Seqanswers Leaderboard Ad

Collapse

Announcement

Collapse
No announcement yet.
This topic is closed.
X
This is a sticky topic.
X
X
 
  • Filter
  • Time
  • Show
Clear All
new posts

  • Thanks for your useful post.

    I’m interested in ABySS and I installed it on my linux server.
    However, I knew it does not use a reference genome, as it is a de novo assembler.
    I think it should be moved from "Align/Assemble to a reference" category to "De novo Align/Assemble" category.

    Cheers! ^^

    Comment


    • Originally posted by odysseus View Post
      ...I think it should be moved from "Align/Assemble to a reference" category to "De novo Align/Assemble" category.
      Done. Thanks

      Comment


      • Great list!
        I'd like to introduce some code I'm working on. I don't know if it deserves to go into the list, but it might be of some use for someone. Is not finished yet, but if someone is interested in trying it out or in working on it just let me know.
        You can find it at biolib.
        It's a library and a set of script targeted to NGS. There are modules to:
        - clean sequences (sanger, 454, ilumina).
        - parse caf, ace and bowtie map files.
        - clean and filter contigs.
        - look for snps and indels.
        - filter snps.
        - do statistics for: reads, contigs and snps.

        Be aware that it's just a work in progress and its in constant flux. The code is available under the AGPL.

        Comment


        • Beta version of the SEQwiki software database up and running...

          Check it out...





          Dan.
          Homepage: Dan Bolser
          MetaBase the database of biological databases.

          Comment


          • Hey, that's awesome - Great Job!
            The more you know, the more you know you don't know. —Aristotle

            Comment


            • Hi all,

              Thanks for the helpful list. Based on reading the post I've tried out Bowtie to align reads from a ChIP-seq experiment run on Illumina GA-II (the facility gave me non-aligned fastq). Worked great!

              I want to put the output into cisGenome or FindPeaks (or both). Can anyone advise me how to get it into the right format? Does FindPeaks convert any of the output options in Bowtie?

              Thanks

              Comment


              • Hi Dinny,

                Findpeaks can use bowtie's reads - but it depends if you want to use PET or SET tags. if you're using PET, you'll need to convert your reads into BED format, which is the only way that you can retain the pairing information. If you're using SET, you should be able to bet Bowtie to produce a .map file (if I recall correctly), which can then be processed natively by FindPeaks.

                If you need help with findPeaks, you can always send an email to the mailing list - I tend to reply more quickly to those inquiries than those on SeqAnswers.

                Cheers,
                Anthony
                The more you know, the more you know you don't know. —Aristotle

                Comment


                • I don't think that CisGenome has support for bowtie output yet. Best bet would be to find scripts to convert to .bed or .aln

                  Comment


                  • Thanks very much Anthony and ewilbanks.
                    I looked closer at Bowtie conversion tools and I can create a .map file from the alignment (I'm working with single-end reads), but I have to get Maq working to do it. I'll give it a go, and compare Maq alignment times while I'm at it ;-)
                    Cheers,
                    Dinny

                    Comment


                    • Hi Dinny,

                      I think there is also a way to get Bowtie to produce it's own alignment in .map format, if I recall correctly.

                      Anyhow, if you're working with SET, you can also convert the bowtie reads directly to .bed: https://sourceforge.net/apps/mediawi...e=ConvertToBed
                      The more you know, the more you know you don't know. —Aristotle

                      Comment


                      • what is the definition of the header line in SOLiD csfasta file, eg
                        1_88_1830_R3 -- What is 88, 1830 stands for ? Thanks

                        Comment


                        • Originally posted by jsun529 View Post
                          what is the definition of the header line in SOLiD csfasta file, eg
                          1_88_1830_R3 -- What is 88, 1830 stands for ? Thanks
                          See http://seqanswers.com/forums/showthread.php?p=7572.

                          Comment


                          • Hi Anthony,
                            Thanks again for the advice. Taking the reads directly into .bed would be better. The .map converter in Bowtie needs a library file created in Maq, so it would be easier to limit the number of applications the data goes through...less opportunity to completely jumble it.
                            Couldn't see a way to align straight to .map, but I'll look again.
                            Dinny

                            Comment


                            • Solexa findpeaks

                              Using Findpeaks sort reads on bowtie mapped alignment is taking up too much memory......!!!!! So I am trying using the GERALD maps reads directly from solexa to convert to wig files...I believe the solexa GERALD mapped alignments are ELAND format?
                              So the aligner type will be -aligner eland, to perform separateReads.jar?
                              Any suggestions?

                              Comment


                              • Hi Ka123,

                                There are other ways to do the sort - including several methods you could try from the linux command line. However, I'm really not sure why it's taking so memory. Could you give me a few ideas as to what your work flow is?

                                In the meantime, documentation and an example command for SeparateReads can be found here:

                                Download Vancouver Short Read Analysis Package for free. This package contains code for use with Short Read DNA Sequencing technologies, and includes packages for ChIP-Seq, Whole Transcriptome Shotgun Sequencing, Whole Genome Shotgun Sequencing, SNP Detection, Transcript expression and file conversion.
                                The more you know, the more you know you don't know. —Aristotle

                                Comment

                                Latest Articles

                                Collapse

                                • seqadmin
                                  Choosing Between NGS and qPCR
                                  by seqadmin



                                  Next-generation sequencing (NGS) and quantitative polymerase chain reaction (qPCR) are essential techniques for investigating the genome, transcriptome, and epigenome. In many cases, choosing the appropriate technique is straightforward, but in others, it can be more challenging to determine the most effective option. A simple distinction is that smaller, more focused projects are typically better suited for qPCR, while larger, more complex datasets benefit from NGS. However,...
                                  10-18-2024, 07:11 AM
                                • seqadmin
                                  Non-Coding RNA Research and Technologies
                                  by seqadmin




                                  Non-coding RNAs (ncRNAs) do not code for proteins but play important roles in numerous cellular processes including gene silencing, developmental pathways, and more. There are numerous types including microRNA (miRNA), long ncRNA (lncRNA), circular RNA (circRNA), and more. In this article, we discuss innovative ncRNA research and explore recent technological advancements that improve the study of ncRNAs.

                                  Nobel Prize for MicroRNA Discovery
                                  This week,...
                                  10-07-2024, 08:07 AM

                                ad_right_rmr

                                Collapse

                                News

                                Collapse

                                Topics Statistics Last Post
                                Started by seqadmin, Yesterday, 05:31 AM
                                0 responses
                                10 views
                                0 likes
                                Last Post seqadmin  
                                Started by seqadmin, 10-24-2024, 06:58 AM
                                0 responses
                                20 views
                                0 likes
                                Last Post seqadmin  
                                Started by seqadmin, 10-23-2024, 08:43 AM
                                0 responses
                                50 views
                                0 likes
                                Last Post seqadmin  
                                Started by seqadmin, 10-17-2024, 07:29 AM
                                0 responses
                                58 views
                                0 likes
                                Last Post seqadmin  
                                Working...
                                X