Question

PacBio data assembly with Celera

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9.5 years ago

mhasa006 ▴ 70

I have a set of PacBio long reads in fastq file. I want to assemble them in contigs. Which assembler will work well? If Celera is the answer, could anyone give me a step by step approach of using celera for assembling PacBio long reads?

PacBio Celera Assembly • 3.6k views

ADD COMMENT • link updated 23 months ago by Ram 44k • written 9.5 years ago by mhasa006 ▴ 70

Ram · Answer 1 · 2015-06-10

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9.5 years ago

rhall ▴ 160

fastq extracted from bax.h5 are not corrected, I would suggest using either HGAP - that is part of PacBio's SMRT Analysis system, or PBcR.

ADD COMMENT • link updated 23 months ago by Ram 44k • written 9.5 years ago by rhall ▴ 160

Ram · Answer 2 · 2015-06-11

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9.5 years ago

thackl ★ 3.0k

Ideally, if you also have some Illumina data, go for hybrid correction (What tools you use or know for PacBio Long Read error correction?) and assembly with SPAdes (genome <100Mbp)

ADD COMMENT • link updated 23 months ago by Ram 44k • written 9.5 years ago by thackl ★ 3.0k

Ram · Answer 3 · 2015-06-10

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9.5 years ago

h.mon 35k

If you are assembling a small genome, and if your PacBio reads are corrected reads, then SPAdes or MIRA should do a good job.

ADD COMMENT • link updated 23 months ago by Ram 44k • written 9.5 years ago by h.mon 35k

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I don't know if my long reads are corrected. I had a bunch of *.bax.h5 file from which I extracted the .fastq file. Is there way to know if the reads are corrected?

ADD REPLY • link 9.5 years ago by mhasa006 ▴ 70

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I don't think your reads are corrected, since usually error-correction methods produce fastq files

ADD REPLY • link updated 24 months ago by Ram 44k • written 9.4 years ago by Rohit ★ 1.5k