## ----setup, include=FALSE------------------------------------------------
knitr::opts_chunk$set(echo = TRUE)
knitr::opts_knit$set(progress = FALSE)
## ----message=FALSE, warning=FALSE, include=FALSE-------------------------
library(TCGAbiolinks)
library(SummarizedExperiment)
library(dplyr)
library(DT)
## ---- eval = TRUE, echo = FALSE------------------------------------------
datatable(TCGAbiolinks:::getGDCprojects(),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 10),
rownames = FALSE,
caption = "List of projects")
## ---- eval = TRUE, echo = FALSE------------------------------------------
datatable(TCGAbiolinks:::getBarcodeDefinition(),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 10),
rownames = FALSE,
caption = "List sample types")
## ------------------------------------------------------------------------
datatable(readr::read_csv("https://docs.google.com/spreadsheets/d/1f98kFdj9mxVDc1dv4xTZdx8iWgUiDYO-qiFJINvmTZs/export?format=csv&gid=2046985454"),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 40),
rownames = FALSE)
## ------------------------------------------------------------------------
datatable(readr::read_csv("https://docs.google.com/spreadsheets/d/1f98kFdj9mxVDc1dv4xTZdx8iWgUiDYO-qiFJINvmTZs/export?format=csv&gid=1817673686"),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 40),
rownames = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
query <- GDCquery(project = c("TCGA-GBM", "TCGA-LGG"),
data.category = "DNA Methylation",
legacy = FALSE,
platform = c("Illumina Human Methylation 450"),
sample.type = "Recurrent Solid Tumor"
)
datatable(getResults(query),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
query.met <- GDCquery(project = "TCGA-COAD",
data.category = "DNA Methylation",
legacy = FALSE,
platform = c("Illumina Human Methylation 450"))
query.exp <- GDCquery(project = "TCGA-COAD",
data.category = "Transcriptome Profiling",
data.type = "Gene Expression Quantification",
workflow.type = "HTSeq - FPKM-UQ")
# Get all patients that have DNA methylation and gene expression.
common.patients <- intersect(substr(getResults(query.met, cols = "cases"), 1, 12),
substr(getResults(query.exp, cols = "cases"), 1, 12))
# Only seelct the first 5 patients
query.met <- GDCquery(project = "TCGA-COAD",
data.category = "DNA Methylation",
legacy = FALSE,
platform = c("Illumina Human Methylation 450"),
barcode = common.patients[1:5])
query.exp <- GDCquery(project = "TCGA-COAD",
data.category = "Transcriptome Profiling",
data.type = "Gene Expression Quantification",
workflow.type = "HTSeq - FPKM-UQ",
barcode = common.patients[1:5])
datatable(getResults(query.met, cols = c("data_type","cases")),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
datatable(getResults(query.exp, cols = c("data_type","cases")),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
query <- GDCquery(project = c("TCGA-BRCA"),
data.category = "Sequencing Reads",
sample.type = "Primary solid Tumor")
# Only first 100 to make render faster
datatable(getResults(query, rows = 1:100,cols = c("file_name","cases")),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
query <- GDCquery(project = c("TCGA-GBM","TCGA-LGG"),
legacy = TRUE,
data.category = "DNA methylation",
platform = c("Illumina Human Methylation 450", "Illumina Human Methylation 27"))
datatable(getResults(query, rows = 1:100),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message = FALSE, warning = FALSE, eval = FALSE----------------------
#
# query <- GDCquery(project = c("TCGA-LUAD"),
# legacy = TRUE,
# data.type = "Methylation percentage",
# experimental.strategy = "Bisulfite-Seq")
#
# # VCF - controlled data
# query <- GDCquery(project = c("TCGA-LUAD"),
# legacy = TRUE,
# data.type = "Bisulfite sequence alignment",
# experimental.strategy = "Bisulfite-Seq")
#
#
# # WGBS BAM files - controlled data
# query <- GDCquery(project = c("TCGA-LUAD"),
# legacy = TRUE,
# data.type = "Aligned reads",
# data.category = "Raw sequencing data",
# experimental.strategy = "Bisulfite-Seq")
## ----message=FALSE, warning=FALSE----------------------------------------
# Gene expression aligned against hg19.
query.exp.hg19 <- GDCquery(project = "TCGA-GBM",
data.category = "Gene expression",
data.type = "Gene expression quantification",
platform = "Illumina HiSeq",
file.type = "normalized_results",
experimental.strategy = "RNA-Seq",
barcode = c("TCGA-14-0736-02A-01R-2005-01", "TCGA-06-0211-02A-02R-2005-01"),
legacy = TRUE)
datatable(getResults(query.exp.hg19),
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
getManifest(query.exp.hg19,save = FALSE)
## ----message=FALSE, warning=FALSE----------------------------------------
datatable(getResults(TCGAbiolinks:::GDCquery_ATAC_seq())[,c("file_name","file_size")],
filter = 'top',
options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
rownames = FALSE)
## ----message=FALSE, warning=FALSE,eval = FALSE---------------------------
# query <- TCGAbiolinks:::GDCquery_ATAC_seq(file.type = "rds")
# GDCdownload(query,method = "client")
#
# query <- TCGAbiolinks:::GDCquery_ATAC_seq(file.type = "bigWigs")
# GDCdownload(query,method = "client")
#
## ----message=FALSE, warning=FALSE,eval = FALSE---------------------------
# tab <- getSampleFilesSummary("TCGA-ACC")
# datatable(tab,
# filter = 'top',
# options = list(scrollX = TRUE, keys = TRUE, pageLength = 5),
# rownames = FALSE)