# HG changeset patch
# User fubar
# Date 1420528855 18000
# Node ID 0de9466084233ca499c8579383b6ea8066661595
# Parent 21b218a7429fe0832fa6ad47f75c7dd2422b860d
Uploaded
diff -r 21b218a7429f -r 0de946608423 rgToolFactory.py
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/rgToolFactory.py Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,638 @@
+# rgToolFactory.py
+# see https://bitbucket.org/fubar/galaxytoolfactory/wiki/Home
+#
+# copyright ross lazarus (ross stop lazarus at gmail stop com) May 2012
+#
+# all rights reserved
+# Licensed under the LGPL
+# suggestions for improvement and bug fixes welcome at https://bitbucket.org/fubar/galaxytoolfactory/wiki/Home
+#
+# march 2014
+# added ghostscript and graphicsmagick as dependencies
+# fixed a wierd problem where gs was trying to use the new_files_path from universe (database/tmp) as ./database/tmp
+# errors ensued
+#
+# august 2013
+# found a problem with GS if $TMP or $TEMP missing - now inject /tmp and warn
+#
+# july 2013
+# added ability to combine images and individual log files into html output
+# just make sure there's a log file foo.log and it will be output
+# together with all images named like "foo_*.pdf
+# otherwise old format for html
+#
+# January 2013
+# problem pointed out by Carlos Borroto
+# added escaping for <>$ - thought I did that ages ago...
+#
+# August 11 2012
+# changed to use shell=False and cl as a sequence
+
+# This is a Galaxy tool factory for simple scripts in python, R or whatever ails ye.
+# It also serves as the wrapper for the new tool.
+#
+# you paste and run your script
+# Only works for simple scripts that read one input from the history.
+# Optionally can write one new history dataset,
+# and optionally collect any number of outputs into links on an autogenerated HTML page.
+
+# DO NOT install on a public or important site - please.
+
+# installed generated tools are fine if the script is safe.
+# They just run normally and their user cannot do anything unusually insecure
+# but please, practice safe toolshed.
+# Read the fucking code before you install any tool
+# especially this one
+
+# After you get the script working on some test data, you can
+# optionally generate a toolshed compatible gzip file
+# containing your script safely wrapped as an ordinary Galaxy script in your local toolshed for
+# safe and largely automated installation in a production Galaxy.
+
+# If you opt for an HTML output, you get all the script outputs arranged
+# as a single Html history item - all output files are linked, thumbnails for all the pdfs.
+# Ugly but really inexpensive.
+#
+# Patches appreciated please.
+#
+#
+# long route to June 2012 product
+# Behold the awesome power of Galaxy and the toolshed with the tool factory to bind them
+# derived from an integrated script model
+# called rgBaseScriptWrapper.py
+# Note to the unwary:
+# This tool allows arbitrary scripting on your Galaxy as the Galaxy user
+# There is nothing stopping a malicious user doing whatever they choose
+# Extremely dangerous!!
+# Totally insecure. So, trusted users only
+#
+# preferred model is a developer using their throw away workstation instance - ie a private site.
+# no real risk. The universe_wsgi.ini admin_users string is checked - only admin users are permitted to run this tool.
+#
+
+import sys
+import shutil
+import subprocess
+import os
+import time
+import tempfile
+import optparse
+import tarfile
+import re
+import shutil
+import math
+
+progname = os.path.split(sys.argv[0])[1]
+myversion = 'V001.1 March 2014'
+verbose = False
+debug = False
+toolFactoryURL = 'https://bitbucket.org/fubar/galaxytoolfactory'
+
+def timenow():
+ """return current time as a string
+ """
+ return time.strftime('%d/%m/%Y %H:%M:%S', time.localtime(time.time()))
+
+html_escape_table = {
+ "&": "&",
+ ">": ">",
+ "<": "<",
+ "$": "\$"
+ }
+
+def html_escape(text):
+ """Produce entities within text."""
+ return "".join(html_escape_table.get(c,c) for c in text)
+
+def cmd_exists(cmd):
+ return subprocess.call("type " + cmd, shell=True,
+ stdout=subprocess.PIPE, stderr=subprocess.PIPE) == 0
+
+
+class ScriptRunner:
+ """class is a wrapper for an arbitrary script
+ """
+
+ def __init__(self,opts=None,treatbashSpecial=True):
+ """
+ cleanup inputs, setup some outputs
+
+ """
+ self.useGM = cmd_exists('gm')
+ self.useIM = cmd_exists('convert')
+ self.useGS = cmd_exists('gs')
+ self.temp_warned = False # we want only one warning if $TMP not set
+ self.treatbashSpecial = treatbashSpecial
+ if opts.output_dir: # simplify for the tool tarball
+ os.chdir(opts.output_dir)
+ self.thumbformat = 'png'
+ self.opts = opts
+ self.toolname = re.sub('[^a-zA-Z0-9_]+', '', opts.tool_name) # a sanitizer now does this but..
+ self.toolid = self.toolname
+ self.myname = sys.argv[0] # get our name because we write ourselves out as a tool later
+ self.pyfile = self.myname # crude but efficient - the cruft won't hurt much
+ self.xmlfile = '%s.xml' % self.toolname
+ s = open(self.opts.script_path,'r').readlines()
+ s = [x.rstrip() for x in s] # remove pesky dos line endings if needed
+ self.script = '\n'.join(s)
+ fhandle,self.sfile = tempfile.mkstemp(prefix=self.toolname,suffix=".%s" % (opts.interpreter))
+ tscript = open(self.sfile,'w') # use self.sfile as script source for Popen
+ tscript.write(self.script)
+ tscript.close()
+ self.indentedScript = '\n'.join([' %s' % x for x in s]) # for restructured text in help
+ self.escapedScript = '\n'.join([html_escape(x) for x in s])
+ self.elog = os.path.join(self.opts.output_dir,"%s_error.log" % self.toolname)
+ if opts.output_dir: # may not want these complexities
+ self.tlog = os.path.join(self.opts.output_dir,"%s_runner.log" % self.toolname)
+ art = '%s.%s' % (self.toolname,opts.interpreter)
+ artpath = os.path.join(self.opts.output_dir,art) # need full path
+ artifact = open(artpath,'w') # use self.sfile as script source for Popen
+ artifact.write(self.script)
+ artifact.close()
+ self.cl = []
+ self.html = []
+ a = self.cl.append
+ a(opts.interpreter)
+ if self.treatbashSpecial and opts.interpreter in ['bash','sh']:
+ a(self.sfile)
+ else:
+ a('-') # stdin
+ a(opts.input_tab)
+ a(opts.output_tab)
+ self.outFormats = 'tabular' # TODO make this an option at tool generation time
+ self.inputFormats = 'tabular' # TODO make this an option at tool generation time
+ self.test1Input = '%s_test1_input.xls' % self.toolname
+ self.test1Output = '%s_test1_output.xls' % self.toolname
+ self.test1HTML = '%s_test1_output.html' % self.toolname
+
+ def makeXML(self):
+ """
+ Create a Galaxy xml tool wrapper for the new script as a string to write out
+ fixme - use templating or something less fugly than this example of what we produce
+
+
+ a tabular file
+
+ reverse.py --script_path "$runMe" --interpreter "python"
+ --tool_name "reverse" --input_tab "$input1" --output_tab "$tab_file"
+
+
+
+
+
+
+
+
+
+
+
+**What it Does**
+
+Reverse the columns in a tabular file
+
+
+
+
+
+# reverse order of columns in a tabular file
+import sys
+inp = sys.argv[1]
+outp = sys.argv[2]
+i = open(inp,'r')
+o = open(outp,'w')
+for row in i:
+ rs = row.rstrip().split('\t')
+ rs.reverse()
+ o.write('\t'.join(rs))
+ o.write('\n')
+i.close()
+o.close()
+
+
+
+
+
+
+ """
+ newXML="""
+ %(tooldesc)s
+ %(command)s
+
+ %(inputs)s
+
+
+ %(outputs)s
+
+
+
+ %(script)s
+
+
+ %(tooltests)s
+
+ %(help)s
+
+ """ # needs a dict with toolname, toolid, interpreter, scriptname, command, inputs as a multi line string ready to write, outputs ditto, help ditto
+
+ newCommand="""
+ %(toolname)s.py --script_path "$runMe" --interpreter "%(interpreter)s"
+ --tool_name "%(toolname)s" %(command_inputs)s %(command_outputs)s
+ """ # may NOT be an input or htmlout
+ tooltestsTabOnly = """
+
+
+
+
+ """
+ tooltestsHTMLOnly = """
+
+
+
+
+ """
+ tooltestsBoth = """
+
+
+
+
+
+ """
+ xdict = {}
+ xdict['tool_version'] = self.opts.tool_version
+ xdict['test1Input'] = self.test1Input
+ xdict['test1HTML'] = self.test1HTML
+ xdict['test1Output'] = self.test1Output
+ if self.opts.make_HTML and self.opts.output_tab <> 'None':
+ xdict['tooltests'] = tooltestsBoth % xdict
+ elif self.opts.make_HTML:
+ xdict['tooltests'] = tooltestsHTMLOnly % xdict
+ else:
+ xdict['tooltests'] = tooltestsTabOnly % xdict
+ xdict['script'] = self.escapedScript
+ # configfile is least painful way to embed script to avoid external dependencies
+ # but requires escaping of <, > and $ to avoid Mako parsing
+ if self.opts.help_text:
+ xdict['help'] = open(self.opts.help_text,'r').read()
+ else:
+ xdict['help'] = 'Please ask the tool author for help as none was supplied at tool generation'
+ coda = ['**Script**','Pressing execute will run the following code over your input file and generate some outputs in your history::']
+ coda.append(self.indentedScript)
+ coda.append('**Attribution** This Galaxy tool was created by %s at %s\nusing the Galaxy Tool Factory.' % (self.opts.user_email,timenow()))
+ coda.append('See %s for details of that project' % (toolFactoryURL))
+ coda.append('Please cite: Creating re-usable tools from scripts: The Galaxy Tool Factory. Ross Lazarus; Antony Kaspi; Mark Ziemann; The Galaxy Team. ')
+ coda.append('Bioinformatics 2012; doi: 10.1093/bioinformatics/bts573')
+ xdict['help'] = '%s\n%s' % (xdict['help'],'\n'.join(coda))
+ if self.opts.tool_desc:
+ xdict['tooldesc'] = '%s ' % self.opts.tool_desc
+ else:
+ xdict['tooldesc'] = ''
+ xdict['command_outputs'] = ''
+ xdict['outputs'] = ''
+ if self.opts.input_tab <> 'None':
+ xdict['command_inputs'] = '--input_tab "$input1" ' # the space may matter a lot if we append something
+ xdict['inputs'] = ' \n' % self.inputFormats
+ else:
+ xdict['command_inputs'] = '' # assume no input - eg a random data generator
+ xdict['inputs'] = ''
+ xdict['inputs'] += ' \n' % self.toolname
+ xdict['toolname'] = self.toolname
+ xdict['toolid'] = self.toolid
+ xdict['interpreter'] = self.opts.interpreter
+ xdict['scriptname'] = self.sfile
+ if self.opts.make_HTML:
+ xdict['command_outputs'] += ' --output_dir "$html_file.files_path" --output_html "$html_file" --make_HTML "yes" '
+ xdict['outputs'] += ' \n'
+ if self.opts.output_tab <> 'None':
+ xdict['command_outputs'] += ' --output_tab "$tab_file"'
+ xdict['outputs'] += ' \n' % self.outFormats
+ xdict['command'] = newCommand % xdict
+ xmls = newXML % xdict
+ xf = open(self.xmlfile,'w')
+ xf.write(xmls)
+ xf.write('\n')
+ xf.close()
+ # ready for the tarball
+
+
+ def makeTooltar(self):
+ """
+ a tool is a gz tarball with eg
+ /toolname/tool.xml /toolname/tool.py /toolname/test-data/test1_in.foo ...
+ """
+ retval = self.run()
+ if retval:
+ print >> sys.stderr,'## Run failed. Cannot build yet. Please fix and retry'
+ sys.exit(1)
+ self.makeXML()
+ tdir = self.toolname
+ os.mkdir(tdir)
+ if self.opts.input_tab <> 'None': # no reproducible test otherwise? TODO: maybe..
+ testdir = os.path.join(tdir,'test-data')
+ os.mkdir(testdir) # make tests directory
+ shutil.copyfile(self.opts.input_tab,os.path.join(testdir,self.test1Input))
+ if self.opts.output_tab <> 'None':
+ shutil.copyfile(self.opts.output_tab,os.path.join(testdir,self.test1Output))
+ if self.opts.make_HTML:
+ shutil.copyfile(self.opts.output_html,os.path.join(testdir,self.test1HTML))
+ if self.opts.output_dir:
+ shutil.copyfile(self.tlog,os.path.join(testdir,'test1_out.log'))
+ op = '%s.py' % self.toolname # new name
+ outpiname = os.path.join(tdir,op) # path for the tool tarball
+ pyin = os.path.basename(self.pyfile) # our name - we rewrite ourselves (TM)
+ notes = ['# %s - a self annotated version of %s generated by running %s\n' % (op,pyin,pyin),]
+ notes.append('# to make a new Galaxy tool called %s\n' % self.toolname)
+ notes.append('# User %s at %s\n' % (self.opts.user_email,timenow()))
+ pi = open(self.pyfile,'r').readlines() # our code becomes new tool wrapper (!) - first Galaxy worm
+ notes += pi
+ outpi = open(outpiname,'w')
+ outpi.write(''.join(notes))
+ outpi.write('\n')
+ outpi.close()
+ stname = os.path.join(tdir,self.sfile)
+ if not os.path.exists(stname):
+ shutil.copyfile(self.sfile, stname)
+ xtname = os.path.join(tdir,self.xmlfile)
+ if not os.path.exists(xtname):
+ shutil.copyfile(self.xmlfile,xtname)
+ tarpath = "%s.gz" % self.toolname
+ tar = tarfile.open(tarpath, "w:gz")
+ tar.add(tdir,arcname=self.toolname)
+ tar.close()
+ shutil.copyfile(tarpath,self.opts.new_tool)
+ shutil.rmtree(tdir)
+ ## TODO: replace with optional direct upload to local toolshed?
+ return retval
+
+
+ def compressPDF(self,inpdf=None,thumbformat='png'):
+ """need absolute path to pdf
+ note that GS gets confoozled if no $TMP or $TEMP
+ so we set it
+ """
+ assert os.path.isfile(inpdf), "## Input %s supplied to %s compressPDF not found" % (inpdf,self.myName)
+ hlog = os.path.join(self.opts.output_dir,"compress_%s.txt" % os.path.basename(inpdf))
+ sto = open(hlog,'a')
+ our_env = os.environ.copy()
+ our_tmp = our_env.get('TMP',None)
+ if not our_tmp:
+ our_tmp = our_env.get('TEMP',None)
+ if not (our_tmp and os.path.exists(our_tmp)):
+ newtmp = os.path.join(self.opts.output_dir,'tmp')
+ try:
+ os.mkdir(newtmp)
+ except:
+ sto.write('## WARNING - cannot make %s - it may exist or permissions need fixing\n' % newtmp)
+ our_env['TEMP'] = newtmp
+ if not self.temp_warned:
+ sto.write('## WARNING - no $TMP or $TEMP!!! Please fix - using %s temporarily\n' % newtmp)
+ self.temp_warned = True
+ outpdf = '%s_compressed' % inpdf
+ cl = ["gs", "-sDEVICE=pdfwrite", "-dNOPAUSE", "-dUseCIEColor", "-dBATCH","-dPDFSETTINGS=/printer", "-sOutputFile=%s" % outpdf,inpdf]
+ x = subprocess.Popen(cl,stdout=sto,stderr=sto,cwd=self.opts.output_dir,env=our_env)
+ retval1 = x.wait()
+ sto.close()
+ if retval1 == 0:
+ os.unlink(inpdf)
+ shutil.move(outpdf,inpdf)
+ os.unlink(hlog)
+ hlog = os.path.join(self.opts.output_dir,"thumbnail_%s.txt" % os.path.basename(inpdf))
+ sto = open(hlog,'w')
+ outpng = '%s.%s' % (os.path.splitext(inpdf)[0],thumbformat)
+ if self.useGM:
+ cl2 = ['gm', 'convert', inpdf, outpng]
+ else: # assume imagemagick
+ cl2 = ['convert', inpdf, outpng]
+ x = subprocess.Popen(cl2,stdout=sto,stderr=sto,cwd=self.opts.output_dir,env=our_env)
+ retval2 = x.wait()
+ sto.close()
+ if retval2 == 0:
+ os.unlink(hlog)
+ retval = retval1 or retval2
+ return retval
+
+
+ def getfSize(self,fpath,outpath):
+ """
+ format a nice file size string
+ """
+ size = ''
+ fp = os.path.join(outpath,fpath)
+ if os.path.isfile(fp):
+ size = '0 B'
+ n = float(os.path.getsize(fp))
+ if n > 2**20:
+ size = '%1.1f MB' % (n/2**20)
+ elif n > 2**10:
+ size = '%1.1f KB' % (n/2**10)
+ elif n > 0:
+ size = '%d B' % (int(n))
+ return size
+
+ def makeHtml(self):
+ """ Create an HTML file content to list all the artifacts found in the output_dir
+ """
+
+ galhtmlprefix = """
+
+
+
+
+
+
+
+
+ """
+ galhtmlattr = """
"""
+ galhtmlpostfix = """
\n"""
+
+ flist = os.listdir(self.opts.output_dir)
+ flist = [x for x in flist if x <> 'Rplots.pdf']
+ flist.sort()
+ html = []
+ html.append(galhtmlprefix % progname)
+ html.append('Galaxy Tool "%s" run at %s
' % (self.toolname,timenow()))
+ fhtml = []
+ if len(flist) > 0:
+ logfiles = [x for x in flist if x.lower().endswith('.log')] # log file names determine sections
+ logfiles.sort()
+ logfiles = [x for x in logfiles if os.path.abspath(x) <> os.path.abspath(self.tlog)]
+ logfiles.append(os.path.abspath(self.tlog)) # make it the last one
+ pdflist = []
+ npdf = len([x for x in flist if os.path.splitext(x)[-1].lower() == '.pdf'])
+ for rownum,fname in enumerate(flist):
+ dname,e = os.path.splitext(fname)
+ sfsize = self.getfSize(fname,self.opts.output_dir)
+ if e.lower() == '.pdf' : # compress and make a thumbnail
+ thumb = '%s.%s' % (dname,self.thumbformat)
+ pdff = os.path.join(self.opts.output_dir,fname)
+ retval = self.compressPDF(inpdf=pdff,thumbformat=self.thumbformat)
+ if retval == 0:
+ pdflist.append((fname,thumb))
+ else:
+ pdflist.append((fname,fname))
+ if (rownum+1) % 2 == 0:
+ fhtml.append('%s %s ' % (fname,fname,sfsize))
+ else:
+ fhtml.append('%s %s ' % (fname,fname,sfsize))
+ for logfname in logfiles: # expect at least tlog - if more
+ if os.path.abspath(logfname) == os.path.abspath(self.tlog): # handled later
+ sectionname = 'All tool run'
+ if (len(logfiles) > 1):
+ sectionname = 'Other'
+ ourpdfs = pdflist
+ else:
+ realname = os.path.basename(logfname)
+ sectionname = os.path.splitext(realname)[0].split('_')[0] # break in case _ added to log
+ ourpdfs = [x for x in pdflist if os.path.basename(x[0]).split('_')[0] == sectionname]
+ pdflist = [x for x in pdflist if os.path.basename(x[0]).split('_')[0] <> sectionname] # remove
+ nacross = 1
+ npdf = len(ourpdfs)
+
+ if npdf > 0:
+ nacross = math.sqrt(npdf) ## int(round(math.log(npdf,2)))
+ if int(nacross)**2 != npdf:
+ nacross += 1
+ nacross = int(nacross)
+ width = min(400,int(1200/nacross))
+ html.append('%s images and outputs
' % sectionname)
+ html.append('(Click on a thumbnail image to download the corresponding original PDF image) ')
+ ntogo = nacross # counter for table row padding with empty cells
+ html.append('\n')
+ for i,paths in enumerate(ourpdfs):
+ fname,thumb = paths
+ s= """ \n""" % (fname,thumb,fname,width,fname)
+ if ((i+1) % nacross == 0):
+ s += ' \n'
+ ntogo = 0
+ if i < (npdf - 1): # more to come
+ s += ''
+ ntogo = nacross
+ else:
+ ntogo -= 1
+ html.append(s)
+ if html[-1].strip().endswith(' '):
+ html.append('
\n')
+ else:
+ if ntogo > 0: # pad
+ html.append(' '*ntogo)
+ html.append('\n')
+ logt = open(logfname,'r').readlines()
+ logtext = [x for x in logt if x.strip() > '']
+ html.append('%s log output
' % sectionname)
+ if len(logtext) > 1:
+ html.append('\n\n')
+ html += logtext
+ html.append('\n \n')
+ else:
+ html.append('%s is empty ' % logfname)
+ if len(fhtml) > 0:
+ fhtml.insert(0,'Output File Name (click to view) Size \n')
+ fhtml.append('
')
+ html.append('All output files available for downloading
\n')
+ html += fhtml # add all non-pdf files to the end of the display
+ else:
+ html.append('### Error - %s returned no files - please confirm that parameters are sane
' % self.opts.interpreter)
+ html.append(galhtmlpostfix)
+ htmlf = file(self.opts.output_html,'w')
+ htmlf.write('\n'.join(html))
+ htmlf.write('\n')
+ htmlf.close()
+ self.html = html
+
+
+ def run(self):
+ """
+ scripts must be small enough not to fill the pipe!
+ """
+ if self.treatbashSpecial and self.opts.interpreter in ['bash','sh']:
+ retval = self.runBash()
+ else:
+ if self.opts.output_dir:
+ ste = open(self.elog,'w')
+ sto = open(self.tlog,'w')
+ sto.write('## Toolfactory generated command line = %s\n' % ' '.join(self.cl))
+ sto.flush()
+ p = subprocess.Popen(self.cl,shell=False,stdout=sto,stderr=ste,stdin=subprocess.PIPE,cwd=self.opts.output_dir)
+ else:
+ p = subprocess.Popen(self.cl,shell=False,stdin=subprocess.PIPE)
+ p.stdin.write(self.script)
+ p.stdin.close()
+ retval = p.wait()
+ if self.opts.output_dir:
+ sto.close()
+ ste.close()
+ err = open(self.elog,'r').read()
+ if retval <> 0 and err: # problem
+ print >> sys.stderr,err
+ if self.opts.make_HTML:
+ self.makeHtml()
+ return retval
+
+ def runBash(self):
+ """
+ cannot use - for bash so use self.sfile
+ """
+ if self.opts.output_dir:
+ s = '## Toolfactory generated command line = %s\n' % ' '.join(self.cl)
+ sto = open(self.tlog,'w')
+ sto.write(s)
+ sto.flush()
+ p = subprocess.Popen(self.cl,shell=False,stdout=sto,stderr=sto,cwd=self.opts.output_dir)
+ else:
+ p = subprocess.Popen(self.cl,shell=False)
+ retval = p.wait()
+ if self.opts.output_dir:
+ sto.close()
+ if self.opts.make_HTML:
+ self.makeHtml()
+ return retval
+
+
+def main():
+ u = """
+ This is a Galaxy wrapper. It expects to be called by a special purpose tool.xml as:
+ rgToolFactory.py --script_path "$scriptPath" --tool_name "foo" --interpreter "Rscript"
+
+ """
+ op = optparse.OptionParser()
+ a = op.add_option
+ a('--script_path',default=None)
+ a('--tool_name',default=None)
+ a('--interpreter',default=None)
+ a('--output_dir',default=None)
+ a('--output_html',default=None)
+ a('--input_tab',default="None")
+ a('--output_tab',default="None")
+ a('--user_email',default='Unknown')
+ a('--bad_user',default=None)
+ a('--make_Tool',default=None)
+ a('--make_HTML',default=None)
+ a('--help_text',default=None)
+ a('--tool_desc',default=None)
+ a('--new_tool',default=None)
+ a('--tool_version',default=None)
+ opts, args = op.parse_args()
+ assert not opts.bad_user,'UNAUTHORISED: %s is NOT authorized to use this tool until Galaxy admin adds %s to admin_users in universe_wsgi.ini' % (opts.bad_user,opts.bad_user)
+ assert opts.tool_name,'## Tool Factory expects a tool name - eg --tool_name=DESeq'
+ assert opts.interpreter,'## Tool Factory wrapper expects an interpreter - eg --interpreter=Rscript'
+ assert os.path.isfile(opts.script_path),'## Tool Factory wrapper expects a script path - eg --script_path=foo.R'
+ if opts.output_dir:
+ try:
+ os.makedirs(opts.output_dir)
+ except:
+ pass
+ r = ScriptRunner(opts)
+ if opts.make_Tool:
+ retcode = r.makeTooltar()
+ else:
+ retcode = r.run()
+ os.unlink(r.sfile)
+ if retcode:
+ sys.exit(retcode) # indicate failure to job runner
+
+
+if __name__ == "__main__":
+ main()
+
+
diff -r 21b218a7429f -r 0de946608423 rgedgeRpaired.xml.camera
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/rgedgeRpaired.xml.camera Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,1084 @@
+
+ models using BioConductor packages
+
+ biocbasics
+ r302
+ graphicsmagick
+ ghostscript
+
+
+
+ rgToolFactory.py --script_path "$runme" --interpreter "Rscript" --tool_name "DifferentialCounts"
+ --output_dir "$html_file.files_path" --output_html "$html_file" --make_HTML "yes"
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+ Do not run edgeR
+ Run edgeR
+
+
+
+
+
+
+
+
+ Do not run DESeq2
+ Run DESeq2
+
+
+
+ Parametric (default) fit for dispersions
+ Local fit - this will automagically be used if parametric fit fails
+ Mean dispersion fit- use this if you really understand what you're doing - read the fine manual linked below in the documentation
+
+
+
+
+
+ Do not run VOOM
+ Run VOOM
+
+
+
+
+ fdr
+ Benjamini Hochberg
+ Benjamini Yukateli
+ Bonferroni
+ Hochberg
+ Holm
+ Hommel
+ no control for multiple tests
+
+
+
+
+ edgeR['doedgeR'] == "T"
+
+
+ DESeq2['doDESeq2'] == "T"
+
+
+ doVoom == "T"
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+ nsamp) {
+ dm =dm[1:nsamp,]
+ #sub = paste('Showing',nsamp,'contigs ranked for evidence for differential abundance out of',nprobes,'total')
+ }
+ newcolnames = substr(colnames(dm),1,20)
+ colnames(dm) = newcolnames
+ pdf(outpdfname)
+ heatmap.2(dm,main=myTitle,ColSideColors=pcols,col=topo.colors(100),dendrogram="col",key=T,density.info='none',
+ Rowv=F,scale='row',trace='none',margins=c(8,8),cexRow=0.4,cexCol=0.5)
+ dev.off()
+}
+
+hmap = function(cmat,nmeans=4,outpdfname="heatMap.pdf",nsamp=250,TName='Treatment',group=NA,myTitle="Title goes here")
+{
+ # for 2 groups only was
+ #col.map = function(g) {if (g==TName) "#FF0000" else "#0000FF"}
+ #pcols = unlist(lapply(group,col.map))
+ gu = unique(group)
+ colours = rainbow(length(gu),start=0.3,end=0.6)
+ pcols = colours[match(group,gu)]
+ nrows = nrow(cmat)
+ mtitle = paste(myTitle,'Heatmap: n contigs =',nrows)
+ if (nrows > nsamp) {
+ cmat = cmat[c(1:nsamp),]
+ mtitle = paste('Heatmap: Top ',nsamp,' DE contigs (of ',nrows,')',sep='')
+ }
+ newcolnames = substr(colnames(cmat),1,20)
+ colnames(cmat) = newcolnames
+ pdf(outpdfname)
+ heatmap(cmat,scale='row',main=mtitle,cexRow=0.3,cexCol=0.4,Rowv=NA,ColSideColors=pcols)
+ dev.off()
+}
+
+qqPlot = function(descr='qqplot',pvector, outpdf='qqplot.pdf',...)
+# stolen from https://gist.github.com/703512
+{
+ o = -log10(sort(pvector,decreasing=F))
+ e = -log10( 1:length(o)/length(o) )
+ o[o==-Inf] = reallysmall
+ o[o==Inf] = reallybig
+ maint = descr
+ pdf(outpdf)
+ plot(e,o,pch=19,cex=1, main=maint, ...,
+ xlab=expression(Expected~~-log[10](italic(p))),
+ ylab=expression(Observed~~-log[10](italic(p))),
+ xlim=c(0,max(e)), ylim=c(0,max(o)))
+ lines(e,e,col="red")
+ grid(col = "lightgray", lty = "dotted")
+ dev.off()
+}
+
+smearPlot = function(DGEList,deTags, outSmear, outMain)
+ {
+ pdf(outSmear)
+ plotSmear(DGEList,de.tags=deTags,main=outMain)
+ grid(col="lightgray", lty="dotted")
+ dev.off()
+ }
+
+boxPlot = function(rawrs,cleanrs,maint,myTitle,pdfname)
+{ #
+ nc = ncol(rawrs)
+ for (i in c(1:nc)) {rawrs[(rawrs[,i] < 0),i] = NA}
+ fullnames = colnames(rawrs)
+ newcolnames = substr(colnames(rawrs),1,20)
+ colnames(rawrs) = newcolnames
+ newcolnames = substr(colnames(cleanrs),1,20)
+ colnames(cleanrs) = newcolnames
+ defpar = par(no.readonly=T)
+ print.noquote('raw contig counts by sample:')
+ print.noquote(summary(rawrs))
+ print.noquote('normalised contig counts by sample:')
+ print.noquote(summary(cleanrs))
+ pdf(pdfname)
+ par(mfrow=c(1,2))
+ boxplot(rawrs,varwidth=T,notch=T,ylab='log contig count',col="maroon",las=3,cex.axis=0.35,main=paste('Raw:',maint))
+ grid(col="lightgray",lty="dotted")
+ boxplot(cleanrs,varwidth=T,notch=T,ylab='log contig count',col="maroon",las=3,cex.axis=0.35,main=paste('After ',maint))
+ grid(col="lightgray",lty="dotted")
+ dev.off()
+ pdfname = "sample_counts_histogram.pdf"
+ nc = ncol(rawrs)
+ print.noquote(paste('Using ncol rawrs=',nc))
+ ncroot = round(sqrt(nc))
+ if (ncroot*ncroot < nc) { ncroot = ncroot + 1 }
+ m = c()
+ for (i in c(1:nc)) {
+ rhist = hist(rawrs[,i],breaks=100,plot=F)
+ m = append(m,max(rhist\$counts))
+ }
+ ymax = max(m)
+ ncols = length(fullnames)
+ if (ncols > 20)
+ {
+ scale = 7*ncols/20
+ pdf(pdfname,width=scale,height=scale)
+ } else {
+ pdf(pdfname)
+ }
+ par(mfrow=c(ncroot,ncroot))
+ for (i in c(1:nc)) {
+ hist(rawrs[,i], main=paste("Contig logcount",i), xlab='log raw count', col="maroon",
+ breaks=100,sub=fullnames[i],cex=0.8,ylim=c(0,ymax))
+ }
+ dev.off()
+ par(defpar)
+
+}
+
+cumPlot = function(rawrs,cleanrs,maint,myTitle)
+{ # updated to use ecdf
+ pdfname = "Filtering_rowsum_bar_charts.pdf"
+ defpar = par(no.readonly=T)
+ lrs = log(rawrs,10)
+ lim = max(lrs)
+ pdf(pdfname)
+ par(mfrow=c(2,1))
+ hist(lrs,breaks=100,main=paste('Before:',maint),xlab="# Reads (log)",
+ ylab="Count",col="maroon",sub=myTitle, xlim=c(0,lim),las=1)
+ grid(col="lightgray", lty="dotted")
+ lrs = log(cleanrs,10)
+ hist(lrs,breaks=100,main=paste('After:',maint),xlab="# Reads (log)",
+ ylab="Count",col="maroon",sub=myTitle,xlim=c(0,lim),las=1)
+ grid(col="lightgray", lty="dotted")
+ dev.off()
+ par(defpar)
+}
+
+cumPlot1 = function(rawrs,cleanrs,maint,myTitle)
+{ # updated to use ecdf
+ pdfname = paste(gsub(" ","", myTitle , fixed=TRUE),"RowsumCum.pdf",sep='_')
+ pdf(pdfname)
+ par(mfrow=c(2,1))
+ lastx = max(rawrs)
+ rawe = knots(ecdf(rawrs))
+ cleane = knots(ecdf(cleanrs))
+ cy = 1:length(cleane)/length(cleane)
+ ry = 1:length(rawe)/length(rawe)
+ plot(rawe,ry,type='l',main=paste('Before',maint),xlab="Log Contig Total Reads",
+ ylab="Cumulative proportion",col="maroon",log='x',xlim=c(1,lastx),sub=myTitle)
+ grid(col="blue")
+ plot(cleane,cy,type='l',main=paste('After',maint),xlab="Log Contig Total Reads",
+ ylab="Cumulative proportion",col="maroon",log='x',xlim=c(1,lastx),sub=myTitle)
+ grid(col="blue")
+ dev.off()
+}
+
+
+
+doGSEAold = function(y=NULL,design=NULL,histgmt="",
+ bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ ntest=0, myTitle="myTitle", outfname="GSEA.xls", minnin=5, maxnin=2000,fdrthresh=0.05,fdrtype="BH")
+{
+ sink('Camera.log')
+ genesets = c()
+ if (bigmt > "")
+ {
+ bigenesets = readLines(bigmt)
+ genesets = bigenesets
+ }
+ if (histgmt > "")
+ {
+ hgenesets = readLines(histgmt)
+ if (bigmt > "") {
+ genesets = rbind(genesets,hgenesets)
+ } else {
+ genesets = hgenesets
+ } # use only history if no bi
+ }
+ print.noquote(paste("@@@read",length(genesets), 'genesets from',histgmt,bigmt))
+ genesets = strsplit(genesets,'\t') # tabular. genesetid\tURLorwhatever\tgene_1\t..\tgene_n
+ outf = outfname
+ head=paste(myTitle,'edgeR GSEA')
+ write(head,file=outfname,append=F)
+ ntest=length(genesets)
+ urownames = toupper(rownames(y))
+ upcam = c()
+ downcam = c()
+ for (i in 1:ntest) {
+ gs = unlist(genesets[i])
+ g = gs[1] # geneset_id
+ u = gs[2]
+ if (u > "") { u = paste("",u," ",sep="") }
+ glist = gs[3:length(gs)] # member gene symbols
+ glist = toupper(glist)
+ inglist = urownames %in% glist
+ nin = sum(inglist)
+ if ((nin > minnin) && (nin < maxnin)) {
+ ### print(paste('@@found',sum(inglist),'genes in glist'))
+ camres = camera(y=y,index=inglist,design=design)
+ if (! is.null(camres)) {
+ rownames(camres) = g # gene set name
+ camres = cbind(GeneSet=g,URL=u,camres)
+ if (camres\$Direction == "Up")
+ {
+ upcam = rbind(upcam,camres) } else {
+ downcam = rbind(downcam,camres)
+ }
+ }
+ }
+ }
+ uscam = upcam[order(upcam\$PValue),]
+ unadjp = uscam\$PValue
+ uscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ nup = max(10,sum((uscam\$adjPValue < fdrthresh)))
+ dscam = downcam[order(downcam\$PValue),]
+ unadjp = dscam\$PValue
+ dscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ ndown = max(10,sum((dscam\$adjPValue < fdrthresh)))
+ write.table(uscam,file=paste('camera_up',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ write.table(dscam,file=paste('camera_down',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera up top',nup,'gene sets:'))
+ write.table(head(uscam,nup),file="",quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera down top',ndown,'gene sets:'))
+ write.table(head(dscam,ndown),file="",quote=F,sep='\t',row.names=F)
+ sink()
+}
+
+
+
+
+doGSEA = function(y=NULL,design=NULL,histgmt="",
+ bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ ntest=0, myTitle="myTitle", outfname="GSEA.xls", minnin=5, maxnin=2000,fdrthresh=0.05,fdrtype="BH")
+{
+ sink('Camera.log')
+ genesets = c()
+ if (bigmt > "")
+ {
+ bigenesets = readLines(bigmt)
+ genesets = bigenesets
+ }
+ if (histgmt > "")
+ {
+ hgenesets = readLines(histgmt)
+ if (bigmt > "") {
+ genesets = rbind(genesets,hgenesets)
+ } else {
+ genesets = hgenesets
+ } # use only history if no bi
+ }
+ print.noquote(paste("@@@read",length(genesets), 'genesets from',histgmt,bigmt))
+ genesets = strsplit(genesets,'\t') # tabular. genesetid\tURLorwhatever\tgene_1\t..\tgene_n
+ outf = outfname
+ head=paste(myTitle,'edgeR GSEA')
+ write(head,file=outfname,append=F)
+ ntest=length(genesets)
+ urownames = toupper(rownames(y))
+ upcam = c()
+ downcam = c()
+ incam = c()
+ urls = c()
+ gsids = c()
+ for (i in 1:ntest) {
+ gs = unlist(genesets[i])
+ gsid = gs[1] # geneset_id
+ url = gs[2]
+ if (url > "") { url = paste("",url," ",sep="") }
+ glist = gs[3:length(gs)] # member gene symbols
+ glist = toupper(glist)
+ inglist = urownames %in% glist
+ nin = sum(inglist)
+ if ((nin > minnin) && (nin < maxnin)) {
+ incam = c(incam,inglist)
+ gsids = c(gsids,gsid)
+ urls = c(urls,url)
+ }
+ }
+ incam = as.list(incam)
+ names(incam) = gsids
+ allcam = camera(y=y,index=incam,design=design)
+ allcamres = cbind(geneset=gsids,allcam,URL=urls)
+ for (i in 1:ntest) {
+ camres = allcamres[i]
+ res = try(test = (camres\$Direction == "Up"))
+ if ("try-error" %in% class(res)) {
+ cat("test failed, camres = :")
+ print.noquote(camres)
+ } else { if (camres\$Direction == "Up")
+ { upcam = rbind(upcam,camres)
+ } else { downcam = rbind(downcam,camres)
+ }
+
+ }
+ }
+ uscam = upcam[order(upcam\$PValue),]
+ unadjp = uscam\$PValue
+ uscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ nup = max(10,sum((uscam\$adjPValue < fdrthresh)))
+ dscam = downcam[order(downcam\$PValue),]
+ unadjp = dscam\$PValue
+ dscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ ndown = max(10,sum((dscam\$adjPValue < fdrthresh)))
+ write.table(uscam,file=paste('camera_up',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ write.table(dscam,file=paste('camera_down',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera up top',nup,'gene sets:'))
+ write.table(head(uscam,nup),file="",quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera down top',ndown,'gene sets:'))
+ write.table(head(dscam,ndown),file="",quote=F,sep='\t',row.names=F)
+ sink()
+ }
+
+
+edgeIt = function (Count_Matrix=c(),group=c(),out_edgeR=F,out_VOOM=F,out_DESeq2=F,fdrtype='fdr',priordf=5,
+ fdrthresh=0.05,outputdir='.', myTitle='Differential Counts',libSize=c(),useNDF=F,
+ filterquantile=0.2, subjects=c(),mydesign=NULL,
+ doDESeq2=T,doVoom=T,doCamera=T,doedgeR=T,org='hg19',
+ histgmt="", bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ doCook=F,DESeq_fitType="parameteric")
+{
+ # Error handling
+ if (length(unique(group))!=2){
+ print("Number of conditions identified in experiment does not equal 2")
+ q()
+ }
+ require(edgeR)
+ options(width = 512)
+ mt = paste(unlist(strsplit(myTitle,'_')),collapse=" ")
+ allN = nrow(Count_Matrix)
+ nscut = round(ncol(Count_Matrix)/2)
+ colTotmillionreads = colSums(Count_Matrix)/1e6
+ counts.dataframe = as.data.frame(c())
+ rawrs = rowSums(Count_Matrix)
+ nonzerod = Count_Matrix[(rawrs > 0),] # remove all zero count genes
+ nzN = nrow(nonzerod)
+ nzrs = rowSums(nonzerod)
+ zN = allN - nzN
+ print('# Quantiles for non-zero row counts:',quote=F)
+ print(quantile(nzrs,probs=seq(0,1,0.1)),quote=F)
+ if (useNDF == T)
+ {
+ gt1rpin3 = rowSums(Count_Matrix/expandAsMatrix(colTotmillionreads,dim(Count_Matrix)) >= 1) >= nscut
+ lo = colSums(Count_Matrix[!gt1rpin3,])
+ workCM = Count_Matrix[gt1rpin3,]
+ cleanrs = rowSums(workCM)
+ cleanN = length(cleanrs)
+ meth = paste( "After removing",length(lo),"contigs with fewer than ",nscut," sample read counts >= 1 per million, there are",sep="")
+ print(paste("Read",allN,"contigs. Removed",zN,"contigs with no reads.",meth,cleanN,"contigs"),quote=F)
+ maint = paste('Filter >=1/million reads in >=',nscut,'samples')
+ } else {
+ useme = (nzrs > quantile(nzrs,filterquantile))
+ workCM = nonzerod[useme,]
+ lo = colSums(nonzerod[!useme,])
+ cleanrs = rowSums(workCM)
+ cleanN = length(cleanrs)
+ meth = paste("After filtering at count quantile =",filterquantile,", there are",sep="")
+ print(paste('Read',allN,"contigs. Removed",zN,"with no reads.",meth,cleanN,"contigs"),quote=F)
+ maint = paste('Filter below',filterquantile,'quantile')
+ }
+ cumPlot(rawrs=rawrs,cleanrs=cleanrs,maint=maint,myTitle=myTitle)
+ allgenes = rownames(workCM)
+ reg = "^chr([0-9]+):([0-9]+)-([0-9]+)"
+ genecards=" 0.8) # is ucsc style string
+ {
+ print("@@ using ucsc substitution for urls")
+ contigurls = paste0(ucsc,"&position=chr",testreg[,2],":",testreg[,3],"-",testreg[,4],"\'>",allgenes," ")
+ } else {
+ print("@@ using genecards substitution for urls")
+ contigurls = paste0(genecards,allgenes,"\'>",allgenes,"")
+ }
+ print.noquote("# urls")
+ print.noquote(head(contigurls))
+ print(paste("# Total low count contigs per sample = ",paste(lo,collapse=',')),quote=F)
+ cmrowsums = rowSums(workCM)
+ TName=unique(group)[1]
+ CName=unique(group)[2]
+ if (is.null(mydesign)) {
+ if (length(subjects) == 0)
+ {
+ mydesign = model.matrix(~group)
+ }
+ else {
+ subjf = factor(subjects)
+ mydesign = model.matrix(~subjf+group) # we block on subject so make group last to simplify finding it
+ }
+ }
+ print.noquote(paste('Using samples:',paste(colnames(workCM),collapse=',')))
+ print.noquote('Using design matrix:')
+ print.noquote(mydesign)
+ if (doedgeR) {
+ sink('edgeR.log')
+ #### Setup DGEList object
+ DGEList = DGEList(counts=workCM, group = group)
+ DGEList = calcNormFactors(DGEList)
+
+ DGEList = estimateGLMCommonDisp(DGEList,mydesign)
+ comdisp = DGEList\$common.dispersion
+ DGEList = estimateGLMTrendedDisp(DGEList,mydesign)
+ if (edgeR_priordf > 0) {
+ print.noquote(paste("prior.df =",edgeR_priordf))
+ DGEList = estimateGLMTagwiseDisp(DGEList,mydesign,prior.df = edgeR_priordf)
+ } else {
+ DGEList = estimateGLMTagwiseDisp(DGEList,mydesign)
+ }
+ DGLM = glmFit(DGEList,design=mydesign)
+ DE = glmLRT(DGLM,coef=ncol(DGLM\$design)) # always last one - subject is first if needed
+ efflib = DGEList\$samples\$lib.size*DGEList\$samples\$norm.factors
+ normData = (1e+06*DGEList\$counts/efflib)
+ uoutput = cbind(
+ Name=as.character(rownames(DGEList\$counts)),
+ DE\$table,
+ adj.p.value=p.adjust(DE\$table\$PValue, method=fdrtype),
+ Dispersion=DGEList\$tagwise.dispersion,totreads=cmrowsums,normData,
+ DGEList\$counts
+ )
+ soutput = uoutput[order(DE\$table\$PValue),] # sorted into p value order - for quick toptable
+ goodness = gof(DGLM, pcutoff=fdrthresh)
+ if (sum(goodness\$outlier) > 0) {
+ print.noquote('GLM outliers:')
+ print(paste(rownames(DGLM)[(goodness\$outlier)],collapse=','),quote=F)
+ } else {
+ print('No GLM fit outlier genes found\n')
+ }
+ z = limma::zscoreGamma(goodness\$gof.statistic, shape=goodness\$df/2, scale=2)
+ pdf("edgeR_GoodnessofFit.pdf")
+ qq = qqnorm(z, panel.first=grid(), main="tagwise dispersion")
+ abline(0,1,lwd=3)
+ points(qq\$x[goodness\$outlier],qq\$y[goodness\$outlier], pch=16, col="maroon")
+ dev.off()
+ estpriorn = getPriorN(DGEList)
+ print(paste("Common Dispersion =",comdisp,"CV = ",sqrt(comdisp),"getPriorN = ",estpriorn),quote=F)
+ efflib = DGEList\$samples\$lib.size*DGEList\$samples\$norm.factors
+ normData = (1e+06*DGEList\$counts/efflib)
+ uniqueg = unique(group)
+ #### Plot MDS
+ sample_colors = match(group,levels(group))
+ sampleTypes = levels(factor(group))
+ print.noquote(sampleTypes)
+ pdf("edgeR_MDSplot.pdf")
+ plotMDS.DGEList(DGEList,main=paste("edgeR MDS for",myTitle),cex=0.5,col=sample_colors,pch=sample_colors)
+ legend(x="topleft", legend = sampleTypes,col=c(1:length(sampleTypes)), pch=19)
+ grid(col="blue")
+ dev.off()
+ colnames(normData) = paste( colnames(normData),'N',sep="_")
+ print(paste('Raw sample read totals',paste(colSums(nonzerod,na.rm=T),collapse=',')))
+ nzd = data.frame(log(nonzerod + 1e-2,10))
+ try( boxPlot(rawrs=nzd,cleanrs=log(normData,10),maint='TMM Normalisation',myTitle=myTitle,pdfname="edgeR_raw_norm_counts_box.pdf") )
+ write.table(soutput,file=out_edgeR, quote=FALSE, sep="\t",row.names=F)
+ tt = cbind(
+ Name=as.character(rownames(DGEList\$counts)),
+ DE\$table,
+ adj.p.value=p.adjust(DE\$table\$PValue, method=fdrtype),
+ Dispersion=DGEList\$tagwise.dispersion,totreads=cmrowsums
+ )
+ print.noquote("# edgeR Top tags\n")
+ tt = cbind(tt,URL=contigurls) # add to end so table isn't laid out strangely
+ tt = tt[order(DE\$table\$PValue),]
+ print.noquote(tt[1:50,])
+ deTags = rownames(uoutput[uoutput\$adj.p.value < fdrthresh,])
+ nsig = length(deTags)
+ print(paste('#',nsig,'tags significant at adj p=',fdrthresh),quote=F)
+ deColours = ifelse(deTags,'red','black')
+ pdf("edgeR_BCV_vs_abundance.pdf")
+ plotBCV(DGEList, cex=0.3, main="Biological CV vs abundance")
+ dev.off()
+ dg = DGEList[order(DE\$table\$PValue),]
+ #normData = (1e+06 * dg\$counts/expandAsMatrix(dg\$samples\$lib.size, dim(dg)))
+ efflib = dg\$samples\$lib.size*dg\$samples\$norm.factors
+ normData = (1e+06*dg\$counts/efflib)
+ outpdfname="edgeR_top_100_heatmap.pdf"
+ hmap2(normData,nsamp=100,TName=TName,group=group,outpdfname=outpdfname,myTitle=paste('edgeR Heatmap',myTitle))
+ outSmear = "edgeR_smearplot.pdf"
+ outMain = paste("Smear Plot for ",TName,' Vs ',CName,' (FDR@',fdrthresh,' N = ',nsig,')',sep='')
+ smearPlot(DGEList=DGEList,deTags=deTags, outSmear=outSmear, outMain = outMain)
+ qqPlot(descr=paste(myTitle,'edgeR adj p QQ plot'),pvector=tt\$adj.p.value,outpdf='edgeR_qqplot.pdf')
+ norm.factor = DGEList\$samples\$norm.factors
+ topresults.edgeR = soutput[which(soutput\$adj.p.value < fdrthresh), ]
+ edgeRcountsindex = which(allgenes %in% rownames(topresults.edgeR))
+ edgeRcounts = rep(0, length(allgenes))
+ edgeRcounts[edgeRcountsindex] = 1 # Create venn diagram of hits
+ sink()
+ } ### doedgeR
+ if (doDESeq2 == T)
+ {
+ sink("DESeq2.log")
+ # DESeq2
+ require('DESeq2')
+ library('RColorBrewer')
+ if (length(subjects) == 0)
+ {
+ pdata = data.frame(Name=colnames(workCM),Rx=group,row.names=colnames(workCM))
+ deSEQds = DESeqDataSetFromMatrix(countData = workCM, colData = pdata, design = formula(~ Rx))
+ } else {
+ pdata = data.frame(Name=colnames(workCM),Rx=group,subjects=subjects,row.names=colnames(workCM))
+ deSEQds = DESeqDataSetFromMatrix(countData = workCM, colData = pdata, design = formula(~ subjects + Rx))
+ }
+ #DESeq2 = DESeq(deSEQds,fitType='local',pAdjustMethod=fdrtype)
+ #rDESeq = results(DESeq2)
+ #newCountDataSet(workCM, group)
+ deSeqDatsizefac = estimateSizeFactors(deSEQds)
+ deSeqDatdisp = estimateDispersions(deSeqDatsizefac,fitType=DESeq_fitType)
+ resDESeq = nbinomWaldTest(deSeqDatdisp, pAdjustMethod=fdrtype)
+ rDESeq = as.data.frame(results(resDESeq))
+ rDESeq = cbind(Contig=rownames(workCM),rDESeq,NReads=cmrowsums,URL=contigurls)
+ srDESeq = rDESeq[order(rDESeq\$pvalue),]
+ qqPlot(descr=paste(myTitle,'DESeq2 adj p qq plot'),pvector=rDESeq\$padj,outpdf='DESeq2_qqplot.pdf')
+ cat("# DESeq top 50\n")
+ print.noquote(srDESeq[1:50,])
+ write.table(srDESeq,file=out_DESeq2, quote=FALSE, sep="\t",row.names=F)
+ topresults.DESeq = rDESeq[which(rDESeq\$padj < fdrthresh), ]
+ DESeqcountsindex = which(allgenes %in% rownames(topresults.DESeq))
+ DESeqcounts = rep(0, length(allgenes))
+ DESeqcounts[DESeqcountsindex] = 1
+ pdf("DESeq2_dispersion_estimates.pdf")
+ plotDispEsts(resDESeq)
+ dev.off()
+ ysmall = abs(min(rDESeq\$log2FoldChange))
+ ybig = abs(max(rDESeq\$log2FoldChange))
+ ylimit = min(4,ysmall,ybig)
+ pdf("DESeq2_MA_plot.pdf")
+ plotMA(resDESeq,main=paste(myTitle,"DESeq2 MA plot"),ylim=c(-ylimit,ylimit))
+ dev.off()
+ rlogres = rlogTransformation(resDESeq)
+ sampledists = dist( t( assay(rlogres) ) )
+ sdmat = as.matrix(sampledists)
+ pdf("DESeq2_sample_distance_plot.pdf")
+ heatmap.2(sdmat,trace="none",main=paste(myTitle,"DESeq2 sample distances"),
+ col = colorRampPalette( rev(brewer.pal(9, "RdBu")) )(255))
+ dev.off()
+ ###outpdfname="DESeq2_top50_heatmap.pdf"
+ ###hmap2(sresDESeq,nsamp=50,TName=TName,group=group,outpdfname=outpdfname,myTitle=paste('DESeq2 vst rlog Heatmap',myTitle))
+ sink()
+ result = try( (ppca = plotPCA( varianceStabilizingTransformation(deSeqDatdisp,blind=T), intgroup=c("Rx","Name")) ) )
+ if ("try-error" %in% class(result)) {
+ print.noquote('DESeq2 plotPCA failed.')
+ } else {
+ pdf("DESeq2_PCA_plot.pdf")
+ #### wtf - print? Seems needed to get this to work
+ print(ppca)
+ dev.off()
+ }
+ }
+
+ if (doVoom == T) {
+ sink('VOOM.log')
+ if (doedgeR == F) {
+ #### Setup DGEList object
+ DGEList = DGEList(counts=workCM, group = group)
+ DGEList = calcNormFactors(DGEList)
+ DGEList = estimateGLMCommonDisp(DGEList,mydesign)
+ DGEList = estimateGLMTrendedDisp(DGEList,mydesign)
+ DGEList = estimateGLMTagwiseDisp(DGEList,mydesign)
+ DGEList = estimateGLMTagwiseDisp(DGEList,mydesign)
+ norm.factor = DGEList\$samples\$norm.factors
+ }
+ pdf("VOOM_mean_variance_plot.pdf")
+ dat.voomed = voom(DGEList, mydesign, plot = TRUE, lib.size = colSums(workCM) * norm.factor)
+ dev.off()
+ # Use limma to fit data
+ fit = lmFit(dat.voomed, mydesign)
+ fit = eBayes(fit)
+ rvoom = topTable(fit, coef = length(colnames(mydesign)), adj = fdrtype, n = Inf, sort="none")
+ qqPlot(descr=paste(myTitle,'VOOM-limma adj p QQ plot'),pvector=rvoom\$adj.P.Val,outpdf='VOOM_qqplot.pdf')
+ rownames(rvoom) = rownames(workCM)
+ rvoom = cbind(rvoom,NReads=cmrowsums,URL=contigurls)
+ srvoom = rvoom[order(rvoom\$P.Value),]
+ cat("# VOOM top 50\n")
+ print(srvoom[1:50,])
+ write.table(srvoom,file=out_VOOM, quote=FALSE, sep="\t",row.names=F)
+ # Use an FDR cutoff to find interesting samples for edgeR, DESeq and voom/limma
+ topresults.voom = rvoom[which(rvoom\$adj.P.Val < fdrthresh), ]
+ voomcountsindex = which(allgenes %in% topresults.voom\$ID)
+ voomcounts = rep(0, length(allgenes))
+ voomcounts[voomcountsindex] = 1
+ sink()
+ }
+
+ if (doCamera) {
+ doGSEA(y=DGEList,design=mydesign,histgmt=histgmt,bigmt=bigmt,ntest=20,myTitle=myTitle,
+ outfname=paste(mt,"GSEA.xls",sep="_"),fdrthresh=fdrthresh,fdrtype=fdrtype)
+ }
+
+ if ((doDESeq2==T) || (doVoom==T) || (doedgeR==T)) {
+ if ((doVoom==T) && (doDESeq2==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'Voom,edgeR and DESeq2 overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, DESeq2 = DESeqcounts,
+ VOOM_limma = voomcounts, row.names = allgenes)
+ } else if ((doDESeq2==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'DESeq2 and edgeR overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, DESeq2 = DESeqcounts, row.names = allgenes)
+ } else if ((doVoom==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'Voom and edgeR overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, VOOM_limma = voomcounts, row.names = allgenes)
+ }
+
+ if (nrow(counts.dataframe > 1)) {
+ counts.venn = vennCounts(counts.dataframe)
+ vennf = "Venn_significant_genes_overlap.pdf"
+ pdf(vennf)
+ vennDiagram(counts.venn,main=vennmain,col="maroon")
+ dev.off()
+ }
+ } #### doDESeq2 or doVoom
+
+}
+#### Done
+
+###sink(stdout(),append=T,type="message")
+builtin_gmt = ""
+history_gmt = ""
+history_gmt_name = ""
+out_edgeR = F
+out_DESeq2 = F
+out_VOOM = "$out_VOOM"
+doDESeq2 = $DESeq2.doDESeq2 # make these T or F
+doVoom = $doVoom
+doCamera = F
+doedgeR = $edgeR.doedgeR
+edgeR_priordf = 0
+
+
+#if $doVoom == "T":
+ out_VOOM = "$out_VOOM"
+#end if
+
+#if $DESeq2.doDESeq2 == "T":
+ out_DESeq2 = "$out_DESeq2"
+ DESeq_fitType = "$DESeq2.DESeq_fitType"
+#end if
+
+#if $edgeR.doedgeR == "T":
+ out_edgeR = "$out_edgeR"
+ edgeR_priordf = $edgeR.edgeR_priordf
+#end if
+
+
+
+if (sum(c(doedgeR,doVoom,doDESeq2)) == 0)
+{
+write("No methods chosen - nothing to do! Please try again after choosing one or more methods", stderr())
+quit(save="no",status=2)
+}
+
+Out_Dir = "$html_file.files_path"
+Input = "$input1"
+TreatmentName = "$treatment_name"
+TreatmentCols = "$Treat_cols"
+ControlName = "$control_name"
+ControlCols= "$Control_cols"
+org = "$input1.dbkey"
+if (org == "") { org = "hg19"}
+fdrtype = "$fdrtype"
+fdrthresh = $fdrthresh
+useNDF = $useNDF
+fQ = $fQ # non-differential centile cutoff
+myTitle = "$title"
+sids = strsplit("$subjectids",',')
+subjects = unlist(sids)
+nsubj = length(subjects)
+TCols = as.numeric(strsplit(TreatmentCols,",")[[1]])-1
+CCols = as.numeric(strsplit(ControlCols,",")[[1]])-1
+cat('Got TCols=')
+cat(TCols)
+cat('; CCols=')
+cat(CCols)
+cat('\n')
+useCols = c(TCols,CCols)
+if (file.exists(Out_Dir) == F) dir.create(Out_Dir)
+Count_Matrix = read.table(Input,header=T,row.names=1,sep='\t') #Load tab file assume header
+snames = colnames(Count_Matrix)
+nsamples = length(snames)
+if (nsubj > 0 & nsubj != nsamples) {
+options("show.error.messages"=T)
+mess = paste('Fatal error: Supplied subject id list',paste(subjects,collapse=','),
+ 'has length',nsubj,'but there are',nsamples,'samples',paste(snames,collapse=','))
+write(mess, stderr())
+quit(save="no",status=4)
+}
+if (length(subjects) != 0) {subjects = subjects[useCols]}
+Count_Matrix = Count_Matrix[,useCols] ### reorder columns
+rn = rownames(Count_Matrix)
+islib = rn %in% c('librarySize','NotInBedRegions')
+LibSizes = Count_Matrix[subset(rn,islib),][1] # take first
+Count_Matrix = Count_Matrix[subset(rn,! islib),]
+group = c(rep(TreatmentName,length(TCols)), rep(ControlName,length(CCols)) ) #Build a group descriptor
+group = factor(group, levels=c(ControlName,TreatmentName))
+colnames(Count_Matrix) = paste(group,colnames(Count_Matrix),sep="_") #Relable columns
+results = edgeIt(Count_Matrix=Count_Matrix,group=group, out_edgeR=out_edgeR, out_VOOM=out_VOOM, out_DESeq2=out_DESeq2,
+ fdrtype='BH',mydesign=NULL,priordf=edgeR_priordf,fdrthresh=fdrthresh,outputdir='.',
+ myTitle=myTitle,useNDF=F,libSize=c(),filterquantile=fQ,subjects=subjects,
+ doDESeq2=doDESeq2,doVoom=doVoom,doCamera=doCamera,doedgeR=doedgeR,org=org,
+ histgmt=history_gmt,bigmt=builtin_gmt,DESeq_fitType=DESeq_fitType)
+sessionInfo()
+]]>
+
+
+
+
+**What it does**
+
+Allows short read sequence counts from controlled experiments to be analysed for differentially expressed genes.
+Optionally adds a term for subject if not all samples are independent or if some other factor needs to be blocked in the design.
+
+**Input**
+
+Requires a count matrix as a tabular file. These are best made using the companion HTSeq_ based counter Galaxy wrapper
+and your fave gene model to generate inputs. Each row is a genomic feature (gene or exon eg) and each column the
+non-negative integer count of reads from one sample overlapping the feature.
+The matrix must have a header row uniquely identifying the source samples, and unique row names in
+the first column. Typically the row names are gene symbols or probe ids for downstream use in GSEA and other methods.
+
+**Specifying comparisons**
+
+This is basically dumbed down for two factors - case vs control.
+
+More complex interfaces are possible but painful at present.
+Probably need to specify a phenotype file to do this better.
+Work in progress. Send code.
+
+If you have (eg) paired samples and wish to include a term in the GLM to account for some other factor (subject in the case of paired samples),
+put a comma separated list of indicators for every sample (whether modelled or not!) indicating (eg) the subject number or
+A list of integers, one for each subject or an empty string if samples are all independent.
+If not empty, there must be exactly as many integers in the supplied integer list as there are columns (samples) in the count matrix.
+Integers for samples that are not in the analysis *must* be present in the string as filler even if not used.
+
+So if you have 2 pairs out of 6 samples, you need to put in unique integers for the unpaired ones
+eg if you had 6 samples with the first two independent but the second and third pairs each being from independent subjects. you might use
+8,9,1,1,2,2
+as subject IDs to indicate two paired samples from the same subject in columns 3/4 and 5/6
+
+**Methods available**
+
+You can run 3 popular Bioconductor packages available for count data.
+
+edgeR - see edgeR_ for details
+
+VOOM/limma - see limma_VOOM_ for details
+
+DESeq2 - see DESeq2_ for details
+
+and optionally camera in edgeR which works better if MSigDB is installed.
+
+**Outputs**
+
+Some helpful plots and analysis results. Note that most of these are produced using R code
+suggested by the excellent documentation and vignettes for the Bioconductor
+packages invoked. The Tool Factory is used to automatically lay these out for you to enjoy.
+
+**Note on Voom**
+
+The voom from limma version 3.16.6 help in R includes this from the authors - but you should read the paper to interpret this method.
+
+This function is intended to process RNA-Seq or ChIP-Seq data prior to linear modelling in limma.
+
+voom is an acronym for mean-variance modelling at the observational level.
+The key concern is to estimate the mean-variance relationship in the data, then use this to compute appropriate weights for each observation.
+Count data almost show non-trivial mean-variance relationships. Raw counts show increasing variance with increasing count size, while log-counts typically show a decreasing mean-variance trend.
+This function estimates the mean-variance trend for log-counts, then assigns a weight to each observation based on its predicted variance.
+The weights are then used in the linear modelling process to adjust for heteroscedasticity.
+
+In an experiment, a count value is observed for each tag in each sample. A tag-wise mean-variance trend is computed using lowess.
+The tag-wise mean is the mean log2 count with an offset of 0.5, across samples for a given tag.
+The tag-wise variance is the quarter-root-variance of normalized log2 counts per million values with an offset of 0.5, across samples for a given tag.
+Tags with zero counts across all samples are not included in the lowess fit. Optional normalization is performed using normalizeBetweenArrays.
+Using fitted values of log2 counts from a linear model fit by lmFit, variances from the mean-variance trend were interpolated for each observation.
+This was carried out by approxfun. Inverse variance weights can be used to correct for mean-variance trend in the count data.
+
+
+Author(s)
+
+Charity Law and Gordon Smyth
+
+References
+
+Law, CW (2013). Precision weights for gene expression analysis. PhD Thesis. University of Melbourne, Australia.
+
+Law, CW, Chen, Y, Shi, W, Smyth, GK (2013). Voom! Precision weights unlock linear model analysis tools for RNA-seq read counts.
+Technical Report 1 May 2013, Bioinformatics Division, Walter and Eliza Hall Institute of Medical Reseach, Melbourne, Australia.
+http://www.statsci.org/smyth/pubs/VoomPreprint.pdf
+
+See Also
+
+A voom case study is given in the edgeR User's Guide.
+
+vooma is a similar function but for microarrays instead of RNA-seq.
+
+
+***old rant on changes to Bioconductor package variable names between versions***
+
+The edgeR authors made a small cosmetic change in the name of one important variable (from p.value to PValue)
+breaking this and all other code that assumed the old name for this variable,
+between edgeR2.4.4 and 2.4.6 (the version for R 2.14 as at the time of writing).
+This means that all code using edgeR is sensitive to the version. I think this was a very unwise thing
+to do because it wasted hours of my time to track down and will similarly cost other edgeR users dearly
+when their old scripts break. This tool currently now works with 2.4.6.
+
+**Note on prior.N**
+
+http://seqanswers.com/forums/showthread.php?t=5591 says:
+
+*prior.n*
+
+The value for prior.n determines the amount of smoothing of tagwise dispersions towards the common dispersion.
+You can think of it as like a "weight" for the common value. (It is actually the weight for the common likelihood
+in the weighted likelihood equation). The larger the value for prior.n, the more smoothing, i.e. the closer your
+tagwise dispersion estimates will be to the common dispersion. If you use a prior.n of 1, then that gives the
+common likelihood the weight of one observation.
+
+In answer to your question, it is a good thing to squeeze the tagwise dispersions towards a common value,
+or else you will be using very unreliable estimates of the dispersion. I would not recommend using the value that
+you obtained from estimateSmoothing()---this is far too small and would result in virtually no moderation
+(squeezing) of the tagwise dispersions. How many samples do you have in your experiment?
+What is the experimental design? If you have few samples (less than 6) then I would suggest a prior.n of at least 10.
+If you have more samples, then the tagwise dispersion estimates will be more reliable,
+so you could consider using a smaller prior.n, although I would hesitate to use a prior.n less than 5.
+
+
+From Bioconductor Digest, Vol 118, Issue 5, Gordon writes:
+
+Dear Dorota,
+
+The important settings are prior.df and trend.
+
+prior.n and prior.df are related through prior.df = prior.n * residual.df,
+and your experiment has residual.df = 36 - 12 = 24. So the old setting of
+prior.n=10 is equivalent for your data to prior.df = 240, a very large
+value. Going the other way, the new setting of prior.df=10 is equivalent
+to prior.n=10/24.
+
+To recover old results with the current software you would use
+
+ estimateTagwiseDisp(object, prior.df=240, trend="none")
+
+To get the new default from old software you would use
+
+ estimateTagwiseDisp(object, prior.n=10/24, trend=TRUE)
+
+Actually the old trend method is equivalent to trend="loess" in the new
+software. You should use plotBCV(object) to see whether a trend is
+required.
+
+Note you could also use
+
+ prior.n = getPriorN(object, prior.df=10)
+
+to map between prior.df and prior.n.
+
+----
+
+**Attributions**
+
+edgeR - edgeR_
+
+VOOM/limma - limma_VOOM_
+
+DESeq2 - DESeq2_ for details
+
+See above for Bioconductor package documentation for packages exposed in Galaxy by this tool and app store package.
+
+Galaxy_ (that's what you are using right now!) for gluing everything together
+
+Otherwise, all code and documentation comprising this tool was written by Ross Lazarus and is
+licensed to you under the LGPL_ like other rgenetics artefacts
+
+.. _LGPL: http://www.gnu.org/copyleft/lesser.html
+.. _HTSeq: http://www-huber.embl.de/users/anders/HTSeq/doc/index.html
+.. _edgeR: http://www.bioconductor.org/packages/release/bioc/html/edgeR.html
+.. _DESeq2: http://www.bioconductor.org/packages/release/bioc/html/DESeq2.html
+.. _limma_VOOM: http://www.bioconductor.org/packages/release/bioc/html/limma.html
+.. _Galaxy: http://getgalaxy.org
+
+
+
+
+
diff -r 21b218a7429f -r 0de946608423 rgedgeRpaired_nocamera.xml
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/rgedgeRpaired_nocamera.xml Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,1069 @@
+
+ models using BioConductor packages
+
+ R
+ graphicsmagick
+ ghostscript
+ biocbasics
+
+
+
+ rgToolFactory.py --script_path "$runme" --interpreter "Rscript" --tool_name "Differential_Counts"
+ --output_dir "$html_file.files_path" --output_html "$html_file" --make_HTML "yes"
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+ Do not run edgeR
+ Run edgeR
+
+
+
+
+ Use ordinary deviance estimates
+ Use robust deviance estimates
+ use Anscombe robust deviance estimates
+
+
+
+
+
+
+ Do not run DESeq2
+ Run DESeq2
+
+
+
+ Parametric (default) fit for dispersions
+ Local fit - this will automagically be used if parametric fit fails
+ Mean dispersion fit- use this if you really understand what you're doing - read the fine manual linked below in the documentation
+
+
+
+
+
+ Do not run VOOM
+ Run VOOM
+
+
+
+ fdr
+ Benjamini Hochberg
+ Benjamini Yukateli
+ Bonferroni
+ Hochberg
+ Holm
+ Hommel
+ no control for multiple tests
+
+
+
+
+ edgeR['doedgeR'] == "T"
+
+
+ DESeq2['doDESeq2'] == "T"
+
+
+ doVoom == "T"
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+ nsamp) {
+ dm =dm[1:nsamp,]
+ #sub = paste('Showing',nsamp,'contigs ranked for evidence for differential abundance out of',nprobes,'total')
+ }
+ newcolnames = substr(colnames(dm),1,20)
+ colnames(dm) = newcolnames
+ pdf(outpdfname)
+ heatmap.2(dm,main=myTitle,ColSideColors=pcols,col=topo.colors(100),dendrogram="col",key=T,density.info='none',
+ Rowv=F,scale='row',trace='none',margins=c(8,8),cexRow=0.4,cexCol=0.5)
+ dev.off()
+}
+
+hmap = function(cmat,nmeans=4,outpdfname="heatMap.pdf",nsamp=250,TName='Treatment',group=NA,myTitle="Title goes here")
+{
+ # for 2 groups only was
+ #col.map = function(g) {if (g==TName) "#FF0000" else "#0000FF"}
+ #pcols = unlist(lapply(group,col.map))
+ gu = unique(group)
+ colours = rainbow(length(gu),start=0.3,end=0.6)
+ pcols = colours[match(group,gu)]
+ nrows = nrow(cmat)
+ mtitle = paste(myTitle,'Heatmap: n contigs =',nrows)
+ if (nrows > nsamp) {
+ cmat = cmat[c(1:nsamp),]
+ mtitle = paste('Heatmap: Top ',nsamp,' DE contigs (of ',nrows,')',sep='')
+ }
+ newcolnames = substr(colnames(cmat),1,20)
+ colnames(cmat) = newcolnames
+ pdf(outpdfname)
+ heatmap(cmat,scale='row',main=mtitle,cexRow=0.3,cexCol=0.4,Rowv=NA,ColSideColors=pcols)
+ dev.off()
+}
+
+qqPlot = function(descr='qqplot',pvector, outpdf='qqplot.pdf',...)
+# stolen from https://gist.github.com/703512
+{
+ o = -log10(sort(pvector,decreasing=F))
+ e = -log10( 1:length(o)/length(o) )
+ o[o==-Inf] = reallysmall
+ o[o==Inf] = reallybig
+ maint = descr
+ pdf(outpdf)
+ plot(e,o,pch=19,cex=1, main=maint, ...,
+ xlab=expression(Expected~~-log[10](italic(p))),
+ ylab=expression(Observed~~-log[10](italic(p))),
+ xlim=c(0,max(e)), ylim=c(0,max(o)))
+ lines(e,e,col="red")
+ grid(col = "lightgray", lty = "dotted")
+ dev.off()
+}
+
+smearPlot = function(myDGEList,deTags, outSmear, outMain)
+ {
+ pdf(outSmear)
+ plotSmear(myDGEList,de.tags=deTags,main=outMain)
+ grid(col="lightgray", lty="dotted")
+ dev.off()
+ }
+
+boxPlot = function(rawrs,cleanrs,maint,myTitle,pdfname)
+{
+ nc = ncol(rawrs)
+ ##### for (i in c(1:nc)) {rawrs[(rawrs[,i] < 0),i] = NA}
+ fullnames = colnames(rawrs)
+ newcolnames = substr(colnames(rawrs),1,20)
+ colnames(rawrs) = newcolnames
+ newcolnames = substr(colnames(cleanrs),1,20)
+ colnames(cleanrs) = newcolnames
+ defpar = par(no.readonly=T)
+ print.noquote('@@@ Raw contig counts by sample:')
+ print.noquote(summary(rawrs))
+ print.noquote('@@@ Library size contig counts by sample:')
+ print.noquote(summary(cleanrs))
+ pdf(pdfname)
+ par(mfrow=c(1,2))
+ boxplot(rawrs,varwidth=T,notch=T,ylab='log contig count',col="maroon",las=3,cex.axis=0.35,main='log2 raw counts')
+ grid(col="lightgray",lty="dotted")
+ boxplot(cleanrs,varwidth=T,notch=T,ylab='log contig count',col="maroon",las=3,cex.axis=0.35,main=paste('log2 counts after ',maint))
+ grid(col="lightgray",lty="dotted")
+ dev.off()
+ pdfname = "sample_counts_histogram.pdf"
+ nc = ncol(rawrs)
+ print.noquote(paste('Using ncol rawrs=',nc))
+ ncroot = round(sqrt(nc))
+ if (ncroot*ncroot < nc) { ncroot = ncroot + 1 }
+ m = c()
+ for (i in c(1:nc)) {
+ rhist = hist(rawrs[,i],breaks=100,plot=F)
+ m = append(m,max(rhist\$counts))
+ }
+ ymax = max(m)
+ ncols = length(fullnames)
+ if (ncols > 20)
+ {
+ scale = 7*ncols/20
+ pdf(pdfname,width=scale,height=scale)
+ } else {
+ pdf(pdfname)
+ }
+ par(mfrow=c(ncroot,ncroot))
+ for (i in c(1:nc)) {
+ hist(rawrs[,i], main=paste("Contig logcount",i), xlab='log raw count', col="maroon",
+ breaks=100,sub=fullnames[i],cex=0.8,ylim=c(0,ymax))
+ }
+ dev.off()
+ par(defpar)
+
+}
+
+cumPlot = function(rawrs,cleanrs,maint,myTitle)
+{ # updated to use ecdf
+ pdfname = "Differential_rowsum_bar_charts.pdf"
+ defpar = par(no.readonly=T)
+ lrs = log(rawrs,10)
+ lim = max(lrs)
+ pdf(pdfname)
+ par(mfrow=c(2,1))
+ hist(lrs,breaks=100,main=paste('Before:',maint),xlab="# Reads (log)",
+ ylab="Count",col="maroon",sub=myTitle, xlim=c(0,lim),las=1)
+ grid(col="lightgray", lty="dotted")
+ lrs = log(cleanrs,10)
+ hist(lrs,breaks=100,main=paste('After:',maint),xlab="# Reads (log)",
+ ylab="Count",col="maroon",sub=myTitle,xlim=c(0,lim),las=1)
+ grid(col="lightgray", lty="dotted")
+ dev.off()
+ par(defpar)
+}
+
+cumPlot1 = function(rawrs,cleanrs,maint,myTitle)
+{ # updated to use ecdf
+ pdfname = paste(gsub(" ","", myTitle , fixed=TRUE),"RowsumCum.pdf",sep='_')
+ pdf(pdfname)
+ par(mfrow=c(2,1))
+ lastx = max(rawrs)
+ rawe = knots(ecdf(rawrs))
+ cleane = knots(ecdf(cleanrs))
+ cy = 1:length(cleane)/length(cleane)
+ ry = 1:length(rawe)/length(rawe)
+ plot(rawe,ry,type='l',main=paste('Before',maint),xlab="Log Contig Total Reads",
+ ylab="Cumulative proportion",col="maroon",log='x',xlim=c(1,lastx),sub=myTitle)
+ grid(col="blue")
+ plot(cleane,cy,type='l',main=paste('After',maint),xlab="Log Contig Total Reads",
+ ylab="Cumulative proportion",col="maroon",log='x',xlim=c(1,lastx),sub=myTitle)
+ grid(col="blue")
+ dev.off()
+}
+
+
+
+doGSEAold = function(y=NULL,design=NULL,histgmt="",
+ bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ ntest=0, myTitle="myTitle", outfname="GSEA.xls", minnin=5, maxnin=2000,fdrthresh=0.05,fdrtype="BH")
+{
+ sink('Camera.log')
+ genesets = c()
+ if (bigmt > "")
+ {
+ bigenesets = readLines(bigmt)
+ genesets = bigenesets
+ }
+ if (histgmt > "")
+ {
+ hgenesets = readLines(histgmt)
+ if (bigmt > "") {
+ genesets = rbind(genesets,hgenesets)
+ } else {
+ genesets = hgenesets
+ } # use only history if no bi
+ }
+ print.noquote(paste("@@@read",length(genesets), 'genesets from',histgmt,bigmt))
+ genesets = strsplit(genesets,'\t') # tabular. genesetid\tURLorwhatever\tgene_1\t..\tgene_n
+ outf = outfname
+ head=paste(myTitle,'edgeR GSEA')
+ write(head,file=outfname,append=F)
+ ntest=length(genesets)
+ urownames = toupper(rownames(y))
+ upcam = c()
+ downcam = c()
+ for (i in 1:ntest) {
+ gs = unlist(genesets[i])
+ g = gs[1] # geneset_id
+ u = gs[2]
+ if (u > "") { u = paste("",u," ",sep="") }
+ glist = gs[3:length(gs)] # member gene symbols
+ glist = toupper(glist)
+ inglist = urownames %in% glist
+ nin = sum(inglist)
+ if ((nin > minnin) && (nin < maxnin)) {
+ ### print(paste('@@found',sum(inglist),'genes in glist'))
+ camres = camera(y=y,index=inglist,design=design)
+ if (! is.null(camres)) {
+ rownames(camres) = g # gene set name
+ camres = cbind(GeneSet=g,URL=u,camres)
+ if (camres\$Direction == "Up")
+ {
+ upcam = rbind(upcam,camres) } else {
+ downcam = rbind(downcam,camres)
+ }
+ }
+ }
+ }
+ uscam = upcam[order(upcam\$PValue),]
+ unadjp = uscam\$PValue
+ uscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ nup = max(10,sum((uscam\$adjPValue < fdrthresh)))
+ dscam = downcam[order(downcam\$PValue),]
+ unadjp = dscam\$PValue
+ dscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ ndown = max(10,sum((dscam\$adjPValue < fdrthresh)))
+ write.table(uscam,file=paste('camera_up',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ write.table(dscam,file=paste('camera_down',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera up top',nup,'gene sets:'))
+ write.table(head(uscam,nup),file="",quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera down top',ndown,'gene sets:'))
+ write.table(head(dscam,ndown),file="",quote=F,sep='\t',row.names=F)
+ sink()
+}
+
+
+
+
+doGSEA = function(y=NULL,design=NULL,histgmt="",
+ bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ ntest=0, myTitle="myTitle", outfname="GSEA.xls", minnin=5, maxnin=2000,fdrthresh=0.05,fdrtype="BH")
+{
+ sink('Camera.log')
+ genesets = c()
+ if (bigmt > "")
+ {
+ bigenesets = readLines(bigmt)
+ genesets = bigenesets
+ }
+ if (histgmt > "")
+ {
+ hgenesets = readLines(histgmt)
+ if (bigmt > "") {
+ genesets = rbind(genesets,hgenesets)
+ } else {
+ genesets = hgenesets
+ } # use only history if no bi
+ }
+ print.noquote(paste("@@@read",length(genesets), 'genesets from',histgmt,bigmt))
+ genesets = strsplit(genesets,'\t') # tabular. genesetid\tURLorwhatever\tgene_1\t..\tgene_n
+ outf = outfname
+ head=paste(myTitle,'edgeR GSEA')
+ write(head,file=outfname,append=F)
+ ntest=length(genesets)
+ urownames = toupper(rownames(y))
+ upcam = c()
+ downcam = c()
+ incam = c()
+ urls = c()
+ gsids = c()
+ for (i in 1:ntest) {
+ gs = unlist(genesets[i])
+ gsid = gs[1] # geneset_id
+ url = gs[2]
+ if (url > "") { url = paste("",url," ",sep="") }
+ glist = gs[3:length(gs)] # member gene symbols
+ glist = toupper(glist)
+ inglist = urownames %in% glist
+ nin = sum(inglist)
+ if ((nin > minnin) && (nin < maxnin)) {
+ incam = c(incam,inglist)
+ gsids = c(gsids,gsid)
+ urls = c(urls,url)
+ }
+ }
+ incam = as.list(incam)
+ names(incam) = gsids
+ allcam = camera(y=y,index=incam,design=design)
+ allcamres = cbind(geneset=gsids,allcam,URL=urls)
+ for (i in 1:ntest) {
+ camres = allcamres[i]
+ res = try(test = (camres\$Direction == "Up"))
+ if ("try-error" %in% class(res)) {
+ cat("test failed, camres = :")
+ print.noquote(camres)
+ } else { if (camres\$Direction == "Up")
+ { upcam = rbind(upcam,camres)
+ } else { downcam = rbind(downcam,camres)
+ }
+
+ }
+ }
+ uscam = upcam[order(upcam\$PValue),]
+ unadjp = uscam\$PValue
+ uscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ nup = max(10,sum((uscam\$adjPValue < fdrthresh)))
+ dscam = downcam[order(downcam\$PValue),]
+ unadjp = dscam\$PValue
+ dscam\$adjPValue = p.adjust(unadjp,method=fdrtype)
+ ndown = max(10,sum((dscam\$adjPValue < fdrthresh)))
+ write.table(uscam,file=paste('camera_up',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ write.table(dscam,file=paste('camera_down',outfname,sep='_'),quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera up top',nup,'gene sets:'))
+ write.table(head(uscam,nup),file="",quote=F,sep='\t',row.names=F)
+ print.noquote(paste('@@@@@ Camera down top',ndown,'gene sets:'))
+ write.table(head(dscam,ndown),file="",quote=F,sep='\t',row.names=F)
+ sink()
+ }
+
+
+edgeIt = function (Count_Matrix=c(),group=c(),out_edgeR=F,out_Voom=F,out_DESeq2=F,fdrtype='fdr',priordf=5,
+ fdrthresh=0.05,outputdir='.', myTitle='Differential Counts',libSize=c(),useNDF=F,
+ filterquantile=0.2, subjects=c(),TreatmentName="Rx",ControlName="Ctrl",mydesign=NULL,
+ doDESeq2=T,doVoom=T,doCamera=T,doedgeR=T,org='hg19',
+ histgmt="", bigmt="/data/genomes/gsea/3.1/Abetterchoice_nocgp_c2_c3_c5_symbols_all.gmt",
+ doCook=F,DESeq_fitType="parameteric",robust_meth='ordinary')
+{
+
+logf = file('Differential.log', open = "a")
+sink(logf,type = c("output", "message"))
+
+
+run_edgeR = function(workCM,pdata,subjects,group,priordf,robust_meth,mydesign,mt,cmrowsums,out_edgeR,nonzerod)
+{
+ logf = file('edgeR.log', open = "a")
+ sink(logf,type = c("output", "message"))
+ #### Setup myDGEList object
+ myDGEList = DGEList(counts=workCM, group = group)
+ myDGEList = calcNormFactors(myDGEList)
+ if (robust_meth == 'ordinary') {
+ myDGEList = estimateGLMCommonDisp(myDGEList,mydesign)
+ myDGEList = estimateGLMTrendedDisp(myDGEList,mydesign)
+ if (priordf > 0) { myDGEList = estimateGLMTagwiseDisp(myDGEList,mydesign,prior.df = priordf)
+ } else { myDGEList = estimateGLMTagwiseDisp(myDGEList,mydesign) }
+ comdisp = myDGEList\$common.dispersion
+ estpriorn = getPriorN(myDGEList)
+ print(paste("Common Dispersion =",comdisp,"CV = ",sqrt(comdisp),"getPriorN = ",estpriorn),quote=F)
+ } else {
+ myDGEList = estimateGLMRobustDisp(myDGEList,design=mydesign, prior.df = priordf, maxit = 6, residual.type = robust_meth)
+ }
+
+
+ DGLM = glmFit(myDGEList,design=mydesign)
+ DE = glmLRT(DGLM,coef=ncol(DGLM\$design)) # always last one - subject is first if needed
+ normData = cpm(myDGEList)
+ uoutput = cbind(
+ Name=as.character(rownames(myDGEList\$counts)),
+ DE\$table,
+ adj.p.value=p.adjust(DE\$table\$PValue, method=fdrtype),
+ Dispersion=myDGEList\$tagwise.dispersion,totreads=cmrowsums,normData,
+ myDGEList\$counts
+ )
+ soutput = uoutput[order(DE\$table\$PValue),] # sorted into p value order - for quick toptable
+ goodness = gof(DGLM, pcutoff=fdrthresh)
+ if (sum(goodness\$outlier) > 0) {
+ print.noquote('GLM outliers:')
+ print(paste(rownames(DGLM)[(goodness\$outlier)],collapse=','),quote=F)
+ } else {
+ print('No GLM fit outlier genes found\n')
+ }
+ z = limma::zscoreGamma(goodness\$gof.statistic, shape=goodness\$df/2, scale=2)
+ pdf(paste("edgeR",mt,"GoodnessofFit.pdf",sep='_'))
+ qq = qqnorm(z, panel.first=grid(), main="tagwise dispersion")
+ abline(0,1,lwd=3)
+ points(qq\$x[goodness\$outlier],qq\$y[goodness\$outlier], pch=16, col="maroon")
+ dev.off()
+ uniqueg = unique(group)
+ write.table(soutput,file=out_edgeR, quote=FALSE, sep="\t",row.names=F)
+ tt = cbind(
+ Name=as.character(rownames(myDGEList)),
+ DE\$table,
+ adj.p.value=p.adjust(DE\$table\$PValue, method=fdrtype),
+ Dispersion=myDGEList\$tagwise.dispersion,totreads=cmrowsums
+ )
+ tt = cbind(tt,URL=contigurls) # add to end so table isn't laid out strangely
+ stt = tt[order(DE\$table\$PValue),]
+ print.noquote("@@ edgeR Top tags\n")
+ print.noquote(stt[1:50,])
+ deTags = rownames(uoutput[uoutput\$adj.p.value < fdrthresh,])
+ nsig = length(deTags)
+ print.noquote(paste('@@',nsig,'tags significant at adj p=',fdrthresh))
+ deColours = ifelse(deTags,'red','black')
+ pdf(paste("edgeR",mt,"BCV_vs_abundance.pdf",sep="_"))
+ plotBCV(myDGEList, cex=0.3, main="Biological CV vs abundance")
+ dev.off()
+ dg = myDGEList[order(DE\$table\$PValue),]
+ outpdfname= paste("edgeR",mt,"top_100_heatmap.pdf",sep="_")
+ ocpm = normData[order(DE\$table\$PValue),]
+ ocpm = ocpm[c(1:100),]
+ hmap2(ocpm,TName=TName,group=group,outpdfname=outpdfname,myTitle=paste(myTitle,'Heatmap'))
+ outSmear = paste("edgeR",mt,"smearplot.pdf",sep="_")
+ outMain = paste("Smear Plot for ",TName,' Vs ',CName,' (FDR@',fdrthresh,' N = ',nsig,')',sep='')
+ smearPlot(myDGEList=myDGEList,deTags=deTags, outSmear=outSmear, outMain = outMain)
+ qqPlot(descr=paste(myTitle,'edgeR adj p QQ plot'),pvector=tt\$adj.p.value,outpdf=paste('edgeR',mt,'qqplot.pdf',sep='_'))
+ topresults.edgeR = soutput[which(soutput\$adj.p.value < fdrthresh), ]
+ edgeRcountsindex = which(allgenes %in% rownames(topresults.edgeR))
+ edgeRcounts = rep(0, length(allgenes))
+ edgeRcounts[edgeRcountsindex] = 1 # Create venn diagram of hits
+ sink()
+ return(list(myDGEList=myDGEList,edgeRcounts=edgeRcounts))
+} ### run_edgeR
+
+
+run_DESeq2 = function(workCM,pdata,subjects,group,out_DESeq2,mt,DESeq_fitType)
+
+ {
+ logf = file("DESeq2.log", open = "a")
+ sink(logf,type = c("output", "message"))
+ # DESeq2
+ require('DESeq2')
+ library('RColorBrewer')
+ if (length(subjects) == 0)
+ {
+ pdata = data.frame(Name=colnames(workCM),Rx=group,row.names=colnames(workCM))
+ deSEQds = DESeqDataSetFromMatrix(countData = workCM, colData = pdata, design = formula(~ Rx))
+ } else {
+ pdata = data.frame(Name=colnames(workCM),Rx=group,subjects=subjects,row.names=colnames(workCM))
+ deSEQds = DESeqDataSetFromMatrix(countData = workCM, colData = pdata, design = formula(~ subjects + Rx))
+ }
+ deSeqDatsizefac = estimateSizeFactors(deSEQds)
+ deSeqDatdisp = estimateDispersions(deSeqDatsizefac,fitType=DESeq_fitType)
+ resDESeq = nbinomWaldTest(deSeqDatdisp)
+ rDESeq = as.data.frame(results(resDESeq))
+ rDESeq = cbind(Contig=rownames(workCM),rDESeq,NReads=cmrowsums,URL=contigurls)
+ srDESeq = rDESeq[order(rDESeq\$pvalue),]
+ qqPlot(descr=paste(myTitle,'DESeq2 adj p qq plot'),pvector=rDESeq\$padj,outpdf=paste('DESeq2',mt,'qqplot.pdf',sep="_"))
+ cat("# DESeq top 50\n")
+ print.noquote(srDESeq[1:50,])
+ write.table(srDESeq,file=out_DESeq2, quote=FALSE, sep="\t",row.names=F)
+ topresults.DESeq = rDESeq[which(rDESeq\$padj < fdrthresh), ]
+ DESeqcountsindex = which(allgenes %in% rownames(topresults.DESeq))
+ DESeqcounts = rep(0, length(allgenes))
+ DESeqcounts[DESeqcountsindex] = 1
+ pdf(paste("DESeq2",mt,"dispersion_estimates.pdf",sep='_'))
+ plotDispEsts(resDESeq)
+ dev.off()
+ ysmall = abs(min(rDESeq\$log2FoldChange))
+ ybig = abs(max(rDESeq\$log2FoldChange))
+ ylimit = min(4,ysmall,ybig)
+ pdf(paste("DESeq2",mt,"MA_plot.pdf",sep="_"))
+ plotMA(resDESeq,main=paste(myTitle,"DESeq2 MA plot"),ylim=c(-ylimit,ylimit))
+ dev.off()
+ rlogres = rlogTransformation(resDESeq)
+ sampledists = dist( t( assay(rlogres) ) )
+ sdmat = as.matrix(sampledists)
+ pdf(paste("DESeq2",mt,"sample_distance_plot.pdf",sep="_"))
+ heatmap.2(sdmat,trace="none",main=paste(myTitle,"DESeq2 sample distances"),
+ col = colorRampPalette( rev(brewer.pal(9, "RdBu")) )(255))
+ dev.off()
+ result = try( (ppca = plotPCA( varianceStabilizingTransformation(deSeqDatdisp,blind=T), intgroup=c("Rx","Name")) ) )
+ if ("try-error" %in% class(result)) {
+ print.noquote('DESeq2 plotPCA failed.')
+ } else {
+ pdf(paste("DESeq2",mt,"PCA_plot.pdf",sep="_"))
+ #### wtf - print? Seems needed to get this to work
+ print(ppca)
+ dev.off()
+ }
+ sink()
+ return(DESeqcounts)
+ }
+
+
+run_Voom = function(workCM,pdata,subjects,group,mydesign,mt,out_Voom)
+ {
+ logf = file('VOOM.log', open = "a")
+ sink(logf,type = c("output", "message"))
+ if (doedgeR == F) {
+ #### Setup myDGEList object
+ myDGEList = DGEList(counts=workCM, group = group)
+ myDGEList = calcNormFactors(myDGEList)
+ myDGEList = estimateGLMCommonDisp(myDGEList,mydesign)
+ myDGEList = estimateGLMTrendedDisp(myDGEList,mydesign)
+ myDGEList = estimateGLMTagwiseDisp(myDGEList,mydesign)
+ }
+ pdf(paste("VOOM",mt,"mean_variance_plot.pdf",sep='_'))
+ dat.voomed <- voom(myDGEList, mydesign, plot = TRUE, normalize.method="quantil", lib.size = NULL)
+ dev.off()
+ # Use limma to fit data
+ fit = lmFit(dat.voomed, mydesign)
+ fit = eBayes(fit)
+ rvoom = topTable(fit, coef = length(colnames(mydesign)), adj = fdrtype, n = Inf, sort="none")
+ qqPlot(descr=paste(myTitle,'VOOM-limma adj p QQ plot'),pvector=rvoom\$adj.P.Val,outpdf=paste('VOOM',mt,'qqplot.pdf',sep='_'))
+ rownames(rvoom) = rownames(workCM)
+ rvoom = cbind(Contig=rownames(workCM),rvoom,NReads=cmrowsums,URL=contigurls)
+ srvoom = rvoom[order(rvoom\$P.Value),]
+ cat("# VOOM top 50\n")
+ print(srvoom[1:50,])
+ write.table(srvoom,file=out_Voom, quote=FALSE, sep="\t",row.names=F)
+ # Use an FDR cutoff to find interesting samples for edgeR, DESeq and voom/limma
+ topresults.voom = rvoom[which(rvoom\$adj.P.Val < fdrthresh), ]
+ voomcountsindex <- which(allgenes %in% rownames(topresults.voom))
+ voomcounts = rep(0, length(allgenes))
+ voomcounts[voomcountsindex] = 1
+ sink()
+ return(voomcounts)
+ }
+
+
+#### data cleaning and analsis control starts here
+
+
+ # Error handling
+ nugroup = length(unique(group))
+ if (nugroup!=2){
+ print("Number of conditions identified in experiment does not equal 2")
+ q()
+ }
+ require(edgeR)
+ options(width = 512)
+ mt = paste(unlist(strsplit(myTitle,'_')),collapse=" ")
+ allN = nrow(Count_Matrix)
+ nscut = round(ncol(Count_Matrix)/2) # half samples
+ colTotmillionreads = colSums(Count_Matrix)/1e6
+ counts.dataframe = as.data.frame(c())
+ rawrs = rowSums(Count_Matrix)
+ nonzerod = Count_Matrix[(rawrs > 0),] # remove all zero count genes
+ nzN = nrow(nonzerod)
+ nzrs = rowSums(nonzerod)
+ zN = allN - nzN
+ print('@@@ Quantiles for non-zero row counts:',quote=F)
+ print(quantile(nzrs,probs=seq(0,1,0.1)),quote=F)
+ if (useNDF == T)
+ {
+ gt1rpin3 = rowSums(Count_Matrix/expandAsMatrix(colTotmillionreads,dim(Count_Matrix)) >= 1) >= nscut
+ lo = colSums(Count_Matrix[!gt1rpin3,])
+ workCM = Count_Matrix[gt1rpin3,]
+ cleanrs = rowSums(workCM)
+ cleanN = length(cleanrs)
+ meth = paste( "After removing",length(lo),"contigs with fewer than ",nscut," sample read counts >= 1 per million, there are",sep="")
+ print(paste("Read",allN,"contigs. Removed",zN,"contigs with no reads.",meth,cleanN,"contigs"),quote=F)
+ maint = paste('Filter >=1/million reads in >=',nscut,'samples')
+ } else {
+ useme = (nzrs > quantile(nzrs,filterquantile))
+ workCM = nonzerod[useme,]
+ lo = colSums(nonzerod[!useme,])
+ cleanrs = rowSums(workCM)
+ cleanN = length(cleanrs)
+ meth = paste("After filtering at count quantile =",filterquantile,", there are",sep="")
+ print(paste('Read',allN,"contigs. Removed",zN,"with no reads.",meth,cleanN,"contigs"),quote=F)
+ maint = paste('Filter below',filterquantile,'quantile')
+ }
+ cumPlot(rawrs=rawrs,cleanrs=cleanrs,maint=maint,myTitle=myTitle)
+ allgenes = rownames(workCM)
+ reg = "^chr([0-9]+):([0-9]+)-([0-9]+)" # ucsc chr:start-end regexp
+ genecards=" 0.8) # is ucsc style string
+ {
+ print("@@ using ucsc substitution for urls")
+ contigurls = paste0(ucsc,"&position=chr",testreg[,2],":",testreg[,3],"-",testreg[,4],"\'>",allgenes," ")
+ } else {
+ print("@@ using genecards substitution for urls")
+ contigurls = paste0(genecards,allgenes,"\'>",allgenes,"")
+ }
+ print.noquote(paste("@@ Total low count contigs per sample = ",paste(table(lo),collapse=',')))
+ cmrowsums = rowSums(workCM)
+ TName=unique(group)[1]
+ CName=unique(group)[2]
+ if (is.null(mydesign)) {
+ if (length(subjects) == 0)
+ {
+ mydesign = model.matrix(~group)
+ }
+ else {
+ subjf = factor(subjects)
+ mydesign = model.matrix(~subjf+group) # we block on subject so make group last to simplify finding it
+ }
+ }
+ print.noquote(paste('Using samples:',paste(colnames(workCM),collapse=',')))
+ print.noquote('Using design matrix:')
+ print.noquote(mydesign)
+ normData = cpm(workCM)*1e6
+ colnames(normData) = paste( colnames(workCM),'N',sep="_")
+ print(paste('Raw sample read totals',paste(colSums(nonzerod,na.rm=T),collapse=',')))
+
+ if (doedgeR == T) {
+ eres = run_edgeR(workCM,pdata,subjects,group,priordf,robust_meth,mydesign,mt,cmrowsums,out_edgeR,nonzerod)
+ myDGEList = eres\$myDGEList
+ edgeRcounts = eres\$edgeRcounts
+ #### Plot MDS
+ sample_colors = match(group,levels(group))
+ sampleTypes = levels(factor(group))
+ print.noquote(sampleTypes)
+ pdf(paste("edgeR",mt,"MDSplot.pdf",sep='_'))
+ plotMDS.DGEList(myDGEList,main=paste("MDS for",myTitle),cex=0.5,col=sample_colors,pch=sample_colors)
+ legend(x="topleft", legend = sampleTypes,col=c(1:length(sampleTypes)), pch=19)
+ grid(col="blue")
+ dev.off()
+ scale <- myDGEList\$samples\$lib.size*myDGEList\$samples\$norm.factors
+ normCounts <- round(t(t(myDGEList\$counts)/scale)*mean(scale))
+ try({boxPlot(rawrs=nzd,cleanrs=log2(normCounts+1),maint='Effects of TMM size normalisation',myTitle=myTitle,pdfname=paste("edgeR",mt,"raw_norm_counts_box.pdf",sep='_'))},T)
+ }
+ if (doDESeq2 == T) { DESeqcounts = run_DESeq2(workCM,pdata,subjects,group,out_DESeq2,mt,DESeq_fitType) }
+ if (doVoom == T) { voomcounts = run_Voom(workCM,pdata,subjects,group,mydesign,mt,out_Voom) }
+
+
+ if (doCamera) {
+ doGSEA(y=myDGEList,design=mydesign,histgmt=histgmt,bigmt=bigmt,ntest=20,myTitle=myTitle,
+ outfname=paste("GSEA_Camera",mt,"table.xls",sep="_"),fdrthresh=fdrthresh,fdrtype=fdrtype)
+ }
+ counts.dataframe = c()
+ vennmain = 'no venn'
+ if ((doDESeq2==T) || (doVoom==T) || (doedgeR==T)) {
+ if ((doVoom==T) && (doDESeq2==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'Voom,edgeR and DESeq2 overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, DESeq2 = DESeqcounts,
+ VOOM_limma = voomcounts, row.names = allgenes)
+ } else if ((doDESeq2==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'DESeq2 and edgeR overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, DESeq2 = DESeqcounts, row.names = allgenes)
+ } else if ((doVoom==T) && (doedgeR==T)) {
+ vennmain = paste(mt,'Voom and edgeR overlap at FDR=',fdrthresh)
+ counts.dataframe = data.frame(edgeR = edgeRcounts, VOOM_limma = voomcounts, row.names = allgenes)
+ }
+
+ if (nrow(counts.dataframe > 1)) {
+ counts.venn = vennCounts(counts.dataframe)
+ vennf = paste("Differential_venn",mt,"significant_genes_overlap.pdf",sep="_")
+ pdf(vennf)
+ vennDiagram(counts.venn,main=vennmain,col="maroon")
+ dev.off()
+ }
+ } #### doDESeq2 or doVoom
+sink()
+}
+#### Done
+]]>
+builtin_gmt = ""
+history_gmt = ""
+history_gmt_name = ""
+out_edgeR = F
+out_DESeq2 = F
+out_Voom = "$out_VOOM"
+edgeR_robust_meth = "ordinary"
+doDESeq2 = $DESeq2.doDESeq2
+doVoom = $doVoom
+doCamera = F
+doedgeR = $edgeR.doedgeR
+edgeR_priordf = 10
+
+
+#if $doVoom == "T":
+ out_Voom = "$out_VOOM"
+#end if
+
+#if $DESeq2.doDESeq2 == "T":
+ out_DESeq2 = "$out_DESeq2"
+ doDESeq2 = T
+ DESeq_fitType = "$DESeq2.DESeq_fitType"
+#end if
+
+#if $edgeR.doedgeR == "T":
+ out_edgeR = "$out_edgeR"
+ edgeR_priordf = $edgeR.edgeR_priordf
+ edgeR_robust_meth = "$edgeR.edgeR_robust_method"
+#end if
+
+
+if (sum(c(doedgeR,doVoom,doDESeq2)) == 0)
+{
+write("No methods chosen - nothing to do! Please try again after choosing one or more methods", stderr())
+quit(save="no",status=2)
+}
+
+Out_Dir = "$html_file.files_path"
+Input = "$input1"
+TreatmentName = "$treatment_name"
+TreatmentCols = "$Treat_cols"
+ControlName = "$control_name"
+ControlCols= "$Control_cols"
+org = "$input1.dbkey"
+if (org == "") { org = "hg19"}
+fdrtype = "$fdrtype"
+fdrthresh = $fdrthresh
+useNDF = $useNDF
+fQ = $fQ # non-differential centile cutoff
+myTitle = "$title"
+sids = strsplit("$subjectids",',')
+subjects = unlist(sids)
+nsubj = length(subjects)
+TCols = as.numeric(strsplit(TreatmentCols,",")[[1]])-1
+CCols = as.numeric(strsplit(ControlCols,",")[[1]])-1
+cat('Got TCols=')
+cat(TCols)
+cat('; CCols=')
+cat(CCols)
+cat('\n')
+ 0 & nsubj != nsamples) {
+options("show.error.messages"=T)
+mess = paste('Fatal error: Supplied subject id list',paste(subjects,collapse=','),
+ 'has length',nsubj,'but there are',nsamples,'samples',paste(snames,collapse=','))
+write(mess, stderr())
+quit(save="no",status=4)
+}
+if (length(subjects) != 0) {subjects = subjects[useCols]}
+Count_Matrix = Count_Matrix[,useCols] ### reorder columns
+rn = rownames(Count_Matrix)
+islib = rn %in% c('librarySize','NotInBedRegions')
+LibSizes = Count_Matrix[subset(rn,islib),][1] # take first
+Count_Matrix = Count_Matrix[subset(rn,! islib),]
+group = c(rep(TreatmentName,length(TCols)), rep(ControlName,length(CCols)) )
+group = factor(group, levels=c(ControlName,TreatmentName))
+colnames(Count_Matrix) = paste(group,colnames(Count_Matrix),sep="_")
+results = edgeIt(Count_Matrix=Count_Matrix,group=group, out_edgeR=out_edgeR, out_Voom=out_Voom, out_DESeq2=out_DESeq2,
+ fdrtype='BH',mydesign=NULL,priordf=edgeR_priordf,fdrthresh=fdrthresh,outputdir='.',
+ myTitle=myTitle,useNDF=F,libSize=c(),filterquantile=fQ,subjects=subjects,TreatmentName=TreatmentName,ControlName=ControlName,
+ doDESeq2=doDESeq2,doVoom=doVoom,doCamera=doCamera,doedgeR=doedgeR,org=org,
+ histgmt=history_gmt,bigmt=builtin_gmt,DESeq_fitType=DESeq_fitType,robust_meth=edgeR_robust_meth)
+sessionInfo()
+
+sink()
+]]>
+
+
+
+
+**What it does**
+
+Allows short read sequence counts from controlled experiments to be analysed for differentially expressed genes.
+Optionally adds a term for subject if not all samples are independent or if some other factor needs to be blocked in the design.
+
+**Input**
+
+Requires a count matrix as a tabular file. These are best made using the companion HTSeq_ based counter Galaxy wrapper
+and your fave gene model to generate inputs. Each row is a genomic feature (gene or exon eg) and each column the
+non-negative integer count of reads from one sample overlapping the feature.
+
+The matrix must have a header row uniquely identifying the source samples, and unique row names in
+the first column. Typically the row names are gene symbols or probe ids for downstream use in GSEA and other methods.
+They must be unique and R names or they will be mangled - please read the fine R docs for the rules on identifiers.
+
+**Specifying comparisons**
+
+This is basically dumbed down for two factors - case vs control.
+
+More complex interfaces are possible but painful at present.
+Probably need to specify a phenotype file to do this better.
+Work in progress. Send code.
+
+If you have (eg) paired samples and wish to include a term in the GLM to account for some other factor (subject in the case of paired samples),
+put a comma separated list of indicators for every sample (whether modelled or not!) indicating (eg) the subject number or
+A list of integers, one for each subject or an empty string if samples are all independent.
+If not empty, there must be exactly as many integers in the supplied integer list as there are columns (samples) in the count matrix.
+Integers for samples that are not in the analysis *must* be present in the string as filler even if not used.
+
+So if you have 2 pairs out of 6 samples, you need to put in unique integers for the unpaired ones
+eg if you had 6 samples with the first two independent but the second and third pairs each being from independent subjects. you might use
+8,9,1,1,2,2
+as subject IDs to indicate two paired samples from the same subject in columns 3/4 and 5/6
+
+**Methods available**
+
+You can run 3 popular Bioconductor packages available for count data.
+
+edgeR - see edgeR_ for details
+
+VOOM/limma - see limma_VOOM_ for details
+
+DESeq2 - see DESeq2_ for details
+
+and optionally camera in edgeR which works better if MSigDB is installed.
+
+**Outputs**
+
+Some helpful plots and analysis results. Note that most of these are produced using R code
+suggested by the excellent documentation and vignettes for the Bioconductor
+packages invoked. The Tool Factory is used to automatically lay these out for you to enjoy.
+
+**Note on Voom**
+
+The voom from limma version 3.16.6 help in R includes this from the authors - but you should read the paper to interpret this method.
+
+This function is intended to process RNA-Seq or ChIP-Seq data prior to linear modelling in limma.
+
+voom is an acronym for mean-variance modelling at the observational level.
+The key concern is to estimate the mean-variance relationship in the data, then use this to compute appropriate weights for each observation.
+Count data almost show non-trivial mean-variance relationships. Raw counts show increasing variance with increasing count size, while log-counts typically show a decreasing mean-variance trend.
+This function estimates the mean-variance trend for log-counts, then assigns a weight to each observation based on its predicted variance.
+The weights are then used in the linear modelling process to adjust for heteroscedasticity.
+
+In an experiment, a count value is observed for each tag in each sample. A tag-wise mean-variance trend is computed using lowess.
+The tag-wise mean is the mean log2 count with an offset of 0.5, across samples for a given tag.
+The tag-wise variance is the quarter-root-variance of normalized log2 counts per million values with an offset of 0.5, across samples for a given tag.
+Tags with zero counts across all samples are not included in the lowess fit. Optional normalization is performed using normalizeBetweenArrays.
+Using fitted values of log2 counts from a linear model fit by lmFit, variances from the mean-variance trend were interpolated for each observation.
+This was carried out by approxfun. Inverse variance weights can be used to correct for mean-variance trend in the count data.
+
+
+Author(s)
+
+Charity Law and Gordon Smyth
+
+References
+
+Law, CW (2013). Precision weights for gene expression analysis. PhD Thesis. University of Melbourne, Australia.
+
+Law, CW, Chen, Y, Shi, W, Smyth, GK (2013). Voom! Precision weights unlock linear model analysis tools for RNA-seq read counts.
+Technical Report 1 May 2013, Bioinformatics Division, Walter and Eliza Hall Institute of Medical Reseach, Melbourne, Australia.
+http://www.statsci.org/smyth/pubs/VoomPreprint.pdf
+
+See Also
+
+A voom case study is given in the edgeR User's Guide.
+
+vooma is a similar function but for microarrays instead of RNA-seq.
+
+
+***old rant on changes to Bioconductor package variable names between versions***
+
+The edgeR authors made a small cosmetic change in the name of one important variable (from p.value to PValue)
+breaking this and all other code that assumed the old name for this variable,
+between edgeR2.4.4 and 2.4.6 (the version for R 2.14 as at the time of writing).
+This means that all code using edgeR is sensitive to the version. I think this was a very unwise thing
+to do because it wasted hours of my time to track down and will similarly cost other edgeR users dearly
+when their old scripts break. This tool currently now works with 2.4.6.
+
+**Note on prior.N**
+
+http://seqanswers.com/forums/showthread.php?t=5591 says:
+
+*prior.n*
+
+The value for prior.n determines the amount of smoothing of tagwise dispersions towards the common dispersion.
+You can think of it as like a "weight" for the common value. (It is actually the weight for the common likelihood
+in the weighted likelihood equation). The larger the value for prior.n, the more smoothing, i.e. the closer your
+tagwise dispersion estimates will be to the common dispersion. If you use a prior.n of 1, then that gives the
+common likelihood the weight of one observation.
+
+In answer to your question, it is a good thing to squeeze the tagwise dispersions towards a common value,
+or else you will be using very unreliable estimates of the dispersion. I would not recommend using the value that
+you obtained from estimateSmoothing()---this is far too small and would result in virtually no moderation
+(squeezing) of the tagwise dispersions. How many samples do you have in your experiment?
+What is the experimental design? If you have few samples (less than 6) then I would suggest a prior.n of at least 10.
+If you have more samples, then the tagwise dispersion estimates will be more reliable,
+so you could consider using a smaller prior.n, although I would hesitate to use a prior.n less than 5.
+
+
+From Bioconductor Digest, Vol 118, Issue 5, Gordon writes:
+
+Dear Dorota,
+
+The important settings are prior.df and trend.
+
+prior.n and prior.df are related through prior.df = prior.n * residual.df,
+and your experiment has residual.df = 36 - 12 = 24. So the old setting of
+prior.n=10 is equivalent for your data to prior.df = 240, a very large
+value. Going the other way, the new setting of prior.df=10 is equivalent
+to prior.n=10/24.
+
+To recover old results with the current software you would use
+
+ estimateTagwiseDisp(object, prior.df=240, trend="none")
+
+To get the new default from old software you would use
+
+ estimateTagwiseDisp(object, prior.n=10/24, trend=TRUE)
+
+Actually the old trend method is equivalent to trend="loess" in the new
+software. You should use plotBCV(object) to see whether a trend is
+required.
+
+Note you could also use
+
+ prior.n = getPriorN(object, prior.df=10)
+
+to map between prior.df and prior.n.
+
+----
+
+**Attributions**
+
+edgeR - edgeR_
+
+VOOM/limma - limma_VOOM_
+
+DESeq2 - DESeq2_ for details
+
+See above for Bioconductor package documentation for packages exposed in Galaxy by this tool and app store package.
+
+Galaxy_ (that's what you are using right now!) for gluing everything together
+
+Otherwise, all code and documentation comprising this tool was written by Ross Lazarus and is
+licensed to you under the LGPL_ like other rgenetics artefacts
+
+.. _LGPL: http://www.gnu.org/copyleft/lesser.html
+.. _HTSeq: http://www-huber.embl.de/users/anders/HTSeq/doc/index.html
+.. _edgeR: http://www.bioconductor.org/packages/release/bioc/html/edgeR.html
+.. _DESeq2: http://www.bioconductor.org/packages/release/bioc/html/DESeq2.html
+.. _limma_VOOM: http://www.bioconductor.org/packages/release/bioc/html/limma.html
+.. _Galaxy: http://getgalaxy.org
+
+
+
+
+
diff -r 21b218a7429f -r 0de946608423 test-data/edgeRtest1out.html
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/edgeRtest1out.html Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,621 @@
+
+
+
+
+
+
+
+
+
+
+
Galaxy Tool "Differential_Counts" run at 28/12/2014 21:02:37
+
DESeq2 images and outputs
+(Click on a thumbnail image to download the corresponding original PDF image)
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
DESeq2 log output
+
+
+
+# DESeq top 50
+
+ Contig baseMean log2FoldChange lfcSE stat pvalue padj NReads URL
+
+Mir192 Mir192 271352.97636 6.965264 0.2150593 32.387646 4.096935e-230 3.818343e-227 2325567 Mir192
+
+Mir122a Mir122a 10112.31117 10.312083 0.3292695 31.318061 2.649329e-215 1.234587e-212 90428 Mir122a
+
+Mir149 Mir149 810.35429 -6.911118 0.2341392 -29.517132 1.735536e-191 5.391733e-189 6164 Mir149
+
+Mir23a Mir23a 1289.18043 -3.104086 0.1191688 -26.047815 1.424245e-149 3.318491e-147 10118 Mir23a
+
+Mir181d Mir181d 275.22797 -3.581172 0.1778187 -20.139461 3.329373e-90 6.205952e-88 2139 Mir181d
+
+Mir204 Mir204 347.57397 -7.284200 0.3771119 -19.315751 3.959346e-83 6.150183e-81 2601 Mir204
+
+Mir23b Mir23b 2028.55377 -2.065110 0.1085802 -19.019217 1.182361e-80 1.574229e-78 16387 Mir23b
+
+Mir27a Mir27a 2788.72629 -3.016676 0.1688167 -17.869539 2.036708e-71 2.372765e-69 21886 Mir27a
+
+Mir195 Mir195 519.86200 -3.152795 0.1784796 -17.664734 7.838131e-70 8.116820e-68 3962 Mir195
+
+Mir194-2 Mir194-2 391.65678 5.222911 0.3099275 16.852045 1.013492e-63 9.445744e-62 3570 Mir194-2
+
+Mir208b Mir208b 1649.77924 -11.396172 0.6771238 -16.830264 1.464482e-63 1.240816e-61 14756 Mir208b
+
+Mir10b Mir10b 27820.40551 -5.071453 0.3044884 -16.655656 2.753110e-62 2.138249e-60 197340 Mir10b
+
+Mir181c Mir181c 2765.96510 -3.660964 0.2275711 -16.087120 3.141152e-58 2.251965e-56 23605 Mir181c
+
+Mir208a Mir208a 616.76981 -10.356524 0.6559218 -15.789267 3.688391e-56 2.455415e-54 4638 Mir208a
+
+Mir490 Mir490 220.99790 -8.059660 0.5142876 -15.671504 2.369067e-55 1.471980e-53 1741 Mir490
+
+Mir203 Mir203 772.92882 1.990849 0.1274099 15.625546 4.877239e-55 2.840992e-53 6739 Mir203
+
+Mir215 Mir215 152.78082 -3.004380 0.1939090 -15.493765 3.822341e-54 2.095542e-52 1182 Mir215
+
+Dnm3os Dnm3os 179.61643 -3.278392 0.2166491 -15.132265 9.922045e-52 5.137415e-50 1401 Dnm3os
+
+Mir214 Mir214 134.69038 -3.216444 0.2154916 -14.926074 2.230149e-50 1.093947e-48 1048 Mir214
+
+Mir21 Mir21 26121.31011 2.963903 0.2008617 14.755939 2.817433e-49 1.312924e-47 229120 Mir21
+
+Mir1948 Mir1948 263.89527 7.074045 0.4867226 14.534039 7.374076e-48 3.272685e-46 2404 Mir1948
+
+Mir27b Mir27b 76478.05753 -1.904653 0.1312889 -14.507339 1.088626e-47 4.611815e-46 625308 Mir27b
+
+Rabggtb Rabggtb 2257.19195 1.988368 0.1401741 14.184987 1.134862e-45 4.598659e-44 19535 Rabggtb
+
+Mir499 Mir499 712.45950 -10.577061 0.7528467 -14.049423 7.766426e-45 3.015962e-43 6527 Mir499
+
+Mir101b Mir101b 6846.19683 3.791681 0.2809666 13.495132 1.670548e-41 6.227801e-40 59019 Mir101b
+
+Mir132 Mir132 106.46062 -2.797928 0.2083376 -13.429779 4.046171e-41 1.450397e-39 857 Mir132
+
+Mir143hg Mir143hg 180217.77425 -2.169143 0.1685614 -12.868566 6.764677e-38 2.335066e-36 1407364 Mir143hg
+
+Mir143 Mir143 179219.35960 -2.170303 0.1696199 -12.795094 1.746402e-37 5.813025e-36 1399819 Mir143
+
+Mir155 Mir155 57.66182 -3.788079 0.3056585 -12.393175 2.845516e-35 9.144898e-34 463 Mir155
+
+Mir322 Mir322 899.53469 -3.126011 0.2622596 -11.919531 9.363380e-33 2.908890e-31 7074 Mir322
+
+Mir378 Mir378 483.21548 -2.994300 0.2577321 -11.617876 3.343461e-31 1.005195e-29 4075 Mir378
+
+Mir24-2 Mir24-2 424.48288 -2.712674 0.2361028 -11.489378 1.491830e-30 4.213289e-29 3470 Mir24-2
+
+Mir3074-2 Mir3074-2 424.48288 -2.712674 0.2361028 -11.489378 1.491830e-30 4.213289e-29 3470 Mir3074-2
+
+Mir199b Mir199b 47.84725 -5.294373 0.4644474 -11.399295 4.215163e-30 1.155451e-28 370 Mir199b
+
+Mir802 Mir802 166.83414 8.816580 0.7782636 11.328527 9.478530e-30 2.523997e-28 1514 Mir802
+
+Mir125b-2 Mir125b-2 493.08516 -2.919341 0.2631193 -11.095122 1.324798e-28 3.429754e-27 3837 Mir125b-2
+
+Mir301 Mir301 260.53406 -1.676984 0.1526772 -10.983852 4.570133e-28 1.151179e-26 2119 Mir301
+
+Snord104 Snord104 3851.90119 2.386573 0.2173857 10.978522 4.847915e-28 1.189015e-26 33458 Snord104
+
+Mir150 Mir150 553.20599 -2.836881 0.2595088 -10.931734 8.127991e-28 1.942381e-26 4229 Mir150
+
+Mir148a Mir148a 118994.46955 2.678852 0.2481801 10.793984 3.675045e-27 8.562855e-26 1002397 Mir148a
+
+5430416N02Rik 5430416N02Rik 62.15966 3.089960 0.2941123 10.506053 8.101331e-26 1.841571e-24 564 5430416N02Rik
+
+Mir193 Mir193 45.70861 4.991530 0.4814098 10.368568 3.446495e-25 7.647936e-24 421 Mir193
+
+Mir3073 Mir3073 98.93199 8.208709 0.7944742 10.332254 5.036321e-25 1.091593e-23 904 Mir3073
+
+Mir125b-1 Mir125b-1 79.01988 -3.020660 0.2937360 -10.283590 8.355635e-25 1.769875e-23 609 Mir125b-1
+
+2610203C20Rik 2610203C20Rik 79.17666 -3.023491 0.2948614 -10.253939 1.136165e-24 2.353124e-23 610 2610203C20Rik
+
+Mir181a-1 Mir181a-1 59.53826 -3.151487 0.3211628 -9.812740 9.923710e-23 2.010630e-21 506 Mir181a-1
+
+Mir184 Mir184 32.23796 -4.865023 0.4962776 -9.803028 1.092606e-22 2.166615e-21 247 Mir184
+
+Mir199a-2 Mir199a-2 44.84878 -3.422216 0.3545647 -9.651880 4.826276e-22 9.371019e-21 352 Mir199a-2
+
+Mir182 Mir182 886.79583 4.919630 0.5101689 9.643140 5.255515e-22 9.996204e-21 7189 Mir182
+
+Snord91a Snord91a 168.95251 2.700421 0.2835464 9.523738 1.670595e-21 3.113990e-20 1437 Snord91a
+
+
+
+
+
Differential images and outputs
+(Click on a thumbnail image to download the corresponding original PDF image)
+
+
+
+
+
+
+
+
+
+
Differential log output
+
+
+
+[1] @@@ Quantiles for non-zero row counts:
+
+ 0% 10% 20% 30% 40% 50% 60% 70% 80% 90% 100%
+
+ 1.0 1.0 2.0 3.0 4.0 8.0 13.0 24.0 86.6 753.0 2325567.0
+
+[1] Read 3242 contigs. Removed 1494 with no reads. After filtering at count quantile =0.3, there are 1141 contigs
+
+[1] "@@ using genecards substitution for urls"
+
+[1] @@ Total low count contigs per sample = 1,1,1,1,1,1,1,1
+
+[1] Using samples: liver_X11706Liv_CAAAAG_L003_R1_001_trimmed.fastq_bwa.sam.bam,liver_X11700Liv_ATTCCT_L003_R1_001_trimmed.fastq_bwa.sam.bam,liver_X11698Liv_ACTGAT_L003_R1_001_trimmed.fastq_bwa.sam.bam,liver_X11699Liv_ATGAGC_L003_R1_001_trimmed.fastq_bwa.sam.bam,heart_X11706He_AGTTCC_L001_R1_001_trimmed.fastq_bwa.sam.bam,heart_X11699He_GGCTAC_L001_R1_001_trimmed.fastq_bwa.sam.bam,heart_X11698He_TAGCTT_L001_R1_001_trimmed.fastq_bwa.sam.bam,heart_X11700He_CTTGTA_L001_R1_001_trimmed.fastq_bwa.sam.bam
+
+[1] Using design matrix:
+
+ (Intercept) groupliver
+
+1 1 1
+
+2 1 1
+
+3 1 1
+
+4 1 1
+
+5 1 0
+
+6 1 0
+
+7 1 0
+
+8 1 0
+
+attr(,"assign")
+
+[1] 0 1
+
+attr(,"contrasts")
+
+attr(,"contrasts")$group
+
+[1] contr.treatment
+
+[1] "Raw sample read totals 2443751,1644652,1682104,1806045,1440960,1341813,2888924,1428365"
+
+[1] heart liver
+
+
+
+
+
Differential log output
+
+
+
+Attaching package: ‘gplots’
+
+The following object is masked from ‘package:stats’:
+
+ lowess
+
+Loading required package: methods
+
+Loading required package: limma
+
+Loading required package: splines
+
+Loading required package: DESeq2
+
+Loading required package: GenomicRanges
+
+Loading required package: BiocGenerics
+
+Loading required package: parallel
+
+Attaching package: ‘BiocGenerics’
+
+The following objects are masked from ‘package:parallel’:
+
+ clusterApply, clusterApplyLB, clusterCall, clusterEvalQ, clusterExport, clusterMap, parApply, parCapply, parLapply, parLapplyLB, parRapply, parSapply, parSapplyLB
+
+The following object is masked from ‘package:limma’:
+
+ plotMA
+
+The following object is masked from ‘package:stats’:
+
+ xtabs
+
+The following objects are masked from ‘package:base’:
+
+ anyDuplicated, append, as.data.frame, as.vector, cbind, colnames, duplicated, eval, evalq, Filter, Find, get, intersect, is.unsorted, lapply, Map, mapply, match, mget, order, paste, pmax, pmax.int, pmin, pmin.int, Position, rank, rbind, Reduce, rep.int, rownames, sapply, setdiff, sort, table, tapply, union, unique, unlist
+
+Loading required package: IRanges
+
+Attaching package: ‘IRanges’
+
+The following object is masked from ‘package:gplots’:
+
+ space
+
+Loading required package: XVector
+
+Loading required package: Rcpp
+
+Loading required package: RcppArmadillo
+
+gene-wise dispersion estimates
+
+mean-dispersion relationship
+
+final dispersion estimates
+
+you had estimated gene-wise dispersions, removing these
+
+you had estimated fitted dispersions, removing these
+
+you had estimated gene-wise dispersions, removing these
+
+you had estimated fitted dispersions, removing these
+
+Warning message:
+
+closing unused connection 4 (edgeR.log)
+
+Warning message:
+
+In sink() : no sink to remove
+
+
+
+
+
VOOM images and outputs
+(Click on a thumbnail image to download the corresponding original PDF image)
+
+
+
+
+
+
+
+
+
+
VOOM log output
+
+
+
+# VOOM top 50
+
+ Contig logFC AveExpr t P.Value adj.P.Val B NReads URL
+
+Mir192 Mir192 6.689950 14.4417888 50.335160 1.802287e-16 2.056409e-13 27.414844 2325567 Mir192
+
+Mir208a Mir208a -10.458438 3.8918506 -29.183545 2.249812e-13 1.283518e-10 19.141041 4638 Mir208a
+
+Mir3073 Mir3073 8.318578 2.6485638 25.821264 1.102217e-12 4.192097e-10 18.063600 904 Mir3073
+
+Mir802 Mir802 8.992449 2.9857711 25.195575 1.514327e-12 4.319618e-10 17.906674 1514 Mir802
+
+Mir208b Mir208b -12.256447 4.4678897 -22.360114 7.074494e-12 1.614400e-09 16.920424 14756 Mir208b
+
+Mir499 Mir499 -11.104485 3.8066799 -21.990054 8.769804e-12 1.667724e-09 16.728874 6527 Mir499
+
+Mir10b Mir10b -4.775768 12.4173688 -21.487387 1.180685e-11 1.924516e-09 17.249348 197340 Mir10b
+
+Mir148a Mir148a 2.751538 15.4237642 20.289553 2.464883e-11 3.515539e-09 16.455471 1002397 Mir148a
+
+Mir490 Mir490 -8.497742 3.6613221 -18.336110 8.980482e-11 1.138526e-08 13.923237 1741 Mir490
+
+Mir122a Mir122a 10.197963 8.1512374 17.467826 1.663427e-10 1.897970e-08 14.215445 90428 Mir122a
+
+Mir133b Mir133b -6.172367 1.3497975 -17.274094 1.916064e-10 1.987481e-08 13.840201 159 Mir133b
+
+Mir149 Mir149 -7.041176 6.0886889 -16.861286 2.602547e-10 2.474589e-08 13.714880 6164 Mir149
+
+Mir101b Mir101b 3.837883 10.6216725 15.443054 7.873164e-10 6.910215e-08 13.054350 59019 Mir101b
+
+Mir143 Mir143 -1.912927 16.0353646 -14.922755 1.209475e-09 9.857220e-08 12.374988 1399819 Mir143
+
+Mir194-2 Mir194-2 5.534694 6.2627211 14.703097 1.455682e-09 1.107289e-07 12.316769 3570 Mir194-2
+
+Mir23a Mir23a -2.905961 8.6431895 -14.558394 1.646894e-09 1.174441e-07 12.339306 10118 Mir23a
+
+Mir1983 Mir1983 -5.612359 1.1061384 -14.266537 2.119488e-09 1.422551e-07 11.743589 101 Mir1983
+
+Mir27a Mir27a -2.849084 10.0939084 -14.158498 2.329669e-09 1.476752e-07 11.960195 21886 Mir27a
+
+Cyp3a25 Cyp3a25 6.312461 1.6425308 13.845627 3.074630e-09 1.846396e-07 11.502713 226 Cyp3a25
+
+Mir200a Mir200a 6.129125 1.8320913 13.226966 5.410979e-09 3.086963e-07 10.979834 264 Mir200a
+
+Mir181d Mir181d -3.405544 6.3702152 -13.064584 6.300369e-09 3.423201e-07 11.006301 2139 Mir181d
+
+Mir153 Mir153 -5.698257 1.5328802 -12.832092 7.856705e-09 3.829623e-07 10.583835 140 Mir153
+
+Mir204 Mir204 -7.718081 4.5031856 -12.808496 8.036265e-09 3.829623e-07 10.353229 2601 Mir204
+
+Gm5441 Gm5441 -5.716851 1.5430406 -12.806028 8.055298e-09 3.829623e-07 10.562881 142 Gm5441
+
+Rabggtb Rabggtb 2.327908 9.9369857 12.760291 8.416902e-09 3.841474e-07 10.654006 19535 Rabggtb
+
+Mir504 Mir504 -5.122304 0.8161671 -12.391521 1.205304e-08 5.289430e-07 10.144865 69 Mir504
+
+Mir133a-1 Mir133a-1 -4.912497 0.7297882 -12.335045 1.274466e-08 5.385801e-07 10.076395 60 Mir133a-1
+
+Mir195 Mir195 -2.954216 7.3530970 -12.081859 1.641098e-08 6.603731e-07 10.055879 3962 Mir195
+
+Mir27b Mir27b -1.496991 14.9464877 -12.059553 1.678424e-08 6.603731e-07 9.674850 625308 Mir27b
+
+Snord52 Snord52 2.631712 9.7652181 11.922618 1.928407e-08 7.334374e-07 9.811774 18059 Snord52
+
+Mir322 Mir322 -3.029558 8.1188344 -11.736839 2.333148e-08 8.587488e-07 9.679815 7074 Mir322
+
+Mir181c Mir181c -3.676262 9.6244506 -11.575598 2.758358e-08 9.835271e-07 9.453057 23605 Mir181c
+
+Mir1948 Mir1948 7.101780 4.7821564 11.471202 3.077353e-08 1.033009e-06 9.233632 2404 Mir1948
+
+0610031O16Rik 0610031O16Rik 4.519875 0.7388871 11.470939 3.078205e-08 1.033009e-06 9.284014 78 0610031O16Rik
+
+Mir201 Mir201 -4.964105 0.7490919 -11.289794 3.729283e-08 1.210650e-06 9.114028 63 Mir201
+
+Mir21 Mir21 2.746616 13.2835800 11.267331 3.819755e-08 1.210650e-06 8.925217 229120 Mir21
+
+Mir184 Mir184 -5.569565 2.3521173 -11.190343 4.148052e-08 1.279170e-06 8.854599 247 Mir184
+
+1810019D21Rik 1810019D21Rik 5.164581 1.0784751 11.082009 4.662057e-08 1.399844e-06 8.951908 117 1810019D21Rik
+
+Mir203 Mir203 2.216791 8.5426169 10.866758 5.896538e-08 1.725115e-06 8.715639 6739 Mir203
+
+1110038B12Rik 1110038B12Rik 2.383720 10.6847245 10.832157 6.125623e-08 1.744094e-06 8.573067 37066 1110038B12Rik
+
+Snord104 Snord104 2.571210 10.4798167 10.811468 6.267120e-08 1.744094e-06 8.561110 33458 Snord104
+
+Mir182 Mir182 5.196800 7.2088299 10.640454 7.579543e-08 2.021320e-06 8.545839 7189 Mir182
+
+Mir547 Mir547 -4.542934 0.5799793 -10.635980 7.617593e-08 2.021320e-06 8.435473 42 Mir547
+
+Mir143hg Mir143hg -2.291921 16.3789153 -10.597275 7.955395e-08 2.062978e-06 7.952584 1407364 Mir143hg
+
+Scnn1b Scnn1b -4.541403 0.5700621 -10.243065 1.190487e-07 3.018546e-06 8.023327 45 Scnn1b
+
+Mir125b-2 Mir125b-2 -2.896115 7.2737925 -10.091091 1.420082e-07 3.522420e-06 7.876068 3837 Mir125b-2
+
+Mir1a-1 Mir1a-1 -4.402568 0.4498447 -9.950346 1.675164e-07 4.066729e-06 7.692790 42 Mir1a-1
+
+Mir378 Mir378 -2.733247 7.2964165 -9.922980 1.730212e-07 4.112858e-06 7.672216 4075 Mir378
+
+Mir199b Mir199b -5.651345 2.8029895 -9.883978 1.812024e-07 4.219426e-06 7.548022 370 Mir199b
+
+Mir155 Mir155 -4.158272 3.8002361 -9.845490 1.896814e-07 4.328530e-06 7.604112 463 Mir155
+
+
+
+
+
edgeR images and outputs
+(Click on a thumbnail image to download the corresponding original PDF image)
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
+
edgeR log output
+
+
+
+[1] Common Dispersion = 0.228651460998105 CV = 0.478175136323613 getPriorN = 3.33333333333333
+
+[1] "No GLM fit outlier genes found\n"
+
+[1] @@ edgeR Top tags\n
+
+ Name logFC logCPM LR PValue adj.p.value Dispersion totreads URL
+
+Mir208a Mir208a -11.840751 8.465017 594.16946 3.104543e-131 3.542284e-128 0.05171220 4638 Mir208a
+
+Mir149 Mir149 -7.008984 8.861767 484.30321 2.473909e-107 1.411365e-104 0.04959937 6164 Mir149
+
+Mir208b Mir208b -13.291635 9.905945 417.69758 7.737463e-93 2.942815e-90 0.10508096 14756 Mir208b
+
+Mir122a Mir122a 10.514683 12.478088 415.17429 2.740525e-92 7.817349e-90 0.10803882 90428 Mir122a
+
+Mir204 Mir204 -7.498162 7.634507 341.30678 3.313430e-76 7.561247e-74 0.06907958 2601 Mir204
+
+Mir499 Mir499 -13.577454 8.700078 325.79199 7.930755e-73 1.508165e-70 0.12042284 6527 Mir499
+
+Mir490 Mir490 -8.534394 6.991023 303.17184 6.710366e-68 1.093790e-65 0.07949711 1741 Mir490
+
+Mir192 Mir192 6.953853 17.169364 217.22867 3.638307e-49 5.189135e-47 0.12700995 2325567 Mir192
+
+Mir802 Mir802 11.440805 6.593380 212.88059 3.231644e-48 4.097007e-46 0.12273671 1514 Mir802
+
+Mir1948 Mir1948 7.418142 7.252734 195.66958 1.840248e-44 2.099723e-42 0.12060221 2404 Mir1948
+
+Mir194-2 Mir194-2 5.298950 7.811522 191.85588 1.250960e-43 1.297587e-41 0.08670751 3570 Mir194-2
+
+Mir23a Mir23a -3.153807 9.529402 177.53185 1.676248e-40 1.593833e-38 0.04442763 10118 Mir23a
+
+Mir181c Mir181c -3.767686 10.639598 169.87390 7.883295e-39 6.919107e-37 0.06368883 23605 Mir181c
+
+Mir3073 Mir3073 10.686337 5.859950 164.86740 9.778593e-38 7.969554e-36 0.14069249 904 Mir3073
+
+Mir181d Mir181d -3.643963 7.300371 162.18591 3.767663e-37 2.865936e-35 0.05729574 2139 Mir181d
+
+Mir195 Mir195 -3.203683 8.215089 150.20548 1.563314e-34 1.114838e-32 0.05235020 3962 Mir195
+
+Mir10b Mir10b -5.182616 13.946466 147.24793 6.926819e-34 4.649118e-32 0.12268790 197340 Mir10b
+
+Mir101b Mir101b 3.759962 11.863187 136.31359 1.703812e-31 1.080028e-29 0.07961343 59019 Mir101b
+
+Mir378 Mir378 -3.115599 8.119617 126.76408 2.092233e-29 1.256441e-27 0.05942391 4075 Mir378
+
+Mir27a Mir27a -3.064687 10.642480 124.98911 5.117477e-29 2.919520e-27 0.06113852 21886 Mir27a
+
+Mir182 Mir182 5.057509 8.846381 123.17765 1.275060e-28 6.927826e-27 0.13653707 7189 Mir182
+
+Mir322 Mir322 -3.194159 9.012888 107.34926 3.732413e-25 1.935765e-23 0.07536483 7074 Mir322
+
+Mir199b Mir199b -5.520119 4.792610 102.10724 5.259607e-24 2.609223e-22 0.13417024 370 Mir199b
+
+Mir181a-2 Mir181a-2 -3.000177 7.637692 101.38361 7.578821e-24 3.603098e-22 0.06896654 2817 Mir181a-2
+
+Mir125b-2 Mir125b-2 -2.987759 8.144514 91.72544 9.957640e-22 4.488356e-20 0.07737381 3837 Mir125b-2
+
+Dnm3os Dnm3os -3.331215 6.686950 91.67250 1.022763e-21 4.488356e-20 0.08810497 1401 Dnm3os
+
+Mir184 Mir184 -5.111350 4.234160 84.35542 4.133639e-20 1.686711e-18 0.13502324 247 Mir184
+
+Mir215 Mir215 -3.058208 6.447966 84.35278 4.139167e-20 1.686711e-18 0.08138517 1182 Mir215
+
+Mir133b Mir133b -8.383611 3.584760 83.96681 5.031517e-20 1.960318e-18 0.17482280 159 Mir133b
+
+Mir150 Mir150 -2.883446 8.307765 83.91918 5.154210e-20 1.960318e-18 0.08008123 4229 Mir150
+
+Mir3074-2 Mir3074-2 -2.778308 7.935651 83.74839 5.619282e-20 2.040616e-18 0.07424646 3470 Mir3074-2
+
+Mir24-2 Mir24-2 -2.778307 7.935651 83.71222 5.723024e-20 2.040616e-18 0.07427992 3470 Mir24-2
+
+Mir193 Mir193 5.176579 4.801090 83.19222 7.445011e-20 2.574169e-18 0.14794861 421 Mir193
+
+Scarna17 Scarna17 2.182159 9.244479 81.91330 1.421894e-19 4.771710e-18 0.04982909 9224 Scarna17
+
+Mir214 Mir214 -3.271172 6.271755 80.43948 2.997458e-19 9.771712e-18 0.09566584 1048 Mir214
+
+Snord104 Snord104 2.330488 11.053611 79.50529 4.809369e-19 1.524303e-17 0.05915990 33458 Snord104
+
+Mir200a Mir200a 7.201555 4.139422 77.35503 1.428304e-18 4.365755e-17 0.19287764 264 Mir200a
+
+Mir200b Mir200b 6.525423 5.752604 77.31985 1.453976e-18 4.365755e-17 0.26237966 888 Mir200b
+
+Mir21 Mir21 2.923147 13.825255 75.51798 3.620938e-18 1.059357e-16 0.09395834 229120 Mir21
+
+Mir203 Mir203 1.956427 8.767610 75.17870 4.299815e-18 1.226522e-16 0.04381710 6739 Mir203
+
+Mir155 Mir155 -3.886731 5.068563 73.81316 8.587210e-18 2.389758e-16 0.12522673 463 Mir155
+
+Cyp3a25 Cyp3a25 8.681501 3.972085 72.29680 1.851471e-17 5.029829e-16 0.23125383 226 Cyp3a25
+
+Rabggtb Rabggtb 1.934093 10.298211 72.02043 2.129809e-17 5.651422e-16 0.04596646 19535 Rabggtb
+
+Mir23b Mir23b -2.100584 10.184110 71.44225 2.854935e-17 7.403367e-16 0.05416378 16387 Mir23b
+
+Snord52 Snord52 2.207491 10.217554 71.27974 3.100027e-17 7.860292e-16 0.05941483 18059 Snord52
+
+Gm5441 Gm5441 -6.881248 3.538457 70.05615 5.764004e-17 1.429724e-15 0.20097284 142 Gm5441
+
+Mir153 Mir153 -6.857671 3.517446 69.37600 8.137282e-17 1.975455e-15 0.20158808 140 Mir153
+
+Mir132 Mir132 -2.858294 5.938312 64.52507 9.531204e-16 2.265647e-14 0.09274248 857 Mir132
+
+1110038B12Rik 1110038B12Rik 2.195962 11.253090 62.92015 2.152583e-15 5.012443e-14 0.06712174 37066 1110038B12Rik
+
+Snord91a Snord91a 2.654072 6.557504 62.40549 2.795431e-15 6.379174e-14 0.08637410 1437 Snord91a
+
+[1] @@ 416 tags significant at adj p= 0.05
+
+
+
+
+
Other log output
+
+
+
+## Toolfactory generated command line = Rscript - None None
+
+Got TCols=1 5 6 7; CCols=2 3 4 8
+
+R version 3.0.2 (2013-09-25)
+
+Platform: x86_64-pc-linux-gnu (64-bit)
+
+locale:
+
+ [1] LC_CTYPE=en_AU.UTF-8 LC_NUMERIC=C LC_TIME=en_AU.UTF-8 LC_COLLATE=en_AU.UTF-8 LC_MONETARY=en_AU.UTF-8 LC_MESSAGES=en_AU.UTF-8 LC_PAPER=en_AU.UTF-8 LC_NAME=C LC_ADDRESS=C LC_TELEPHONE=C LC_MEASUREMENT=en_AU.UTF-8 LC_IDENTIFICATION=C
+
+attached base packages:
+
+[1] parallel splines methods stats graphics grDevices utils datasets base
+
+other attached packages:
+
+ [1] RColorBrewer_1.0-5 DESeq2_1.2.10 RcppArmadillo_0.4.400.0 Rcpp_0.11.2 GenomicRanges_1.14.4 XVector_0.2.0 IRanges_1.20.7 BiocGenerics_0.8.0 edgeR_3.4.2 limma_3.18.13 gplots_2.15.0 stringr_0.6.2
+
+loaded via a namespace (and not attached):
+
+ [1] annotate_1.40.1 AnnotationDbi_1.24.0 Biobase_2.22.0 bitops_1.0-6 caTools_1.17.1 DBI_0.3.0 gdata_2.13.3 genefilter_1.44.0 grid_3.0.2 gtools_3.4.1 KernSmooth_2.23-13 lattice_0.20-29 locfit_1.5-9.1 RSQLite_0.11.4 stats4_3.0.2 survival_2.37-7 XML_3.98-1.1 xtable_1.7-4
+
+
+
+
+
All output files available for downloading
+
+
+
+
diff -r 21b218a7429f -r 0de946608423 test-data/edgeRtest1out.xls
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/edgeRtest1out.xls Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,1142 @@
+Name logFC logCPM LR PValue adj.p.value Dispersion totreads liver_X11706Liv_CAAAAG_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11700Liv_ATTCCT_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11698Liv_ACTGAT_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11699Liv_ATGAGC_L003_R1_001_trimmed.fastq_bwa.sam.bam heart_X11706He_AGTTCC_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11699He_GGCTAC_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11698He_TAGCTT_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11700He_CTTGTA_L001_R1_001_trimmed.fastq_bwa.sam.bam liver_X11706Liv_CAAAAG_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11700Liv_ATTCCT_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11698Liv_ACTGAT_L003_R1_001_trimmed.fastq_bwa.sam.bam liver_X11699Liv_ATGAGC_L003_R1_001_trimmed.fastq_bwa.sam.bam heart_X11706He_AGTTCC_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11699He_GGCTAC_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11698He_TAGCTT_L001_R1_001_trimmed.fastq_bwa.sam.bam heart_X11700He_CTTGTA_L001_R1_001_trimmed.fastq_bwa.sam.bam
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diff -r 21b218a7429f -r 0de946608423 test-data/gentestdata.sh
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/gentestdata.sh Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,9 @@
+#!/bin/bash
+# generate test data for rgGSEA
+# ross lazarus June 2013
+# adjust gseajar_path !
+GSEAJAR_PATH=/home/rlazarus/galaxy-central/tool_dependency_dir/gsea_jar/2.0.12/fubar/rg_gsea_test/8e291f464aa0/jars/gsea2-2.0.12.jar
+python ../rgGSEA.py --input_tab "gsea_test_DGE.xls" --adjpvalcol "5" --signcol "2" --idcol "1" --outhtml "gseatestout.html" --input_name "gsea_test" --setMax "500" --setMin "15" --nPerm "10" --plotTop "20" --gsea_jar "$GSEAJAR_PATH" --output_dir "gseatestout" --mode "Max_probe"
+--title "GSEA test" --builtin_gmt "gseatestdata.gmt"
+
+
diff -r 21b218a7429f -r 0de946608423 test-data/test_bams2mx.xls
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/test_bams2mx.xls Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,3243 @@
+Contigname 11706Liv_CAAAAG_L003_R1_001_trimmed.fastq_bwa.sam.bam 11706He_AGTTCC_L001_R1_001_trimmed.fastq_bwa.sam.bam 11699He_GGCTAC_L001_R1_001_trimmed.fastq_bwa.sam.bam 11698He_TAGCTT_L001_R1_001_trimmed.fastq_bwa.sam.bam 11700Liv_ATTCCT_L003_R1_001_trimmed.fastq_bwa.sam.bam 11698Liv_ACTGAT_L003_R1_001_trimmed.fastq_bwa.sam.bam 11699Liv_ATGAGC_L003_R1_001_trimmed.fastq_bwa.sam.bam 11700He_CTTGTA_L001_R1_001_trimmed.fastq_bwa.sam.bam
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diff -r 21b218a7429f -r 0de946608423 tool_dependencies.xml
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/tool_dependencies.xml Tue Jan 06 02:20:55 2015 -0500
@@ -0,0 +1,62 @@
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+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/quantreg_5.05.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/nlme_3.1-118.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/polspline_1.1.9.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/mvtnorm_1.0-2.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/TH.data_1.0-5.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/zoo_1.7-11.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/sandwich_2.3-2.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/multcomp_1.3-8.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/rms_4.2-1.tar.gz?raw=true
+ https://github.com/fubar2/galaxy_tool_source/blob/master/RELEASE_2_14/pec_2.4.4.tar.gz?raw=true
+
+
+
+
+
+ Differential gene expression analysis
+ You may need libxml2-dev for XML to compile
+ Ubuntu has a bug with libgfortran. To fix that create a symlink like: sudo ln -s /usr/lib/x86_64-linux-gnu/libgfortran.so.3 /usr/lib/x86_64-linux-gnu/libgfortran.so
+
+
+