... | @@ -114,9 +114,9 @@ Start by getting the full processed dada data: |
... | @@ -114,9 +114,9 @@ Start by getting the full processed dada data: |
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$ cp /bioinf/home/tfrancis/marmic_NGS2020/16S_amplicons/demultiplexed/seqtab_final.rds .
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$ cp /bioinf/home/tfrancis/marmic_NGS2020/16S_amplicons/demultiplexed/seqtab_final.rds .
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$ cp /bioinf/home/tfrancis/marmic_NGS2020/16S_amplicons/demultiplexed/taxa_final.rds .
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$ cp /bioinf/home/tfrancis/marmic_NGS2020/16S_amplicons/demultiplexed/taxa_final.rds .
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Then start R (any R, doesn't matter this time)
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Then R
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$ R
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$ /home/tfrancis/R-3.6.2/bin/R
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load the data:
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load the data:
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... | @@ -159,13 +159,13 @@ then do the plotting :) |
... | @@ -159,13 +159,13 @@ then do the plotting :) |
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theme(axis.text.x=element_text(angle=45, hjust=1))
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theme(axis.text.x=element_text(angle=45, hjust=1))
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}
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}
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plotTaxon(seqtab.nochim, taxa, "Bacteroidetes", 0.01, "Genus")
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# Ignore this bit about making pdfs
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So the bit above creates the function called `plotTaxon()`, which we can then use to generate the plots. We're going to create a pdf of the plot by first opening a pdf file with the `pdf()` command, then run the `plotTaxon()` function, then switch off the plotting device.
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So the bit above creates the function called `plotTaxon()`, which we can then use to generate the plots. We're going to create a pdf of the plot by first opening a pdf file with the `pdf()` command, then run the `plotTaxon()` function, then switch off the plotting device.
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> pdf("Marmic-amplicon-plot.pdf")
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> pdf("Marmic-amplicon-plot.pdf")
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>
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> plotTaxon(seqtab.nochim, taxa, "Bacteroidetes", 0.01, "Genus")
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> dev.off()
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> dev.off()
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Once you have your plot, you can open a new terminal (don't quit R because we will want to create different plots for different taxa - just change the file name for the pdf) and run:
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Once you have your plot, you can open a new terminal (don't quit R because we will want to create different plots for different taxa - just change the file name for the pdf) and run:
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