Hi Neva
I am trying to run juicer pipeline. I have some questions related to it and need some help too (I don’t have skills set that a bioinformatician do like you). Please can you help me in the following.
Here is a brief description of my work
We have done a Hi-C experiment on a plant genotype of a fruit species. Now we want to use Juicer to test that if Hi-C data from this genotype (sex-male ) can help in doing two things
1. In assembling the scaffolds generated from another fruit genotype (but same species). Can juicer be used for it-
2. 3D visualisation of the fruit genome of another genotype (but same species)
At the moment I am trying to do step 2 to visualise the 3D configuration for the fruit genome based on my H-iC dataset. For this purpose I m facing problem in understanding the kind of files I need to use for following folders in opt
References (Here I am using an already assembled genome fasta files in form of pseudomoleucles/chromosome AND NOT the scaffolds that are not assembled)
Restriction sites ( If I m correct, here we have to use the restriction enzyme used for HiC. In our case it is Sau3AI enzyme. So we generate a list of positions that Sau3AI restriction would cut on the References Pseudomolecules/chromosomes, meaning a list of cut positions for all pseudomolecules/Chr. If this is the case please can you advise me how to do it)
Looking forward to your response
cheers
Jibran
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File "<ipython-input-9-05b3a5e573de>", line 9 print 'Usage: %s <restriction enzyme> <genome> [hrpjxt/bioinf_HiC/myjuicer/opt/juicer/restriction_sites]' % (sys.argv[0]) ^ SyntaxError: invalid syntax
On Friday, June 23, 2017 at 6:21:06 PM UTC+12, Muhammad Shamim wrote:
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I would be happy to help, but I am not sure I fully understand your question about genotype. If you can elaborate I hope I might be able to answer that to a more satisfactory extent.
With respect to Lachesis these are pipelines with somewhat different functionality (3d-dna includes misassembly detection and does not rely on preliminary clustering of sequences based on chromosome territories) but they are designed with the same goal in mind: assembling chromosome-length genomes from draft sequences using Hi-C signal.
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juicer.sh-z <path to genome fasta file>,-p <path to mygenome.chrom.sizes>, and-y <path to mygenome_myenzyme.txt>
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