks for your reply Daniel.
You are correct that there is not currently a tool to trim directly > by quality in Galaxy; currently the the Summary statistics and boxplot tools > are used to determine good cut off for use in the trim by column tool; > percentage of read length can be more useful on variable length reads. > However, adding a tool that can directly trim reads based upon a threshold > quality score seems like a natural fit for Galaxy, when uniform read length > is not present at the start and/or not a requirement at the end and the > percentage-of-read-length method is not sufficient > > > > That's right... I did not even think about using the boxplot tool to find how much to trim the ends. My reads all have the same length, but still, is seems more natural to only trim as much as needed and no more. For example, I have some reads that are completely low quality and should entirely trimmed/removed, whereas some might of good quality over almost all their length.
Lets verify that you are looking for something like this, where 'x' > is a low quality base and 'o' is a high quality base: > Start with: > xxxooooxxooooxxx > after trimming ends for 'x': > ooooxxoooo > So that trimming happens only from the ends and stops as soon as a > base above the threshold is found and internal low quality bases are not > considered. > > > > It's probaby better to use a short sliding window (of, say, 5 bp) and trim the ends until the window has no more than, say zero low quality base pairs. So, the following sequence would be converted from: xxxoxooooooxxooooooxoxxx to: ooooooxxoooooo
Florent
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_______________________________________________
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--
Yanwei Tan Institute of Neurobiology 1.OG, AG Bading Im Neuenheimer Feld 364 University of Heidelberg 69120 Heidelberg Germany
Tel:+49-6221-548319 Fax:+49-6221-546700
------------------------------
Message: 2 Date: Wed, 07 Apr 2010 17:21:37 +0200 From: Yanwei Tan<Tan@nbio.uni-heidelberg.de> To: Daniel Blankenberg<dan@bx.psu.edu> Cc:galaxy-user@lists.bx.psu.edu <Cc%3Agalaxy-user@lists.bx.psu.edu> Subject: Re: [galaxy-user] Upload file Message-ID:<4BBCA301.80907@nbio.uni-heidelberg.de> Content-Type: text/plain; charset=ISO-8859-1; format=flowed
Hi Dan,
Many thanks for your reply. I just upload the file from my computer and browse the location. If I upload the zip compressed file, should I choose txtseq.zip format? My data is fastq file in txt file. And how could I put the file in a web-accessible location? You mean the FTP server?
Thanks for your help! Wei
On 4/7/10 3:53 PM, Daniel Blankenberg wrote:
Hi Wei,
3Gb is not that large of a file and should upload without issue. How are you uploading the file? - May I suggest that you try placing the file in a web-accessable location and provide the url to the upload tool in the paste box.
Galaxy does accept the upload of individual gzipped files which can greatly reduce the time required for the transfer.
Thanks,
Dan
On Apr 6, 2010, at 6:04 PM, Yanwei Tan wrote:
Hi Dan,
Here I met a problem regarding the speed of upload file into Galaxy. Since my data is around 3G fastq file, I uploaded two days ago, the uploading still did not finish yet. I was wondering if I should try the zip compressed file.
Many thanks! Wei
On 4/6/10 5:00 PM, Daniel Blankenberg wrote:
Hi Florent,
Thanks very much for the comments. A sliding window sounds like an excellent approach: allow users to specify the window size, step size, an aggregation action to perform on the window (min, max, sum, mean, etc ), a comparison method (<,<=, ==, etc) and a threshold quality value; allowing users to specify the ends (both or only one or the other) to trim would also likely be useful. Would it also be desirable to allow specifying a number of quality scores that can be excluded from the aggregation action (the zero low quality base pairs in your example)? A window size of 1 would handle the simple case of only trimming the very ends while allowing the user to configure more complex windowing schemes. Thoughts?
Thanks,
Dan
On Apr 6, 2010, at 4:00 AM, Florent Angly wrote:
Thanks for your reply Daniel. > > > > You are correct that there is not currently a tool to trim directly >> by quality in Galaxy; currently the the Summary statistics and boxplot tools >> are used to determine good cut off for use in the trim by column tool; >> percentage of read length can be more useful on variable length reads. >> However, adding a tool that can directly trim reads based upon a threshold >> quality score seems like a natural fit for Galaxy, when uniform read length >> is not present at the start and/or not a requirement at the end and the >> percentage-of-read-length method is not sufficient >> >> >> >> >> That's right... I did not even think about using the boxplot tool > to find how much to trim the ends. My reads all have the same length, but > still, is seems more natural to only trim as much as needed and no more. For > example, I have some reads that are completely low quality and should > entirely trimmed/removed, whereas some might of good quality over almost all > their length. > > > > > Lets verify that you are looking for something like this, where 'x' >> is a low quality base and 'o' is a high quality base: >> Start with: >> xxxooooxxooooxxx >> after trimming ends for 'x': >> ooooxxoooo >> So that trimming happens only from the ends and stops as soon as a >> base above the threshold is found and internal low quality bases are not >> considered. >> >> >> >> >> It's probaby better to use a short sliding window (of, say, 5 bp) > and trim the ends until the window has no more than, say zero low quality > base pairs. So, the following sequence would be converted from: > xxxoxooooooxxooooooxoxxx > to: > ooooooxxoooooo > > Florent > > _______________________________________________ > galaxy-user mailing list > galaxy-user@lists.bx.psu.edu > http://lists.bx.psu.edu/listinfo/galaxy-user > > > > _______________________________________________ galaxy-user mailing list galaxy-user@lists.bx.psu.edu http://lists.bx.psu.edu/listinfo/galaxy-user
------------------------------
Message: 3 Date: Wed, 7 Apr 2010 11:32:05 -0400 From: Daniel Blankenberg<dan@bx.psu.edu> To: Yanwei Tan<Tan@nbio.uni-heidelberg.de> Cc:galaxy-user@lists.bx.psu.edu <Cc%3Agalaxy-user@lists.bx.psu.edu> Subject: Re: [galaxy-user] Upload file Message-ID:<54E8CB9D-5C36-4A20-8C8A-188B3F908012@bx.psu.edu> Content-Type: text/plain; charset=us-ascii
Hi Wei,
To upload a gzipped file (e.g. somefile.fastq.gz), just upload as you normally would (don't set to txtseq.zip - this is a special format), the file will be ungzipped automatically; zip files are not yet supported.
As far as a web-accessible location, you can specify http(s) and ftp locations by entering e.g.http://someserver.org/somefile.fastq orftp:// someserver.org/somefile.fastq into the 'paste' box in the upload tool, if you have access this type of resource.
Thanks,
Dan
On Apr 7, 2010, at 11:21 AM, Yanwei Tan wrote:
Hi Dan,
Many thanks for your reply. I just upload the file from my computer and browse the location. If I upload the zip compressed file, should I choose txtseq.zip format? My data is fastq file in txt file. And how could I put the file in a web-accessible location? You mean the FTP server?
Thanks for your help! Wei
On 4/7/10 3:53 PM, Daniel Blankenberg wrote:
Hi Wei,
3Gb is not that large of a file and should upload without issue. How are you uploading the file? - May I suggest that you try placing the file in a web-accessable location and provide the url to the upload tool in the paste box.
Galaxy does accept the upload of individual gzipped files which can greatly reduce the time required for the transfer.
Thanks,
Dan
On Apr 6, 2010, at 6:04 PM, Yanwei Tan wrote:
Hi Dan,
Here I met a problem regarding the speed of upload file into Galaxy. Since my data is around 3G fastq file, I uploaded two days ago, the uploading still did not finish yet. I was wondering if I should try the zip compressed file.
Many thanks! Wei
On 4/6/10 5:00 PM, Daniel Blankenberg wrote:
Hi Florent, > > Thanks very much for the comments. A sliding window sounds like an > excellent approach: allow users to specify the window size, step size, an > aggregation action to perform on the window (min, max, sum, mean, etc ), a > comparison method (<,<=, ==, etc) and a threshold quality value; allowing > users to specify the ends (both or only one or the other) to trim would also > likely be useful. Would it also be desirable to allow specifying a number of > quality scores that can be excluded from the aggregation action (the zero > low quality base pairs in your example)? A window size of 1 would handle the > simple case of only trimming the very ends while allowing the user to > configure more complex windowing schemes. Thoughts? > > Thanks, > > Dan > > On Apr 6, 2010, at 4:00 AM, Florent Angly wrote: > > > > > Thanks for your reply Daniel. >> >> >> >> You are correct that there is not currently a tool to trim directly >>> by quality in Galaxy; currently the the Summary statistics and boxplot tools >>> are used to determine good cut off for use in the trim by column tool; >>> percentage of read length can be more useful on variable length reads. >>> However, adding a tool that can directly trim reads based upon a threshold >>> quality score seems like a natural fit for Galaxy, when uniform read length >>> is not present at the start and/or not a requirement at the end and the >>> percentage-of-read-length method is not sufficient >>> >>> >>> >>> >>> That's right... I did not even think about using the boxplot tool >> to find how much to trim the ends. My reads all have the same length, but >> still, is seems more natural to only trim as much as needed and no more. For >> example, I have some reads that are completely low quality and should >> entirely trimmed/removed, whereas some might of good quality over almost all >> their length. >> >> >> >> >> Lets verify that you are looking for something like this, where 'x' >>> is a low quality base and 'o' is a high quality base: >>> Start with: >>> xxxooooxxooooxxx >>> after trimming ends for 'x': >>> ooooxxoooo >>> So that trimming happens only from the ends and stops as soon as a >>> base above the threshold is found and internal low quality bases are not >>> considered. >>> >>> >>> >>> >>> It's probaby better to use a short sliding window (of, say, 5 bp) >> and trim the ends until the window has no more than, say zero low quality >> base pairs. So, the following sequence would be converted from: >> xxxoxooooooxxooooooxoxxx >> to: >> ooooooxxoooooo >> >> Florent >> >> _______________________________________________ >> galaxy-user mailing list >> galaxy-user@lists.bx.psu.edu >> http://lists.bx.psu.edu/listinfo/galaxy-user >> >> >> >> _______________________________________________ > galaxy-user mailing list > galaxy-user@lists.bx.psu.edu > http://lists.bx.psu.edu/listinfo/galaxy-user > > > >
------------------------------
Message: 4 Date: Wed, 7 Apr 2010 16:25:37 -0500 From: Jesse Erdmann<jerdmann@umn.edu> To:galaxy-user@bx.psu.edu <To%3Agalaxy-user@bx.psu.edu> Subject: [galaxy-user] Problem w/Cheetah, repeating dataset input Message-ID: <m2h97174eb21004071425o9cba9384i648744371304d210@mail.gmail.com> Content-Type: text/plain; charset=ISO-8859-1
Hi all,
I'm using the following XML:
... <inputs> <param type="data" format="txt" name="seqmeta" label="PAPS.seqmeta"/> <param type="data" format="txt" name="lib_info" label="Label Info"/> <repeat name="to_merge" title="Evaluation Inputs and Results"> <param type="select" name="pmm" label="Mismatch %" help="Maximum % of mismatch between the construct sequence and the comparison sequence."> <option value="10">10%</option> <option value="15">15%</option> <option value="20">20%</option> </param> <param type="text" name="max_length" label="Max Construct Length" value="25" /> <param format="fasta" name="fasta_in" type="data" label="FastA Output"/> <param format="txt" name="seq_stats" type="data" label="Sequence Stats"/> </repeat> </inputs> ... <configfiles> <configfile name="file_info"> #for $merge_set in enumerate( $to_merge ) #silent sys.stderr.write($merge_set.__str__() + "\n") #silent sys.stderr.write($merge_set.fasta_in.__str__()) #end for </configfile> </configfiles> ...
And getting the resulting output:
127.0.0.1 - - [07/Apr/2010:15:31:50 -0500] "POST /admin/tool_reload HTTP/1.1" 200 -"http://localhost:8080/admin/reload_tool" "Mozilla/5.0 (Macintosh; U; Intel Mac OS X 10.5; en-US; rv:1.9.2.2) Gecko/20100316 Firefox/3.6.2" 127.0.0.1 - - [07/Apr/2010:15:31:59 -0500] "POST /tool_runner/index HTTP/1.1" 200 -"http://localhost:8080/tool_runner/index" "Mozilla/5.0 (Macintosh; U; Intel Mac OS X 10.5; en-US; rv:1.9.2.2) Gecko/20100316 Firefox/3.6.2" galaxy.jobs.schedulingpolicy.roundrobin DEBUG 2010-04-07 15:32:03,765 RoundRobin queue: user/session did not exist, created new jobqueue for session = 6 galaxy.jobs DEBUG 2010-04-07 15:32:03,766 job 234 put in policy queue galaxy.jobs.schedulingpolicy.roundrobin DEBUG 2010-04-07 15:32:03,766 RoundRobin queue: retrieving job from job queue for session = 6 galaxy.jobs DEBUG 2010-04-07 15:32:03,766 dispatching job 234 to local runner galaxy.jobs DEBUG 2010-04-07 15:32:05,423 job 234 dispatched (0, {'seq_stats':<galaxy.tools.DatasetFilenameWrapper object at 0x572b390>, '__index__': 0, 'max_length': <galaxy.tools.InputValueWrapper object at 0x572b8d0>, 'fasta_in': <galaxy.tools.DatasetFilenameWrapper object at 0x572b810>, 'pmm': <galaxy.tools.SelectToolParameterWrapper object at 0x572b290>}) 127.0.0.1 - - [07/Apr/2010:15:32:03 -0500] "GET /history HTTP/1.1" 200 -"http://localhost:8080/tool_runner/index" "Mozilla/5.0 (Macintosh; U; Intel Mac OS X 10.5; en-US; rv:1.9.2.2) Gecko/20100316 Firefox/3.6.2" galaxy.jobs.runners.local ERROR 2010-04-07 15:32:07,356 failure running job 234 Traceback (most recent call last): File "/Users/jerdmann/Python/galaxy-central/lib/galaxy/jobs/runners/local.py", line 55, in run_job job_wrapper.prepare() File "/Users/jerdmann/Python/galaxy-central/lib/galaxy/jobs/__init__.py", line 386, in prepare config_filenames = self.tool.build_config_files( param_dict, self.working_directory ) File "/Users/jerdmann/Python/galaxy-central/lib/galaxy/tools/__init__.py", line 1364, in build_config_files f.write( fill_template( template_text, context=param_dict ) ) File "/Users/jerdmann/Python/galaxy-central/lib/galaxy/util/template.py", line 9, in fill_template return str( Template( source=template_text, searchList=[context] ) ) File "/Users/jerdmann/Python/galaxy-central/eggs/Cheetah-2.2.2-py2.5-macosx-10.3-fat-ucs2.egg/Cheetah/Template.py", line 1004, in __str__ return getattr(self, mainMethName)() File "cheetah_DynamicallyCompiledCheetahTemplate_1270672326_31_15888.py", line 86, in respond NotFound: cannot find 'fasta_in' while searching for 'merge_set.fasta_in'
So, I'm printing the merge_set dictionary and seeing a fasta_in key, but when I try to use fasta_in it can not be found. I'm assuming this is probably a syntax oversight on my part, but I'm not seeing it.
-- -------------- Peter Andrews Programmer Computational Genetics Lab Dartmouth Hitchcock Medical Center (603) 653-9963
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-- Dan Webster Ph.D. Student - Cancer Biology Laboratory of Paul Khavari CCSR BLDG, Rm 2150 269 Campus Drive Stanford, CA 94305 DanWebster@stanford.edu