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  • Unclassified 16SrRNA using green gene taxonomy

    Hello Fellow NGS users,
    I recently sequenced my micro biome (Five body sites) using the Illumina 16SrRNA V4 metagenomics platform. The paired reads were analyzed on base space with sample information showing 100% quality filtering. From the classification statistics, one of the samples had over 50% as unclassified at Kingdom level, phylum, class, order, family, genus and species levels. What could be responsible for this and is there a way of extracting the sequence reads that were reported as unclassified.

  • #2
    Have you looked at the distribution of read lengths in the badly behaved sample. I was having this issue a while back and found that many more reads in poor samples were the wrong length. If I'm expecting a 240bp PCR product, then getting rid of any read which is more than 5bp away from 240bp massively reduces the number of unclassified reads. I suspect that it is some kind of PCR artefact, caused by a poor initial DNA sample.
    You could play around with read lengths, seeing what kind of filtering works best for you.

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    • #3
      The basespace applications are just a very basic first pass. I'd suggest your run your sequences through mothur (my preferred software for amplicons) or qiime to really see what's going on.
      Microbial ecologist, running a sequencing core. I have lots of strong opinions on how to survey communities, pretty sure some are even correct.

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