MIRA3 has done really good jobs here, assembling yeast 454 and ill PE 90x90 data.
give it a try!
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Because you are wanting only the BAC portion in your final assembly, have you thought of filtering the Illumina data for reads that have, say, 50% identity to the 454 reads prior to a combined assembly?Leave a comment:
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I am not sure whether Newbler incorporates the FASTQ reads as part of the overlapping stage or whether it uses some kind of mapping assembly algorithm, but I would certainly give it a try and see how it goes. Obviously there's always a danger of running into memory or CPU issues with that many reads.Leave a comment:
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For what its worth, i can vouch for newbler 2.6 with 1.2 million titantium plus up to 2million HiSeq 100bp SE. did a good job with eukaryotic cDNALeave a comment:
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Can newbler really manage the quantity of data produced by Illumina? I have 171 million 100bp PE reads. It was my understanding that the typical OLC assemblers could not handle this.Leave a comment:
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I mean run Newbler with the 454 and Illumina reads. V2.6 supports Illumina FASTQ files and seems to do a pretty good job with the bacterial datasets I've tried it on. If you are finding it takes too long consider using the -large flag.Leave a comment:
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Thanks nick,
I had a look at your blog and I can see there are several alternatives. Just to clarify, when you say "add your illumina reads to a newbler 2.6 assembly" what program would you recommend for a first shot? Presumably not newbler itself, but a de Bruijn assembler like velvet?
Best,
KyleLeave a comment:
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I wrote a blog post on this subject:
I'd be inclined to add your Illumina reads to a Newbler 2.6 assembly as your starting point.Leave a comment:
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454 + Illumina Combined Assembly
Hi All,
I am looking for suggestions on how to combine data from both 454 and Illumina platforms. Briefly, I have 454 sequenced BACs with average insert sizes of 150kb covered to approximately 30X and an illumina 100bp PE genome of the same species covered to ~25X. I am interested in obtaining the least gapped assembly of the BAC sequences only - not a completely assembled genome of this species.
The only assembler I have attempted is velvet with -long libraries in addition to the -shortPaired library and this does not produce an assembly of comparable quality to my 454-only newbler 2.5p1 assemblies of just the BAC sequences. Any advice is greatly appreciated.
Best,
Kyle
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