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README.md
# <img src="logo_mid.png" align="right" /> # CytoML: Cross-Platform Cytometry Data Sharing. This package is designed to import/export the hierarchical gated cytometry data to and from R (specifically the [openCyto](https://github.com/RGLab/openCyto) framework) using the [`gatingML2.0`](https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4874733/) and [`FCS3.0`](http://isac-net.org/Resources/Standards/FCS3-1.aspx) cytometry data standards. This package makes use of the `GatingSet` R object and data model so that imported data can easily be manipulated and visualized in R using tools like [openCyto](https://github.com/RGLab/openCyto) and [ggCyto](https://github.com/RGLab/ggcyto). ## What problems does CytoML solve? CytoML allows you to: - Import manually gated data into R from [Diva](http://www.bdbiosciences.com/us/instruments/clinical/software/flow-cytometry-acquisition/bd-facsdiva-software/m/333333/overview), [FlowJo](https://www.flowjo.com/) and [Cytobank](https://cytobank.org/). - Combine manual gating strategies with automated gating strategies in R. - Export data gated manually, auto-gated, or gated using a combination of manual and automated strategies from R to [Diva](http://www.bdbiosciences.com/us/instruments/clinical/software/flow-cytometry-acquisition/bd-facsdiva-software/m/333333/overview), [FlowJo](https://www.flowjo.com/) and [Cytobank](https://cytobank.org/). - Share computational flow analyses with users on other platforms. - Perform comparative analyses between computational and manual gating approaches. ### Reporting Bugs or Issues - Use the issue template in github when creating a new issue. - Follow the instructions in the template (do your background reading). - Search and verify that the issue hasn't already been addressed. - Check the Bioconductor support site. - Make sure your flow packages are up to date. - THEN if your issue persists, file a bug report. Otherwise, we may close your issue without responding. ## INSTALLATION CytoML can be installed in several ways: ### For all versions: For all versions, you must have dependencies installed ``` r library(BiocManager) # This should pull all dependencies. BiocManager::install("openCyto") # Then install latest dependencies from github, using devtools. install.packages("devtools") library(devtools) #load it install_github("RGLab/flowWorkspace") install_github("RGLab/openCyto") ``` ### Installing from [BioConductor](https://www.bioconductor.org). - [Current BioConductor Relase](https://doi.org/doi:10.18129/B9.bioc.CytoML) <!-- end list --> ``` r library(BiocManager) #this should pull all dependencies. BiocManager::install("CytoML", version = "devel") ``` - [Current BioConductor Development Version](http://bioconductor.org/packages/devel/bioc/html/CytoML.html) <!-- end list --> ``` r library(BiocManager) #this should pull all dependencies. BiocManager::install("CytoML", version = "devel") ``` ### Installing from GitHub - [Latest GitHub Version](https://github.com/RGLab/CytoML) <!-- end list --> ``` r install.packges("devtools") devtools::install_github("RGLab/CytoML") ``` - [Latest GitHub Release](https://github.com/RGLab/CytoML/releases) <!-- end list --> ``` r install.packges("devtools") devtools::install_github("RGLab/CytoML@*release") ``` ## Reproducible examples from the CytoML paper - A reproducible workflow can be found at the [RGLab site](http://www.rglab.org/CytoML), and was prepared with version 1.7.10 of CytoML, R v3.5.0, and dependencies that can be installed by: <!-- end list --> ``` r # We recomend using R version 3.5.0 devtools::install_github("RGLab/RProtoBufLib@v1.3.7") devtools::install_github("RGLab/cytolib@v1.3.2") devtools::install_github("RGLab/flowCore@v1.47.7") devtools::install_github("RGLab/flowWorkspace@v3.29.7") devtools::install_github("RGLab/openCyto@v1.19.2") devtools::install_github("RGLab/CytoML@v1.7.10") devtools::install_github("RGLab/ggcyto@v1.9.12") ``` ## Examples ### Import data To import data you need the xml workspace and the raw FCS files. #### Import `gatingML` generated from [Cytobank](https://cytobank.org/). ``` r library(CytoML) acsfile <- system.file("extdata/cytobank_experiment.acs", package = "CytoML") ce <- open_cytobank_experiment(acsfile) xmlfile <- ce$gatingML fcsFiles <- list.files(ce$fcsdir, full.names = TRUE) gs <- cytobank_to_gatingset(xmlfile, fcsFiles) ``` #### Import a [Diva](http://www.bdbiosciences.com/us/instruments/clinical/software/flow-cytometry-acquisition/bd-facsdiva-software/m/333333/overview) workspace. ``` r ws <- open_diva_xml(system.file('extdata/diva/PE_2.xml', package = "flowWorkspaceData")) # The path to the FCS files is stored in ws@path. # It can also be passed in to parseWorksapce via the `path` argument. gs <- diva_to_gatingset(ws, name = 2, subset = 1, swap_cols = FALSE) ``` #### Interact with the gated data (`GatingSet`) We need `flowWorkspace` to interact with the imported data. ``` r library(flowWorkspace) ``` We can visualize the gating tree as follows: ``` r #get the first sample gh <- gs[[1]] #plot the hierarchy tree plot(gh) ``` ![](README_files/figure-gfm/unnamed-chunk-4-1.png)<!-- --> For more information see the [flowWorkspace](http://www.github.com/RGLab/flowWorkspace) package. We can print all the cell populations defined in the gating tree. ``` r #show all the cell populations(/nodes) gs_get_pop_paths(gh) ``` ## [1] "root" "/P1" "/P1/P2" "/P1/P2/P3" ## [5] "/P1/P2/P3/P4" "/P1/P2/P3/P4/P5" We can extract the cell population statistics. ``` r #show the population statistics gh_pop_compare_stats(gh) ``` ## openCyto.freq xml.freq openCyto.count xml.count node ## 1: 1.00000000 1.00000000 19090 19090 root ## 2: 0.93609219 0.93776847 17870 17902 P1 ## 3: 0.97991046 0.97994637 17511 17543 P2 ## 4: 0.70327223 0.70307245 12315 12334 P3 ## 5: 0.09378806 0.09404897 1155 1160 P4 ## 6: 0.95151515 0.94827586 1099 1100 P5 The `openCyto.count` column shows the cell counts computed via the import. The `xml.count` column shows the cell counts computed by FlowJo (note not all platforms report cell counts in the workspace). It is normal for these to differ by a few cells due to numerical differences in the implementation of data transformations. CytoML and openCyto are *reproducing* the data analysis from the raw data based on the information in the workspace. We can plot all the gates defined in the workspace. ``` r #plot the gates plotGate(gh) ``` ![](README_files/figure-gfm/unnamed-chunk-7-1.png)<!-- --> #### Access information about cells in a specific population. Because CytoML and flowWorkspace reproduce the entire analysis in a workspace in R, we have access to information about which cells are part of which cell popualtions. flowWorkspace has convenience methods to extract the cells from specific cell populations: ``` r gh_pop_get_data(gh,"P3") ``` ## flowFrame object '9a1897d7-ebc9-4077-aa34-6d9e1367fa67' ## with 12315 cells and 15 observables: ## name desc range minRange maxRange ## $P1 Time <NA> 262144 0.0000000 262144.0 ## $P2 FSC-A <NA> 262144 0.0000000 262144.0 ## $P3 FSC-H <NA> 262144 0.0000000 262144.0 ## $P4 FSC-W <NA> 262144 0.0000000 262144.0 ## $P5 SSC-A <NA> 262144 0.0000000 262144.0 ## $P6 SSC-H <NA> 262144 0.0000000 262144.0 ## $P7 SSC-W <NA> 262144 0.0000000 262144.0 ## $P8 FITC-A <NA> 262144 0.1516347 4.5 ## $P9 PE-A CD3 262144 0.2953046 4.5 ## $P10 PerCP-Cy5-5-A <NA> 262144 0.4697134 4.5 ## $P11 PE-Cy7-A <NA> 262144 0.5638024 4.5 ## $P12 APC-A bob 262144 0.7838544 4.5 ## $P13 APC-Cy7-A Viab 262144 0.6886181 4.5 ## $P14 Bd Horizon V450-A CD44 262144 0.6413334 4.5 ## $P15 Pacific Orange-A CD8 262144 0.3376040 4.5 ## 231 keywords are stored in the 'description' slot This returns a `flowFrame` with the cells in gate P3 (70% of the cells according to the plot). The matrix of expression can be extracted from a `flowFrame` using the `exprs()` method from the `flowCore` package: ``` r library(flowCore) e <- exprs(gh_pop_get_data(gh,"P3")) class(e) ``` ## [1] "matrix" ``` r dim(e) ``` ## [1] 12315 15 ``` r colnames(e) ``` ## [1] "Time" "FSC-A" "FSC-H" ## [4] "FSC-W" "SSC-A" "SSC-H" ## [7] "SSC-W" "FITC-A" "PE-A" ## [10] "PerCP-Cy5-5-A" "PE-Cy7-A" "APC-A" ## [13] "APC-Cy7-A" "Bd Horizon V450-A" "Pacific Orange-A" ``` r #compute the MFI of the fluorescence channels. colMeans(e[,8:15]) ``` ## FITC-A PE-A PerCP-Cy5-5-A PE-Cy7-A ## 0.8305630 1.3162132 0.7743459 0.8017827 ## APC-A APC-Cy7-A Bd Horizon V450-A Pacific Orange-A ## 1.0482663 1.1636818 2.2960554 1.3684453 ### Export gated data to other platforms. In order to export gated data, it must be in `GatingSet` format. #### Export a `GatingSet` from R to [Cytobank](https://cytobank.org/) or [FlowJo](https://www.flowjo.com/) Load something to export. ``` r dataDir <- system.file("extdata",package="flowWorkspaceData") gs <- load_gs(list.files(dataDir, pattern = "gs_manual",full = TRUE)) ``` ## loading R object... ## loading tree object... ## Done ##### Export to Cytobank ``` r #Cytobank outFile <- tempfile(fileext = ".xml") gatingset_to_cytobank(gs, outFile) ``` ## Warning in gatingset_to_cytobank(gs, outFile): With ## 'cytobank.default.scale' set to 'TRUE', data and gates will be re- ## transformed with cytobank's default scaling settings, which may affect how ## gates look like. ## [1] "/tmp/RtmpV1ZasG/file4b9f7e4e25c1.xml" ##### Export to FlowJo ``` r #flowJo outFile <- tempfile(fileext = ".wsp") gatingset_to_flowjo(gs, outFile) ``` ## [1] "/tmp/RtmpV1ZasG/file4b9f18da0869.wsp" ## Next Steps See the [flowWorskspace](http://www.github.com/RGLab/flowWorkspace) and [openCyto](<http://www.github.com/RGLab/openCyto>) packages to learn more about what can be done with `GatingSet` objects. ## Code of conduct Please note that this project is released with a [Contributor Code of Conduct](CODE_OF_CONDUCT.md). By participating in this project you agree to abide by its terms.