Paul J. McMurdie and Susan Holmes
If you find phyloseq and/or its tutorials useful, please acknowledge and cite phyloseq in your publications:
phyloseq: An R package for reproducible interactive analysis and graphics of microbiome census data (2013) PLoS ONE 8(4):e61217 http://dx.plos.org/10.1371/journal.pone.0061217
The phyloseq project also has a number of supporting online resources, most of which can by found at the phyloseq home page, or from the phyloseq stable release page on Bioconductor.
To post feature requests or ask for help, try the phyloseq Issue Tracker.
In this example I use the publicly available data from a study on colorectal cancer:
Genomic analysis identifies association of Fusobacterium with colorectal carcinoma. Kostic, A. D., Gevers, D., Pedamallu, C. S., Michaud, M., Duke, F., Earl, A. M., et al. (2012). Genome research, 22(2), 292-298.
As a side-note, this work was published ahead of print in Genome Research alongside a highly-related article from a separate group of researchers (long-live reproducible observations!): Fusobacterium nucleatum infection is prevalent in human colorectal carcinoma. In case you are interested. For the purposes of example, however, we will stick to the data from the former study, with data available at the microbio.me/qiime server.
Data source, from methods section in article:
The 16S gene data set consists of 454 FLX Titanium sequences spanning the V3 to V5 variable regions obtained for 190 samples (95 pairs). Detailed protocols used for 16S amplification and se- quencing are available on the HMP Data Analysis and Coordination Center website (http://www.hmpdacc.org/tools_protocols/tools_ protocols.php).
Study ID: 1457
Project Name: Kostic_colorectal_cancer_fusobacterium
Study Abstract:
The tumor microenvironment of colorectal carcinoma is a complex community of genomically altered cancer cells, nonneoplastic cells, and a diverse collection of microorganisms. Each of these components may contribute to carcino genesis; however, the role of the microbiota is the least well understood. We have characterized the composition of the microbiota in colorectal carcinoma using whole genome sequences from nine tumor/normal pairs. Fusobacterium sequences were enriched in carcinomas, confirmed by quantitative PCR and 16S rDNA sequence analysis of 95 carcinoma/normal DNA pairs, while the Bacteroidetes and Firmicutes phyla were depleted in tumors. Fusobacteria were also visualized within colorectal tumors using FISH. These findings reveal alterations in the colorectal cancer microbiota; however, the precise role of Fusobacteria in colorectal carcinoma pathogenesis requires further investigation.
Start by loading phyloseq.
library("phyloseq"); packageVersion("phyloseq")
## [1] '1.34.0'
Defined file path, and import the published OTU count data into R.
filepath = system.file("extdata", "study_1457_split_library_seqs_and_mapping.zip", package="phyloseq")
kostic = microbio_me_qiime(filepath)
## Found biom-format file, now parsing it...
## Done parsing biom...
## Importing Sample Metdadata from mapping file...
## Merging the imported objects...
## Successfully merged, phyloseq-class created.
## Returning...
Here I had to use a relative file path so that this example works on all systems that have phyloseq installed. In practice, your file path will look like this (if you’ve downloaded the data ahead of time):
filepath = "~/Downloads/study_1457_split_library_seqs_and_mapping.zip"
kostic = microbio_me_qiime(filepath)
Or like this (if you’re accessing data directly from the microbio.me/qiime server directly):
kostic = microbio_me_qiime(1457)
In this example I’m using the major sample covariate, DIAGNOSIS
, as the study design factor. The focus of this study was to compare the microbiomes of pairs of healthy and cancerous tissues, so this makes sense. Your study could have a more complex or nested design, and you should think carefully about the study design formula, because this is critical to the test results and their meaning. You might even need to define a new factor if none of the variables in your current table appropriately represent your study’s design. See the DESeq2 home page for more details.
Here is the summary of the data variable kostic
that we are about to use, as well as the first few entries of the DIAGNOSIS
factor.
kostic
## phyloseq-class experiment-level object
## otu_table() OTU Table: [ 2505 taxa and 190 samples ]
## sample_data() Sample Data: [ 190 samples by 71 sample variables ]
## tax_table() Taxonomy Table: [ 2505 taxa by 7 taxonomic ranks ]
head(sample_data(kostic)$DIAGNOSIS, 10)
## [1] "Healthy" "Tumor" "Tumor" "Healthy" "Healthy" "Healthy" "Tumor"
## [8] "Healthy" "Healthy" "Healthy"
First load DESeq2.
library("DESeq2"); packageVersion("DESeq2")
## [1] '1.30.0'
The following two lines actually do all the complicated DESeq2 work. The function phyloseq_to_deseq2
converts your phyloseq-format microbiome data into a DESeqDataSet
with dispersions estimated, using the experimental design formula, also shown (the ~DIAGNOSIS
term). The DESeq
function does the rest of the testing, in this case with default testing framework, but you can actually use alternatives.
First remove the 5 samples that had no DIAGNOSIS
attribute assigned.
These introduce a spurious third design class
that is actually a rare artifact in the dataset.
Also remove samples with less than 500
reads (counts).
Note that this kind of data cleanup
is useful, necessary, and should be well-documented
because it can also be dangerous to alter or omit data
without clear documentation.
In this case I actually explored the data first,
and am omitting some of the details
(and explanatory plots) here for clarity.
kostic <- subset_samples(kostic, DIAGNOSIS != "None")
kostic <- prune_samples(sample_sums(kostic) > 500, kostic)
kostic
## phyloseq-class experiment-level object
## otu_table() OTU Table: [ 2505 taxa and 177 samples ]
## sample_data() Sample Data: [ 177 samples by 71 sample variables ]
## tax_table() Taxonomy Table: [ 2505 taxa by 7 taxonomic ranks ]
diagdds = phyloseq_to_deseq2(kostic, ~ DIAGNOSIS)
# calculate geometric means prior to estimate size factors
gm_mean = function(x, na.rm=TRUE){
exp(sum(log(x[x > 0]), na.rm=na.rm) / length(x))
}
geoMeans = apply(counts(diagdds), 1, gm_mean)
diagdds = estimateSizeFactors(diagdds, geoMeans = geoMeans)
diagdds = DESeq(diagdds, fitType="local")
Note: The default multiple-inference correction is Benjamini-Hochberg, and occurs within the DESeq
function.
The following results
function call creates a table of the results of the tests. Very fast. The hard work was already stored with the rest of the DESeq2-related data in our latest version of the diagdds
object (see above). I then order by the adjusted p-value, removing the entries with an NA
value. The rest of this example is just formatting the results table with taxonomic information for nice(ish) display in the HTML output.
res = results(diagdds)
res = res[order(res$padj, na.last=NA), ]
alpha = 0.01
sigtab = res[(res$padj < alpha), ]
sigtab = cbind(as(sigtab, "data.frame"), as(tax_table(kostic)[rownames(sigtab), ], "matrix"))
head(sigtab)
## baseMean log2FoldChange lfcSE stat pvalue padj
## 64396 181.564648 2.195547 0.4282121 5.127241 2.940185e-07 0.0007238735
## 72853 28.633097 -1.604873 0.3310712 -4.847515 1.250173e-06 0.0015389626
## 374052 75.002469 2.523486 0.5411855 4.662885 3.118073e-06 0.0025588983
## 307981 3.258919 2.153038 0.4832019 4.455773 8.359162e-06 0.0051450643
## 180285 168.356513 -1.204357 0.2782362 -4.328542 1.501000e-05 0.0073909224
## Kingdom Phylum Class Order
## 64396 Bacteria Fusobacteria Fusobacteria (class) Fusobacteriales
## 72853 Bacteria Firmicutes Clostridia Clostridiales
## 374052 Bacteria Fusobacteria Fusobacteria (class) Fusobacteriales
## 307981 Bacteria Proteobacteria Gammaproteobacteria Enterobacteriales
## 180285 Bacteria Firmicutes Clostridia Clostridiales
## Family Genus Species
## 64396 Fusobacteriaceae Fusobacterium <NA>
## 72853 Ruminococcaceae Faecalibacterium <NA>
## 374052 Fusobacteriaceae Fusobacterium <NA>
## 307981 Enterobacteriaceae Klebsiella <NA>
## 180285 Ruminococcaceae Faecalibacterium <NA>
Let’s look at just the OTUs that were significantly enriched in the carcinoma tissue. First, cleaning up the table a little for legibility.
posigtab = sigtab[sigtab[, "log2FoldChange"] > 0, ]
posigtab = posigtab[, c("baseMean", "log2FoldChange", "lfcSE", "padj", "Phylum", "Class", "Family", "Genus")]
OTU | baseMean | log2FoldChange | lfcSE | padj | Phylum | Class | Family | Genus |
---|---|---|---|---|---|---|---|---|
64396 | 181.564648 | 2.195547 | 0.4282121 | 0.0007238735 | Fusobacteria | Fusobacteria (class) | Fusobacteriaceae | Fusobacterium |
374052 | 75.002469 | 2.523486 | 0.5411855 | 0.0025588983 | Fusobacteria | Fusobacteria (class) | Fusobacteriaceae | Fusobacterium |
307981 | 3.258919 | 2.153038 | 0.4832019 | 0.0051450643 | Proteobacteria | Gammaproteobacteria | Enterobacteriaceae | Klebsiella |
As expected from the original study abstract and title, a Fusobacterium OTU was among the most-significantly differentially abundant between the cancerous and healthy samples.
Here is a bar plot showing the log2-fold-change, showing Genus and Phylum. Uses some ggplot2 commands.
library("ggplot2")
theme_set(theme_bw())
sigtabgen = subset(sigtab, !is.na(Genus))
# Phylum order
x = tapply(sigtabgen$log2FoldChange, sigtabgen$Phylum, function(x) max(x))
x = sort(x, TRUE)
sigtabgen$Phylum = factor(as.character(sigtabgen$Phylum), levels=names(x))
# Genus order
x = tapply(sigtabgen$log2FoldChange, sigtabgen$Genus, function(x) max(x))
x = sort(x, TRUE)
sigtabgen$Genus = factor(as.character(sigtabgen$Genus), levels=names(x))
ggplot(sigtabgen, aes(y=Genus, x=log2FoldChange, color=Phylum)) +
geom_vline(xintercept = 0.0, color = "gray", size = 0.5) +
geom_point(size=6) +
theme(axis.text.x = element_text(angle = -90, hjust = 0, vjust=0.5))