Back to Multiple platform build/check report for BioC 3.8 |
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This page was generated on 2019-04-13 11:23:39 -0400 (Sat, 13 Apr 2019).
Package 1222/1649 | Hostname | OS / Arch | INSTALL | BUILD | CHECK | BUILD BIN | ||||||
QDNAseq 1.18.0 Daoud Sie
| malbec1 | Linux (Ubuntu 16.04.6 LTS) / x86_64 | OK | OK | WARNINGS | |||||||
tokay1 | Windows Server 2012 R2 Standard / x64 | OK | OK | [ WARNINGS ] | OK | |||||||
merida1 | OS X 10.11.6 El Capitan / x86_64 | OK | OK | WARNINGS | OK |
Package: QDNAseq |
Version: 1.18.0 |
Command: C:\Users\biocbuild\bbs-3.8-bioc\R\bin\R.exe CMD check --force-multiarch --install=check:QDNAseq.install-out.txt --library=C:\Users\biocbuild\bbs-3.8-bioc\R\library --no-vignettes --timings QDNAseq_1.18.0.tar.gz |
StartedAt: 2019-04-13 04:46:13 -0400 (Sat, 13 Apr 2019) |
EndedAt: 2019-04-13 04:51:47 -0400 (Sat, 13 Apr 2019) |
EllapsedTime: 334.4 seconds |
RetCode: 0 |
Status: WARNINGS |
CheckDir: QDNAseq.Rcheck |
Warnings: 2 |
############################################################################## ############################################################################## ### ### Running command: ### ### C:\Users\biocbuild\bbs-3.8-bioc\R\bin\R.exe CMD check --force-multiarch --install=check:QDNAseq.install-out.txt --library=C:\Users\biocbuild\bbs-3.8-bioc\R\library --no-vignettes --timings QDNAseq_1.18.0.tar.gz ### ############################################################################## ############################################################################## * using log directory 'C:/Users/biocbuild/bbs-3.8-bioc/meat/QDNAseq.Rcheck' * using R version 3.5.3 (2019-03-11) * using platform: x86_64-w64-mingw32 (64-bit) * using session charset: ISO8859-1 * using option '--no-vignettes' * checking for file 'QDNAseq/DESCRIPTION' ... OK * this is package 'QDNAseq' version '1.18.0' * checking package namespace information ... OK * checking package dependencies ...Warning: unable to access index for repository https://CRAN.R-project.org/src/contrib: cannot open URL 'https://CRAN.R-project.org/src/contrib/PACKAGES' OK * checking if this is a source package ... OK * checking if there is a namespace ... OK * checking for hidden files and directories ... OK * checking for portable file names ... OK * checking whether package 'QDNAseq' can be installed ... WARNING Found the following significant warnings: Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/applyFilters.Rd:31: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/binReadCounts.Rd:28: file link 'AnnotatedDataFrame' in package 'Biobase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/estimateCorrection.Rd:43: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/getBinAnnotations.Rd:43: file link 'AnnotatedDataFrame' in package 'Biobase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/highlightFilters.Rd:32: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:37: file link 'cghRaw' in package 'CGHbase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:38: file link 'cghSeg' in package 'CGHbase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:39: file link 'cghCall' in package 'CGHbase' does not exist and so has been treated as a topic See 'C:/Users/biocbuild/bbs-3.8-bioc/meat/QDNAseq.Rcheck/00install.out' for details. * checking installed package size ... OK * checking package directory ... OK * checking 'build' directory ... OK * checking DESCRIPTION meta-information ... OK * checking top-level files ... OK * checking for left-over files ... OK * checking index information ... OK * checking package subdirectories ... OK * checking R files for non-ASCII characters ... OK * checking R files for syntax errors ... OK * loading checks for arch 'i386' ** checking whether the package can be loaded ... OK ** checking whether the package can be loaded with stated dependencies ... OK ** checking whether the package can be unloaded cleanly ... OK ** checking whether the namespace can be loaded with stated dependencies ... OK ** checking whether the namespace can be unloaded cleanly ... OK * loading checks for arch 'x64' ** checking whether the package can be loaded ... OK ** checking whether the package can be loaded with stated dependencies ... OK ** checking whether the package can be unloaded cleanly ... OK ** checking whether the namespace can be loaded with stated dependencies ... OK ** checking whether the namespace can be unloaded cleanly ... OK * checking dependencies in R code ... OK * checking S3 generic/method consistency ... OK * checking replacement functions ... OK * checking foreign function calls ... OK * checking R code for possible problems ... OK * checking Rd files ... OK * checking Rd metadata ... OK * checking Rd cross-references ... OK * checking for missing documentation entries ... WARNING Undocumented code objects: 'exportVCF' All user-level objects in a package should have documentation entries. See chapter 'Writing R documentation files' in the 'Writing R Extensions' manual. * checking for code/documentation mismatches ... OK * checking Rd \usage sections ... OK * checking Rd contents ... OK * checking for unstated dependencies in examples ... OK * checking contents of 'data' directory ... OK * checking data for non-ASCII characters ... OK * checking data for ASCII and uncompressed saves ... OK * checking files in 'vignettes' ... OK * checking examples ... ** running examples for arch 'i386' ... OK Examples with CPU or elapsed time > 5s user system elapsed frequencyPlot 17.89 0.06 17.95 callBins 16.54 0.17 16.70 normalizeSegmentedBins 7.80 0.03 7.83 segmentBins 7.19 0.03 7.22 ** running examples for arch 'x64' ... OK Examples with CPU or elapsed time > 5s user system elapsed callBins 15.79 0.07 15.84 frequencyPlot 15.40 0.03 15.44 segmentBins 5.07 0.02 5.08 * checking for unstated dependencies in 'tests' ... OK * checking tests ... ** running tests for arch 'i386' ... Running 'QDNAseq,reproducibility.R' Running 'QDNAseq.R' OK ** running tests for arch 'x64' ... Running 'QDNAseq,reproducibility.R' Running 'QDNAseq.R' OK * checking for unstated dependencies in vignettes ... OK * checking package vignettes in 'inst/doc' ... OK * checking running R code from vignettes ... SKIPPED * checking re-building of vignette outputs ... SKIPPED * checking PDF version of manual ... OK * DONE Status: 2 WARNINGs See 'C:/Users/biocbuild/bbs-3.8-bioc/meat/QDNAseq.Rcheck/00check.log' for details.
QDNAseq.Rcheck/00install.out
############################################################################## ############################################################################## ### ### Running command: ### ### C:\cygwin\bin\curl.exe -O https://malbec1.bioconductor.org/BBS/3.8/bioc/src/contrib/QDNAseq_1.18.0.tar.gz && rm -rf QDNAseq.buildbin-libdir && mkdir QDNAseq.buildbin-libdir && C:\Users\biocbuild\bbs-3.8-bioc\R\bin\R.exe CMD INSTALL --merge-multiarch --build --library=QDNAseq.buildbin-libdir QDNAseq_1.18.0.tar.gz && C:\Users\biocbuild\bbs-3.8-bioc\R\bin\R.exe CMD INSTALL QDNAseq_1.18.0.zip && rm QDNAseq_1.18.0.tar.gz QDNAseq_1.18.0.zip ### ############################################################################## ############################################################################## % Total % Received % Xferd Average Speed Time Time Time Current Dload Upload Total Spent Left Speed 0 0 0 0 0 0 0 0 --:--:-- --:--:-- --:--:-- 0 100 573k 100 573k 0 0 15.4M 0 --:--:-- --:--:-- --:--:-- 17.4M install for i386 * installing *source* package 'QDNAseq' ... ** R ** data ** inst ** byte-compile and prepare package for lazy loading ** help *** installing help indices converting help for package 'QDNAseq' finding HTML links ... done LGG150 html QDNAseq-defunct html QDNAseq-package html QDNAseqCopyNumbers html QDNAseqReadCounts html QDNAseqSignals html addPhenodata html applyFilters html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/applyFilters.Rd:31: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic binReadCounts html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/binReadCounts.Rd:28: file link 'AnnotatedDataFrame' in package 'Biobase' does not exist and so has been treated as a topic callBins html compareToReference html correctBins html createBins html estimateCorrection html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/estimateCorrection.Rd:43: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic exportBins html finding level-2 HTML links ... done frequencyPlot html getBinAnnotations html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/getBinAnnotations.Rd:43: file link 'AnnotatedDataFrame' in package 'Biobase' does not exist and so has been treated as a topic highlightFilters html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/highlightFilters.Rd:32: file link 'madDiff' in package 'matrixStats' does not exist and so has been treated as a topic isobarPlot html makeCgh html Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:37: file link 'cghRaw' in package 'CGHbase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:38: file link 'cghSeg' in package 'CGHbase' does not exist and so has been treated as a topic Rd warning: C:/Users/biocbuild/bbs-3.8-bioc/tmpdir/RtmpYzQsLT/R.INSTALL194826ed6bab/QDNAseq/man/makeCgh.Rd:39: file link 'cghCall' in package 'CGHbase' does not exist and so has been treated as a topic noisePlot html normalizeBins html normalizeSegmentedBins html plot html poolRuns html segmentBins html smoothOutlierBins html ** building package indices ** installing vignettes ** testing if installed package can be loaded In R CMD INSTALL install for x64 * installing *source* package 'QDNAseq' ... ** testing if installed package can be loaded * MD5 sums packaged installation of 'QDNAseq' as QDNAseq_1.18.0.zip * DONE (QDNAseq) In R CMD INSTALL In R CMD INSTALL * installing to library 'C:/Users/biocbuild/bbs-3.8-bioc/R/library' package 'QDNAseq' successfully unpacked and MD5 sums checked In R CMD INSTALL
QDNAseq.Rcheck/tests_i386/QDNAseq.Rout R version 3.5.3 (2019-03-11) -- "Great Truth" Copyright (C) 2019 The R Foundation for Statistical Computing Platform: i386-w64-mingw32/i386 (32-bit) R is free software and comes with ABSOLUTELY NO WARRANTY. You are welcome to redistribute it under certain conditions. Type 'license()' or 'licence()' for distribution details. R is a collaborative project with many contributors. Type 'contributors()' for more information and 'citation()' on how to cite R or R packages in publications. Type 'demo()' for some demos, 'help()' for on-line help, or 'help.start()' for an HTML browser interface to help. Type 'q()' to quit R. > library("QDNAseq") > > # Load data > data(LGG150) > data <- LGG150 > print(data) QDNAseqReadCounts (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: counts protocolData: none phenoData sampleNames: LGG150 varLabels: name reads used.reads expected.variance varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > stopifnot(inherits(data, "QDNAseqReadCounts")) > > # Plot isobars of read counts > isobarPlot(data) Plotting sample LGG150 median read counts > > # Plot copy number profile > plot(data, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > highlightFilters(data, residual=TRUE, blacklist=TRUE) Highlighted 3,375 bins. > > # Filter out "bad" bins > dataF <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > print(dataF) QDNAseqReadCounts (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: counts protocolData: none phenoData sampleNames: LGG150 varLabels: name reads used.reads expected.variance varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataF, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataF, "QDNAseqReadCounts")) > > # Correct read counts as a function of GC content and mappability > dataC <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > print(dataC) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataC, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataC, "QDNAseqCopyNumbers")) > > # Normalize binned read counts to have diploid normal copy number > dataN <- normalizeBins(dataC) Applying median normalization ... > print(dataN) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataN) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataN, "QDNAseqCopyNumbers")) > > # Plot noise > noisePlot(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > > # Segment copy numbers > fit <- segmentBins(dataN) Performing segmentation: Segmenting: LGG150 (1 of 1) ... > print(fit) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber, segmented protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(fit) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(fit, "QDNAseqCopyNumbers")) > > # Call copy-number segments > #fitC <- callBins(fit) > #print(fitC) > #plot(fitC) > > proc.time() user system elapsed 11.46 0.40 11.86 |
QDNAseq.Rcheck/tests_x64/QDNAseq.Rout R version 3.5.3 (2019-03-11) -- "Great Truth" Copyright (C) 2019 The R Foundation for Statistical Computing Platform: x86_64-w64-mingw32/x64 (64-bit) R is free software and comes with ABSOLUTELY NO WARRANTY. You are welcome to redistribute it under certain conditions. Type 'license()' or 'licence()' for distribution details. R is a collaborative project with many contributors. Type 'contributors()' for more information and 'citation()' on how to cite R or R packages in publications. Type 'demo()' for some demos, 'help()' for on-line help, or 'help.start()' for an HTML browser interface to help. Type 'q()' to quit R. > library("QDNAseq") > > # Load data > data(LGG150) > data <- LGG150 > print(data) QDNAseqReadCounts (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: counts protocolData: none phenoData sampleNames: LGG150 varLabels: name reads used.reads expected.variance varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > stopifnot(inherits(data, "QDNAseqReadCounts")) > > # Plot isobars of read counts > isobarPlot(data) Plotting sample LGG150 median read counts > > # Plot copy number profile > plot(data, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > highlightFilters(data, residual=TRUE, blacklist=TRUE) Highlighted 3,375 bins. > > # Filter out "bad" bins > dataF <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > print(dataF) QDNAseqReadCounts (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: counts protocolData: none phenoData sampleNames: LGG150 varLabels: name reads used.reads expected.variance varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataF, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataF, "QDNAseqReadCounts")) > > # Correct read counts as a function of GC content and mappability > dataC <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > print(dataC) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataC, ylim=c(-100, 200)) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataC, "QDNAseqCopyNumbers")) > > # Normalize binned read counts to have diploid normal copy number > dataN <- normalizeBins(dataC) Applying median normalization ... > print(dataN) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(dataN) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(dataN, "QDNAseqCopyNumbers")) > > # Plot noise > noisePlot(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > > # Segment copy numbers > fit <- segmentBins(dataN) Performing segmentation: Segmenting: LGG150 (1 of 1) ... > print(fit) QDNAseqCopyNumbers (storageMode: lockedEnvironment) assayData: 38819 features, 1 samples element names: copynumber, segmented protocolData: none phenoData sampleNames: LGG150 varLabels: name reads ... loess.family (6 total) varMetadata: labelDescription featureData featureNames: 7:1-15000 7:15001-30000 ... 10:135525001-135534747 (38819 total) fvarLabels: chromosome start ... use (9 total) fvarMetadata: labelDescription experimentData: use 'experimentData(object)' Annotation: > plot(fit) Plotting sample LGG150 (1 of 1) ... > stopifnot(inherits(fit, "QDNAseqCopyNumbers")) > > # Call copy-number segments > #fitC <- callBins(fit) > #print(fitC) > #plot(fitC) > > proc.time() user system elapsed 9.67 0.29 11.07 |
QDNAseq.Rcheck/tests_i386/QDNAseq,reproducibility.Rout R version 3.5.3 (2019-03-11) -- "Great Truth" Copyright (C) 2019 The R Foundation for Statistical Computing Platform: i386-w64-mingw32/i386 (32-bit) R is free software and comes with ABSOLUTELY NO WARRANTY. You are welcome to redistribute it under certain conditions. Type 'license()' or 'licence()' for distribution details. R is a collaborative project with many contributors. Type 'contributors()' for more information and 'citation()' on how to cite R or R packages in publications. Type 'demo()' for some demos, 'help()' for on-line help, or 'help.start()' for an HTML browser interface to help. Type 'q()' to quit R. > ###################################################################### > # This scripts asserts that for each processing step of QDNAseq > # the output/results are reproducible (numerically equal). > ###################################################################### > library("QDNAseq") > > # Load data > data(LGG150) > data <- LGG150 > > # Filter out "bad" bins > dataF <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > dataFr <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > stopifnot(all.equal(dataFr, dataF)) > > # Correct read counts as a function of GC content and mappability > dataC <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > dataCr <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > stopifnot(all.equal(dataCr, dataC)) > > # Normalize binned read counts to have diploid normal copy number > dataN <- normalizeBins(dataC) Applying median normalization ... > dataNr <- normalizeBins(dataC) Applying median normalization ... > stopifnot(all.equal(dataNr, dataN)) > > proc.time() user system elapsed 5.23 0.26 5.50 |
QDNAseq.Rcheck/tests_x64/QDNAseq,reproducibility.Rout R version 3.5.3 (2019-03-11) -- "Great Truth" Copyright (C) 2019 The R Foundation for Statistical Computing Platform: x86_64-w64-mingw32/x64 (64-bit) R is free software and comes with ABSOLUTELY NO WARRANTY. You are welcome to redistribute it under certain conditions. Type 'license()' or 'licence()' for distribution details. R is a collaborative project with many contributors. Type 'contributors()' for more information and 'citation()' on how to cite R or R packages in publications. Type 'demo()' for some demos, 'help()' for on-line help, or 'help.start()' for an HTML browser interface to help. Type 'q()' to quit R. > ###################################################################### > # This scripts asserts that for each processing step of QDNAseq > # the output/results are reproducible (numerically equal). > ###################################################################### > library("QDNAseq") > > # Load data > data(LGG150) > data <- LGG150 > > # Filter out "bad" bins > dataF <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > dataFr <- applyFilters(data, residual=TRUE, blacklist=TRUE) 38,819 total bins 38,819 of which in selected chromosomes 36,722 of which with reference sequence 33,347 final bins > stopifnot(all.equal(dataFr, dataF)) > > # Correct read counts as a function of GC content and mappability > dataC <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > dataCr <- correctBins(dataF) Calculating correction for GC content and mappability Calculating fit for sample LGG150 (1 of 1) ... Done. > stopifnot(all.equal(dataCr, dataC)) > > # Normalize binned read counts to have diploid normal copy number > dataN <- normalizeBins(dataC) Applying median normalization ... > dataNr <- normalizeBins(dataC) Applying median normalization ... > stopifnot(all.equal(dataNr, dataN)) > > proc.time() user system elapsed 6.20 0.26 6.45 |
QDNAseq.Rcheck/examples_i386/QDNAseq-Ex.timings
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QDNAseq.Rcheck/examples_x64/QDNAseq-Ex.timings
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