Question

How to assess the quality of metagenomics assembly?

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9.8 years ago

beloved2012 ▴ 20

Hello everyone! I'm a beginner of metagenomics research. Presently we use soapdenovo package to perform metagenomics assembly then choose the optimal Scaffold according to N50 length (the longest one). I'm wondering that how should we assess the quality of metagenomics assembly except according to the N50 length? Thanks very much!

Assembly Metagenomics • 4.9k views

ADD COMMENT • link updated 2.6 years ago by Ram 44k • written 9.8 years ago by beloved2012 ▴ 20

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OK, thanks all of you. I'll try QUAST later.

ADD REPLY • link updated 2.6 years ago by Ram 44k • written 9.8 years ago by beloved2012 ▴ 20

Ram · Answer 1 · 2015-01-28

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9.8 years ago

Brian Bushnell 20k

Quast is, indeed, very useful. However, it is most useful when you have a reference, where it can calculate the number of misassemblies and error rates. For metagenomes, another crucial metric - arguably, the most important metric - is the percentage of reads that map back to the assembly. If only 50% of your reads map to the assembly... it is not very complete. But if 95% of your reads map to the assembly, then even if it is somewhat fragmented, that's probably very good.

ADD COMMENT • link updated 2.6 years ago by Ram 44k • written 9.8 years ago by Brian Bushnell 20k

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It might also help to look at the percentage properly paired reads to detect any chimeras, something that seems especially relevant in a metagenome assembly.

ADD REPLY • link 9.8 years ago by rens.holmer ▴ 20

Ram · Answer 2 · 2015-01-28

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9.8 years ago

marina.v.yurieva ▴ 580

Try quast

It gives you a report with the quality of your assembly.

ADD COMMENT • link updated 2.6 years ago by Ram 44k • written 9.8 years ago by marina.v.yurieva ▴ 580