inst/vignettes/CRMAv2,Mapping50K_Hind240.R
In HenrikBengtsson/aroma.affymetrix: Analysis of Large Affymetrix Microarray Data Sets
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
if (interactive()) savehistory()
library("aroma.affymetrix")
# Avoid being masked by affy::plotDensity()
plotDensity <- aroma.light::plotDensity
# Use a nicer palette of colors
colors <- RColorBrewer::brewer.pal(12, "Paired")
palette(colors)
# Default width of plots
width <- 7
devNew2 <- function(...) {
imgFormat <- c("x11", "png")[2]
if (imgFormat == "x11") {
devNew("x11", width=width, height=height, label=fig)
} else {
# Rescale for PNG
c <- 640/7
width <- c*width
height <- c*height
figPath <- "figures"
mkdirs(figPath)
filename <- sprintf("%s.png", fig)
pathname <- filePath(figPath, filename)
devNew("png", file=pathname, width=width, height=height, label=fig)
}
}
# Setup the Verbose object
verbose <- Arguments$getVerbose(-10, timestamp=TRUE)
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup of raw data set
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
if (!exists("cdf")) {
cdf <- AffymetrixCdfFile$byChipType("Mapping50K_Hind240")
print(cdf)
gi <- getGenomeInformation(cdf)
print(gi)
si <- getSnpInformation(cdf)
print(si)
acs <- AromaCellSequenceFile$byChipType(getChipType(cdf, fullname=FALSE))
print(acs)
}
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup of raw data set
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
csR <- AffymetrixCelSet$byName("HapMap,CEU,testSet", cdf=cdf)
print(getFullNames(csR))
## [1] "NA06985_Hind_B5_3005533" "NA06991_Hind_B6_3005533"
## [3] "NA06993_Hind_B4_4000092" "NA06994_Hind_A7_3005533"
## [5] "NA07000_Hind_A8_3005533" "NA07019_Hind_A12_4000092"
## [7] "NA07022_Hind_A10_4000092" "NA07029_Hind_A9_4000092"
## [9] "NA07034_Hind_B1_4000092" "NA07048_Hind_B3_4000092"
# The CEL files downloaded from HapMap has file names such as
# NA07000_Hind_A8_3005533.CEL. In order for aroma.affymetrix to identify
# 'NA07000' as the sample name, and 'A8' and '3005533' as tags (ignore
# the 'Hind' part), we will utilize so called fullname translators that
# translates the full name to a comma-separated fullname, e.g.
# 'NA07000_Hind_A8_3005533' to 'NA07000,A8,3005533'.
setFullNamesTranslator(csR, function(names, ...) {
# Turn into comma-separated tags
names <- gsub("_", ",", names)
# Drop any Hind/Xba tags
names <- gsub(",(Hind|Xba)", "", names)
names
})
print(getFullNames(csR))
## [1] "NA06985,B5,3005533" "NA06991,B6,3005533"
## [3] "NA06993,B4,4000092" "NA06994,A7,3005533"
## [5] "NA07000,A8,3005533" "NA07019,A12,4000092"
## [7] "NA07022,A10,4000092" "NA07029,A9,4000092"
## [9] "NA07034,B1,4000092" "NA07048,B3,4000092"
print(csR)
## AffymetrixCelSet:
## Name: HapMap
## Tags: CEU,testSet
## Path: rawData/HapMap,CEU,testSet/Mapping50K_Hind240
## Platform: Affymetrix
## Chip type: Mapping50K_Hind240
## Number of arrays: 10
## Names: NA06985, NA06991, ..., NA07048
## Time period: 2004-01-14 14:02:08 -- 2004-02-13 11:51:01
## Total file size: 244.78MB
## RAM: 0.01MB
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Brief about different types of probes
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# On Affymetrix arrays, there are different types of probes (cells).
# The most well known are perfect-match (PM) and mismatch (MM) probes.
# In addition to these, there are also QC probes, e.g. so called
# landing-light probes and chequered-flag probes etc.
# One can query the CDF for the indices of the cells for each type.
# If one ask for "all", then all cells on the array are returned.
types <- c("all", "pmmm", "pm", "mm")
cells <- lapply(types, FUN=function(type) identifyCells(cdf, types=type))
names(cells) <- types
str(cells)
## $ all : int [1:2560000] 1 2 3 4 5 6 7 8 9 10 ...
## $ pmmm: int [1:2291560] 1606 1607 1609 1610 1611 1613 1614 1615
## $ pm : int [1:1145780] 1606 1607 1609 1610 1611 1613 1614 1615
## $ mm : int [1:1145780] 3206 3207 3209 3210 3211 3213 3214 3215
# As we will see next, one can specify these types also when plotting
# the empirical densities and when doing quantile normalization.
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Raw probe-signal densities
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# The plotDensity() method for an AffymetrixCelSet estimates and draws
# smooth empirical density functions for each array in set. It is
# possible to stratify by probe type (see above) by setting the 'types'
# argument. For instance, types="all" uses all probes on the chip,
# types="pmmm" uses all PM & MM probes, types="pm" only the PM probes etc.
# Internally, the stats::density() function is used.
height <- 0.618*width
cols <- seq_along(types)
fig <- "plotDensity,raw"
if (!devIsOpen(fig) && FALSE) {
devNew2(width=width, height=height, label=fig)
for (kk in seq_along(types)) {
plotDensity(csR, types=types[kk], col=cols[kk], subset=NULL,
lwd=2, ylim=c(0,0.45), add=(kk > 1))
}
legend("topleft", col=cols, lwd=4, types)
title("Raw probe signals")
devDone()
}
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Rank-based quantile normalization
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# The QuantileNormalization class provide methods for doing rank-based quantile normalization of probe signals. By specifying argument 'typesToUpdates' one can specify what type of probes should be normalized (and used in the model fitting). All other probe signals are left unchanged. The default is typesToUpdates="all", but any of "pmmm", "pm" and "mm" can also be used. We will here show the how they produce different results.
for (type in types) {
verbose && enter(verbose, "Rank-based quantile normalization on ",
type, " probes")
verbose && cat(verbose, "typesToUpdate: ", type)
qn <- QuantileNormalization(csR, typesToUpdate=type, tags=c("*", type))
print(qn)
csN <- process(qn, verbose=verbose)
fig <- sprintf("plotDensity,QN,%s", type)
if (!devIsOpen(fig)) {
devNew2(width=width, height=height, label=fig)
# Plot the type normalized by last.
kks <- match(c(setdiff(types, type), type), types)
for (kk in kks) {
plotDensity(csN, types=types[kk], subset=NULL,
col=cols[kk], lwd=2, ylim=c(0,0.45), add=(kk != kks[1]))
}
legend("topleft", col=cols, lwd=4, types)
title(sprintf("QuantileNormalization(..., typesToUpdate=\"%s\")", type))
devDone()
}
verbose && exit(verbose)
}
# TO DO: identifyCells(cdf, types="qc") returns an empty vector.
HenrikBengtsson/aroma.affymetrix documentation built on Feb. 20, 2024, 9:07 p.m.
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# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
if (interactive()) savehistory()
library("aroma.affymetrix")
# Avoid being masked by affy::plotDensity()
plotDensity <- aroma.light::plotDensity
# Use a nicer palette of colors
colors <- RColorBrewer::brewer.pal(12, "Paired")
palette(colors)
# Default width of plots
width <- 7
devNew2 <- function(...) {
imgFormat <- c("x11", "png")[2]
if (imgFormat == "x11") {
devNew("x11", width=width, height=height, label=fig)
} else {
# Rescale for PNG
c <- 640/7
width <- c*width
height <- c*height
figPath <- "figures"
mkdirs(figPath)
filename <- sprintf("%s.png", fig)
pathname <- filePath(figPath, filename)
devNew("png", file=pathname, width=width, height=height, label=fig)
}
}
# Setup the Verbose object
verbose <- Arguments$getVerbose(-10, timestamp=TRUE)
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup of raw data set
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
if (!exists("cdf")) {
cdf <- AffymetrixCdfFile$byChipType("Mapping50K_Hind240")
print(cdf)
gi <- getGenomeInformation(cdf)
print(gi)
si <- getSnpInformation(cdf)
print(si)
acs <- AromaCellSequenceFile$byChipType(getChipType(cdf, fullname=FALSE))
print(acs)
}
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Setup of raw data set
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
csR <- AffymetrixCelSet$byName("HapMap,CEU,testSet", cdf=cdf)
print(getFullNames(csR))
## [1] "NA06985_Hind_B5_3005533" "NA06991_Hind_B6_3005533"
## [3] "NA06993_Hind_B4_4000092" "NA06994_Hind_A7_3005533"
## [5] "NA07000_Hind_A8_3005533" "NA07019_Hind_A12_4000092"
## [7] "NA07022_Hind_A10_4000092" "NA07029_Hind_A9_4000092"
## [9] "NA07034_Hind_B1_4000092" "NA07048_Hind_B3_4000092"
# The CEL files downloaded from HapMap has file names such as
# NA07000_Hind_A8_3005533.CEL. In order for aroma.affymetrix to identify
# 'NA07000' as the sample name, and 'A8' and '3005533' as tags (ignore
# the 'Hind' part), we will utilize so called fullname translators that
# translates the full name to a comma-separated fullname, e.g.
# 'NA07000_Hind_A8_3005533' to 'NA07000,A8,3005533'.
setFullNamesTranslator(csR, function(names, ...) {
# Turn into comma-separated tags
names <- gsub("_", ",", names)
# Drop any Hind/Xba tags
names <- gsub(",(Hind|Xba)", "", names)
names
})
print(getFullNames(csR))
## [1] "NA06985,B5,3005533" "NA06991,B6,3005533"
## [3] "NA06993,B4,4000092" "NA06994,A7,3005533"
## [5] "NA07000,A8,3005533" "NA07019,A12,4000092"
## [7] "NA07022,A10,4000092" "NA07029,A9,4000092"
## [9] "NA07034,B1,4000092" "NA07048,B3,4000092"
print(csR)
## AffymetrixCelSet:
## Name: HapMap
## Tags: CEU,testSet
## Path: rawData/HapMap,CEU,testSet/Mapping50K_Hind240
## Platform: Affymetrix
## Chip type: Mapping50K_Hind240
## Number of arrays: 10
## Names: NA06985, NA06991, ..., NA07048
## Time period: 2004-01-14 14:02:08 -- 2004-02-13 11:51:01
## Total file size: 244.78MB
## RAM: 0.01MB
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Brief about different types of probes
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# On Affymetrix arrays, there are different types of probes (cells).
# The most well known are perfect-match (PM) and mismatch (MM) probes.
# In addition to these, there are also QC probes, e.g. so called
# landing-light probes and chequered-flag probes etc.
# One can query the CDF for the indices of the cells for each type.
# If one ask for "all", then all cells on the array are returned.
types <- c("all", "pmmm", "pm", "mm")
cells <- lapply(types, FUN=function(type) identifyCells(cdf, types=type))
names(cells) <- types
str(cells)
## $ all : int [1:2560000] 1 2 3 4 5 6 7 8 9 10 ...
## $ pmmm: int [1:2291560] 1606 1607 1609 1610 1611 1613 1614 1615
## $ pm : int [1:1145780] 1606 1607 1609 1610 1611 1613 1614 1615
## $ mm : int [1:1145780] 3206 3207 3209 3210 3211 3213 3214 3215
# As we will see next, one can specify these types also when plotting
# the empirical densities and when doing quantile normalization.
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Raw probe-signal densities
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# The plotDensity() method for an AffymetrixCelSet estimates and draws
# smooth empirical density functions for each array in set. It is
# possible to stratify by probe type (see above) by setting the 'types'
# argument. For instance, types="all" uses all probes on the chip,
# types="pmmm" uses all PM & MM probes, types="pm" only the PM probes etc.
# Internally, the stats::density() function is used.
height <- 0.618*width
cols <- seq_along(types)
fig <- "plotDensity,raw"
if (!devIsOpen(fig) && FALSE) {
devNew2(width=width, height=height, label=fig)
for (kk in seq_along(types)) {
plotDensity(csR, types=types[kk], col=cols[kk], subset=NULL,
lwd=2, ylim=c(0,0.45), add=(kk > 1))
}
legend("topleft", col=cols, lwd=4, types)
title("Raw probe signals")
devDone()
}
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# Rank-based quantile normalization
# - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - - -
# The QuantileNormalization class provide methods for doing rank-based quantile normalization of probe signals. By specifying argument 'typesToUpdates' one can specify what type of probes should be normalized (and used in the model fitting). All other probe signals are left unchanged. The default is typesToUpdates="all", but any of "pmmm", "pm" and "mm" can also be used. We will here show the how they produce different results.
for (type in types) {
verbose && enter(verbose, "Rank-based quantile normalization on ",
type, " probes")
verbose && cat(verbose, "typesToUpdate: ", type)
qn <- QuantileNormalization(csR, typesToUpdate=type, tags=c("*", type))
print(qn)
csN <- process(qn, verbose=verbose)
fig <- sprintf("plotDensity,QN,%s", type)
if (!devIsOpen(fig)) {
devNew2(width=width, height=height, label=fig)
# Plot the type normalized by last.
kks <- match(c(setdiff(types, type), type), types)
for (kk in kks) {
plotDensity(csN, types=types[kk], subset=NULL,
col=cols[kk], lwd=2, ylim=c(0,0.45), add=(kk != kks[1]))
}
legend("topleft", col=cols, lwd=4, types)
title(sprintf("QuantileNormalization(..., typesToUpdate=\"%s\")", type))
devDone()
}
verbose && exit(verbose)
}
# TO DO: identifyCells(cdf, types="qc") returns an empty vector.
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Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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