Mercurial > repos > bornea > saint_preproc

--- a/saint_preproc/SAINT_preprocessing_v5.xml	Tue Nov 10 13:13:22 2015 -0500
+++ /dev/null	Thu Jan 01 00:00:00 1970 +0000
@@ -1,91 +0,0 @@
-<tool id="SAINT_preprocessing_v5" name="SAINT pre-processing">
-  <description></description>
-  <command interpreter="python">
-    #if (str($type) == 'Scaffold'):
-      SAINT_preprocessing_v6.py $input $preybool $fasta_db $Inter_file $Prey_file
-      "
-        #for $ba in $bait
-         ${ba.bait1}
-         ${ba.assign}
-         ${ba.T_C}
-        #end for
-        "
-      $Bait_file \$INSTALL_RUN_PATH/
-    #elif (str($type) == 'MaxQuant'):
-      SAINT_preprocessing_v6_mq_pep.py $input $preybool $fasta_db $Inter_file $Prey_file
-        "
-        #for $ba in $bait
-          ${ba.bait1}
-          ${ba.assign}
-          ${ba.T_C}
-        #end for
-        "
-      $Bait_file \$INSTALL_RUN_PATH/
-    #end if
-  </command>
-  <requirements>
-    <requirement type="set_environment">INSTALL_RUN_PATH</requirment>
-  </requirments>
-  <inputs>
-    <param type="select" name="type" label="MaxQuant or Scaffold">
-      <option value="MaxQuant">MaxQuant</option>
-      <option value="Scaffold">Scaffold</option>
-    </param>
-    <param format="dat" name="input" type="data" label="Scaffold or MaxQuant proteinGroup Output"/>
-    <param type="boolean" name="preybool" checked="true" label="Create Prey File"/>
-    <param type="data" name="fasta_db" format="fasta"  label="Provide Uniprot Fasta database" />
-    <repeat name="bait" title="Bait Create">
-      <param name="bait1" type="text" size="100"/>
-      <param name="assign" type="text" size="100"/>
-      <param name="T_C" type="boolean" checked="true" label="Is this a Control?"/>
-    </repeat>
-  </inputs>
-  <outputs>
-    <data format="txt" name="Inter_file" label="Inter File"/>
-    <data format="txt" name="Prey_file" label="Prey File" />
-    <data format="txt" name="Bait_file" label="Bait File" />
-  </outputs>
-  <stdio>
-    <regex match="error"
-	   source="stdout"
-           level="fatal"
-           description="Unknown error"/>
-    <regex match="Error: bad bait"
-           source="stdout"
-           level="fatal"
-           description="Error: bad bait"/>
-  </stdio>
-
-  <tests>
-    <test>
-      <param name="input" value="fa_gc_content_input.fa"/>
-      <output name="out_file1" file="fa_gc_content_output.txt"/>
-    </test>
-  </tests>
-  <help>
-Pre-processing:
-APOSTL is able to recognize either a Scaffold "Samples Report" file (tab-delimited
-txt file) or the "peptides.txt" file output in the maxquant "txt" output folder. No
-modifications should be made to these files. Using the "Bait Create" tool, you can
-create your "bait.txt" file. It is important that the individual bait names match the
-bait names within your scaffold or maxquant output. APOSTL uses the bait file to find
-the user's baits of interest. Additionally there is an option to make the prey file (Y/N).
-When making a prey file, APOSTL queries uniprot in order to extract protein amino acid
-lengths and gene names. This takes several minutes depending on your internet connection.
-Some users may want to run SAINTexpress using the same data set while changing which baits
-are considered test or control. It is useful to toggle "Make Prey" off in order to save
-time by circumventing this step as the same prey file can be used for both SAINTexpress
-runs.
-
-INPUTS:
-
-Scaffold file:
-
-- Scaffold "Samples Report" output (tab-delimited txt file)
-
-
-Maxquant file:
-
-- maxquant "peptides.txt" file (tab-delimited txt file)
-  </help>
-</tool>
--- a/saint_preproc/SAINT_preprocessing_v6.py	Tue Nov 10 13:13:22 2015 -0500
+++ /dev/null	Thu Jan 01 00:00:00 1970 +0000
@@ -1,245 +0,0 @@
-#######################################################################################
-# Python-code: SAINT pre-processing from Scaffold "Samples Report" output
-# Author: Brent Kuenzi
-#######################################################################################
-# This program reads in a raw Scaffold "Samples Report" output and a user generated
-# bait file and autoformats it into prey and interaction files for SAINTexpress
-# analysis
-#######################################################################################
-import sys
-import urllib2
-import os.path
-#######################################################################################
-## REQUIRED INPUT ##
-
-# 1) infile: Scaffold "Samples Report" output
-# 2) baitfile: SAINT formatted bait file generated in Galaxy
-# 3) prey: Y or N for generating a prey file (requires internet connection)
-#######################################################################################
-infile = sys.argv[1] #Scaffold "Samples Report" output
-prey = sys.argv[2] # Y or N
-fasta_db = sys.argv[3]
-tool_path = sys.argv[8]
-if fasta_db == "None":
-    fasta_db = str(tool_path)  + "/SwissProt_HUMAN_2014_08.fasta"
-make_bait= sys.argv[5]
-
-
-baits = make_bait.split()
-i = 0
-bait_file_tmp = open("bait.txt", "wr")
-order = []
-bait_cache = []
-
-while i < len(baits):
-    if baits[i+2] == "true":
-        T_C = "C"
-    else:
-        T_C = "T"
-    line1 = baits[i] + "\t" + baits[i+1] + "\t" + T_C + "\n"
-    q = open(infile,"r")
-    for line2 in q:
-        line2 = line2.strip()
-        temp = line2.split('\t')
-        if "Quantitative Variance" in str(temp):
-            if baits[i] in temp:
-                number_bait = temp.index(str(baits[i]))
-                number_bait = number_bait - 9
-                bait_cache.append((number_bait, str(line1)))
-            else:
-                print "Error: bad bait " + str(baits[i])
-                sys.exit()
-        else:
-            pass
-    i = i + 3
-
-bait_cache.sort()
-for line in bait_cache:
-    bait_file_tmp.write(line[1])
-
-bait_file_tmp.close()
-baitfile = "bait.txt"
-
-class ReturnValue1(object):
-    def __init__(self, sequence, gene):
-     self.seqlength = sequence
-     self.genename = gene
-class ReturnValue2(object):
-    def __init__(self, getdata, getproteins, getheader):
-        self.data = getdata
-        self.proteins = getproteins
-        self.header = getheader
-
-def main(scaffold_input, baitfile):
-    bait_check(baitfile, scaffold_input)
-    make_inter(scaffold_input)
-    if prey == 'true':
-        make_prey(scaffold_input)
-        no_error_inter(scaffold_input)
-        os.rename('prey.txt', sys.argv[5])
-    elif prey == 'false':
-        if os.path.isfile('error proteins.txt') == True:
-            no_error_inter(scaffold_input)
-        pass
-    elif prey != 'true' or 'false':
-        sys.exit("Invalid Prey Argument: Y or N")
-
-def get_info(uniprot_accession_in): # get aa lengths and gene name
-    error = open('error proteins.txt', 'a+')
-#    while True:
-#        i = 0
-#	try:
-#            data = urllib2.urlopen("http://www.uniprot.org/uniprot/" + uniprot_accession_in + ".fasta")
-#            break
-#        except urllib2.HTTPError, err:
-#            i = i + 1
-#            if i == 50:
-#                sys.exit("More than 50 errors. Check your file or try again later.")
-#            if err.code == 404:
-#                error.write(uniprot_accession_in + '\t' + "Invalid URL. Check protein" + '\n')
-#                seqlength = 'NA'
-#                genename = 'NA'
-#                return ReturnValue1(seqlength, genename)
-#            elif err.code == 302:
-#                sys.exit("Request timed out. Check connection and try again.")
-#            else:
-#                sys.exit("Uniprot had some other error")
-#    lines = data.readlines()
-#    if lines == []:
-#        error.write(uniprot_accession_in + '\t' + "Blank Fasta" + '\n')
-#        error.close
-#        seqlength = 'NA'
-#        genename = 'NA'
-#        return ReturnValue1(seqlength, genename)
-#    if lines != []:
-#        seqlength = 0
-#        header = lines[0]
-#        for line in lines[1:]:
-#            line = line.replace("\n","") # strip \n or else it gets counted in the length
-#            seqlength += len(line)
-#        if 'GN=' in header:
-#            lst = header.split('GN=')
-#            lst2 = lst[1].split(' ')
-#            genename = lst2[0]
-#            error.close
-#            return ReturnValue1(seqlength, genename)
-#        if 'GN=' not in header:
-#            genename = 'NA'
-#            error.close
-#            return ReturnValue1(seqlength, genename)
-    data = open(fasta_db,'r')
-    lines = data.readlines()
-    db_len = len(lines)
-    seqlength = 0
-    count = 0
-    for i in lines:
-        if ">sp" in i:
-            if uniprot_accession_in == i.split("|")[1]:
-                match = count+1
-                if 'GN=' in i:
-                    lst = i.split('GN=')
-                    lst2 = lst[1].split(' ')
-                    genename = lst2[0]
-                if 'GN=' not in i:
-                    genename = 'NA'
-                while ">sp" not in lines[match]:
-                    if match <= db_len:
-                        seqlength = seqlength + len(lines[match].strip())
-                        match = match + 1
-                    else:
-                        break
-                return ReturnValue1(seqlength, genename)
-        count = count + 1
-
-
-    if seqlength == 0:
-        error.write(uniprot_accession_in + '\t' + "Uniprot not in Fasta" + '\n')
-        error.close
-        seqlength = 'NA'
-        genename = 'NA'
-        return ReturnValue1(seqlength, genename)
-
-def readtab(infile):
-    with open(infile,'r') as x: # read in tab-delim text
-        output = []
-        for line in x:
-            line = line.strip()
-            temp = line.split('\t')
-            output.append(temp)
-    return output
-def read_scaffold(scaffold_input): # Get data, proteins and header from scaffold output
-    dupes = readtab(scaffold_input)
-    cnt = 0
-    for i in dupes:
-        cnt += 1
-        if i[0] == '#': # finds the start of second header
-            header_start = cnt-1
-    header = dupes[header_start]
-    prot_start = header.index("Accession Number")
-    data = dupes[header_start+1:len(dupes)-2] # cut off blank line and END OF FILE
-    proteins = []
-    for i in data:
-        i[4] = i[4].split()[0] # removes the (+##) that sometimes is attached
-    for protein in data:
-        proteins.append(protein[prot_start])
-    return ReturnValue2(data, proteins, header)
-def make_inter(scaffold_input):
-    bait = readtab(baitfile)
-    data = read_scaffold(scaffold_input).data
-    header = read_scaffold(scaffold_input).header
-    proteins = read_scaffold(scaffold_input).proteins
-    bait_index = []
-    for i in bait:
-        bait_index.append(header.index(i[0])) # Find just the baits defined in bait file
-    with open('inter.txt', 'w') as y:
-            a = 0; l=0
-            for bb in bait:
-                for lst in data:
-                    y.write(header[bait_index[l]] + '\t' + bb[1] + '\t' + proteins[a] + '\t' + lst[bait_index[l]] + '\n')
-                    a+=1
-                    if a == len(proteins):
-                        a = 0; l+=1
-def make_prey(scaffold_input):
-    proteins = read_scaffold(scaffold_input).proteins
-    output_file = open("prey.txt",'w')
-    for a in proteins:
-        a = a.replace("\n","") # remove \n for input into function
-        a = a.replace("\r","") # ditto for \r
-        seq = get_info(a).seqlength
-        GN = get_info(a).genename
-        if seq != 'NA':
-            output_file.write(a+"\t"+str(seq)+ "\t" + str(GN) + "\n")
-    output_file.close()
-def no_error_inter(scaffold_input): # remake inter file without protein errors from Uniprot
-    err = readtab("error proteins.txt")
-    bait = readtab(baitfile)
-    data = read_scaffold(scaffold_input).data
-    header = read_scaffold(scaffold_input).header
-    bait_index = []
-    for i in bait:
-        bait_index.append(header.index(i[0]))
-    proteins = read_scaffold(scaffold_input).proteins
-    errors = []
-    for e in err:
-        errors.append(e[0])
-    with open('inter.txt', 'w') as y:
-        l = 0; a = 0
-        for bb in bait:
-            for lst in data:
-                if proteins[a] not in errors:
-                    y.write(header[bait_index[l]] + '\t' + bb[1] + '\t' + proteins[a] + '\t' + lst[bait_index[l]] + '\n')
-                a+=1
-                if a == len(proteins):
-                    l += 1; a = 0
-def bait_check(bait, scaffold_input): # check that bait names share header titles
-    bait_in = readtab(bait)
-    header = read_scaffold(scaffold_input).header
-    for i in bait_in:
-        if i[0] not in header:
-            sys.exit("Bait must share header titles with Scaffold output")
-
-if __name__ == '__main__':
-    main(infile, baitfile)
-
-os.rename('inter.txt', sys.argv[4])
-os.rename("bait.txt", sys.argv[7])
--- a/saint_preproc/SAINT_preprocessing_v6_mq_pep.py	Tue Nov 10 13:13:22 2015 -0500
+++ /dev/null	Thu Jan 01 00:00:00 1970 +0000
@@ -1,262 +0,0 @@
-#######################################################################################
-# Python-code: SAINT pre-processing from maxquant "Samples Report" output
-# Author: Brent Kuenzi
-#######################################################################################
-# This program reads in a raw maxquant "Samples Report" output and a user generated
-# bait file and autoformats it into prey and interaction files for SAINTexpress
-# analysis
-#######################################################################################
-import sys
-import urllib2
-import os
-#######################################################################################
-## REQUIRED INPUT ##
-
-# 1) infile: maxquant "Samples Report" output
-# 2) baitfile: SAINT formatted bait file generated in Galaxy
-# 3) prey: Y or N for generating a prey file (requires internet connection)
-#######################################################################################
-mq_file = sys.argv[1]
-cmd = r"Rscript /home/bornea/galaxy_moffitt_dev/tools/Moffitt_Tools/bubblebeam/pre_process_protein_name_set.R " + str(mq_file)
-os.system(cmd)
-
-infile = "./tukeys_output.txt" #maxquant "Samples Report" output
-prey = sys.argv[2] # Y or N
-fasta_db = sys.argv[3]
-if fasta_db == "None":
-    fasta_db = "/home/bornea/galaxy_moffitt_dev/tools/Moffitt_Tools/bubblebeam/SwissProt_HUMAN_2014_08.fasta"
-make_bait= sys.argv[6]
-
-def bait_create(baits, infile):
-    #Takes the Bait specified by the user and makes them into a Bait file and includes a check to make sure they are using valid baits.
-    baits = make_bait.split()
-    i = 0
-    bait_file_tmp = open("bait.txt", "wr")
-    order = []
-    bait_cache = []
-    while i < len(baits):
-        if baits[i+2] == "true":
-            T_C = "C"
-        else:
-            T_C = "T"
-        line1 = baits[i] + "\t" + baits[i+1] + "\t" + T_C + "\n"
-        q = open(infile,"r")
-        for line2 in q:
-           line2 = line2.replace("\"", "")
-           line2 = line2.replace(r"Intensity.", "") #R coerces "-" into "." this changes them back and remove Intensity from the Bait names.
-           line2 = line2.replace(r".", r"-")
-           temp = line2.split()
-           if "mapped_protein" in str(temp):
-                #If the bait is in the original file then write to cache it if not exit.
-                if baits[i] in temp:
-                    number_bait = temp.index(str(baits[i]))
-                    number_bait = number_bait - 9
-                    bait_cache.append((number_bait, str(line1)))
-                else:
-                    print "Error: bad bait " + str(baits[i])
-                    sys.exit()
-           else:
-                pass
-        i = i + 3
-    #Writes cache to file.
-    bait_cache.sort()
-    for line in bait_cache:
-        bait_file_tmp.write(line[1])
-
-    bait_file_tmp.close()
-
-
-baitfile = "bait.txt"
-
-class ReturnValue1(object):
-    def __init__(self, sequence, gene):
-     self.seqlength = sequence
-     self.genename = gene
-class ReturnValue2(object):
-    def __init__(self, getdata, getproteins, getheader):
-        self.data = getdata
-        self.proteins = getproteins
-        self.header = getheader
-
-def main(maxquant_input, make_bait):
-    bait_create(make_bait, infile)
-    baitfile = "bait.txt"
-    #bait_check(baitfile, maxquant_input)
-    make_inter(maxquant_input)
-    if prey == 'true':
-        make_prey(maxquant_input)
-        no_error_inter(maxquant_input)
-        os.rename('prey.txt', sys.argv[5])
-    elif prey == 'false':
-        if os.path.isfile('error proteins.txt') == True:
-            no_error_inter(maxquant_input)
-        pass
-    elif prey != 'true' or 'false':
-        sys.exit("Invalid Prey Argument: Y or N")
-    os.rename('inter.txt', sys.argv[4])
-    os.rename("bait.txt", sys.argv[7])
-
-
-def get_info(uniprot_accession_in): # get aa lengths and gene name
-    error = open('error proteins.txt', 'a+')
-#    while True:
-#        i = 0
-#	try:
-#            data = urllib2.urlopen("http://www.uniprot.org/uniprot/" + uniprot_accession_in + ".fasta")
-#            break
-#        except urllib2.HTTPError, err:
-#            i = i + 1
-#            if i == 50:
-#                sys.exit("More than 50 errors. Check your file or try again later.")
-#            if err.code == 404:
-#                error.write(uniprot_accession_in + '\t' + "Invalid URL. Check protein" + '\n')
-#                seqlength = 'NA'
-#                genename = 'NA'
-#                return ReturnValue1(seqlength, genename)
-#            elif err.code == 302:
-#                sys.exit("Request timed out. Check connection and try again.")
-#            else:
-#                sys.exit("Uniprot had some other error")
-#
-#
-#    if lines == []:
-#        error.write(uniprot_accession_in + '\t' + "Blank Fasta" + '\n')
-#        error.close
-# if lines == []:
-#        error.write(uniprot_accession_in + '\t' + "Blank Fasta" + '\n')
-#        error.close
-#        seqlength = 'NA'
-#        genename = 'NA'
-#        return ReturnValue1(seqlength, genename)
-#    if lines != []:
-#        seqlength = 0
-#        header = lines[0]
-#        for line in lines[1:]:
-#            line = line.replace("\n","") # strip \n or else it gets counted in the length
-#            seqlength += len(line)
-#        if 'GN=' in header:
-#            lst = header.split('GN=')
-#            lst2 = lst[1].split(' ')
-#            genename = lst2[0]
-#            error.close
-#            return ReturnValue1(seqlength, genename)
-#        if 'GN=' not in header:
-#            genename = 'NA'
-#            error.close
-#            return ReturnValue1(seqlength, genename)
-
-    data = open(fasta_db,'r')
-    lines = data.readlines()
-    db_len = len(lines)
-    seqlength = 0
-    count = 0
-    for i in lines:
-        if ">sp" in i:
-            if uniprot_accession_in == i.split("|")[1]:
-                match = count+1
-                if 'GN=' in i:
-                    lst = i.split('GN=')
-                    lst2 = lst[1].split(' ')
-                    genename = lst2[0]
-                if 'GN=' not in i:
-                    genename = 'NA'
-                while ">sp" not in lines[match]:
-                    if match <= db_len:
-                        seqlength = seqlength + len(lines[match].strip())
-                        match = match + 1
-                    else:
-                        break
-                return ReturnValue1(seqlength, genename)
-        count = count + 1
-
-
-    if seqlength == 0:
-        error.write(uniprot_accession_in + '\t' + "Uniprot not in Fasta" + '\n')
-        error.close
-        seqlength = 'NA'
-        genename = 'NA'
-        return ReturnValue1(seqlength, genename)
-
-
-def readtab(infile):
-    with open(infile,'r') as x: # read in tab-delim text
-        output = []
-        for line in x:
-            line = line.strip()
-            temp = line.split('\t')
-            output.append(temp)
-    return output
-def read_maxquant(maxquant_input): # Get data, proteins and header from maxquant output
-    dupes = readtab(maxquant_input)
-    header_start = 0
-    header = dupes[header_start]
-    for i in header:
-        i = i.replace(r"\"", "")
-        i = i.replace(r"Intensity.", r"")
-        i = i.replace(r".", r"-")
-    data = dupes[header_start+1:len(dupes)] #cut off blank line and END OF FILE
-    proteins = []
-    for protein in data:
-        proteins.append(protein[0])
-    return ReturnValue2(data, proteins, header)
-def make_inter(maxquant_input):
-    bait = readtab(baitfile)
-    data = read_maxquant(maxquant_input).data
-    header = read_maxquant(maxquant_input).header
-    proteins = read_maxquant(maxquant_input).proteins
-    bait_index = []
-    for i in bait:
-        bait_index.append(header.index("mapped_protein") + 1) # Find just the baits defined in bait file
-    with open('inter.txt', 'w') as y:
-            a = 0; l=0
-            for bb in bait:
-                for lst in data:
-                    y.write(header[bait_index[l]] + '\t' + bb[1] + '\t' + proteins[a] + '\t' + lst[bait_index[l]] + '\n')
-                    a+=1
-                    if a == len(proteins):
-                        a = 0; l+=1
-def make_prey(maxquant_input):
-    proteins = read_maxquant(maxquant_input).proteins
-    output_file = open("prey.txt",'w')
-    for a in proteins:
-        a = a.replace("\n","") # remove \n for input into function
-        a = a.replace("\r","") # ditto for \r
-        seq = get_info(a).seqlength
-        GN = get_info(a).genename
-        if seq != 'NA':
-            output_file.write(a+"\t"+str(seq)+ "\t" + str(GN) + "\n")
-    output_file.close()
-def no_error_inter(maxquant_input): # remake inter file without protein errors from Uniprot
-    err = readtab("error proteins.txt")
-    bait = readtab(baitfile)
-    data = read_maxquant(maxquant_input).data
-    header = read_maxquant(maxquant_input).header
-    header = [i.replace(r"\"", "") for i in header]
-    header = [i.replace(r"Intensity.", r"") for i in header]
-    header = [i.replace(r".", r"-") for i in header]
-    print header
-    bait_index = []
-    for i in bait:
-        bait_index.append(header.index(i[0]))
-    proteins = read_maxquant(maxquant_input).proteins
-    errors = []
-    for e in err:
-        errors.append(e[0])
-    with open('inter.txt', 'w') as y:
-        l = 0; a = 0
-        for bb in bait:
-            for lst in data:
-                if proteins[a] not in errors:
-                    y.write(header[bait_index[l]] + '\t' + bb[1] + '\t' + proteins[a] + '\t' + lst[bait_index[l]] + '\n')
-                a+=1
-                if a == len(proteins):
-                    l += 1; a = 0
-def bait_check(bait, maxquant_input): # check that bait names share header titles
-    bait_in = readtab(bait)
-    header = read_maxquant(maxquant_input).header
-    for i in bait_in:
-        if i[0] not in header:
-            sys.exit("Bait must share header titles with maxquant output")
-
-if __name__ == '__main__':
-    main(infile, make_bait)
--- a/saint_preproc/pre_process_protein_name_set.R	Tue Nov 10 13:13:22 2015 -0500
+++ /dev/null	Thu Jan 01 00:00:00 1970 +0000
@@ -1,77 +0,0 @@
-library(data.table)
-library(affy)
-library(stringr)
-library(mygene)
-library(VennDiagram)
-#####
-#data
-main <- function(peptides_file) {
-	peptides_file = read.delim(peptides_file,header=TRUE,stringsAsFactors=FALSE,fill=TRUE)
-  peptides_txt = peptides_file
-	intensity_columns = names(peptides_txt[,str_detect(names(peptides_txt),"Intensity\\.*")]) #Pulls out all lines with Intensity in them.
-	intensity_columns = intensity_columns[2:length(intensity_columns)] #Removes the first column that does not have a bait.
-	peptides_txt_mapped = as.data.frame(map_peptides_proteins(peptides_txt)) #This function as below sets every line to a 1 to 1 intensity to each possible protein.
-	peptides_txt_mapped$Uniprot = str_extract(peptides_txt_mapped$mapped_protein, "[OPQ][0-9][A-Z0-9]{3}[0-9]|[A-NR-Z][0-9]([A-Z][A-Z0-9]{2}[0-9]){1,2}") #Pulls out just Uniprot id from the script.
-	peptides_txt_mapped = subset(peptides_txt_mapped,!is.na(Uniprot)) #removes reverse sequences and any that didn't match a uniprot accession
-	columns_comb = c("Uniprot", intensity_columns)
-	peptides_mapped_intensity = subset(peptides_txt_mapped, select = columns_comb) #Subsets out only the needed cloumns for Tukeys (Uniprot IDS and baited intensities)
-	swissprot_fasta = scan("/home/philip/galaxy/tools/Moffitt_Tools/uniprot_names.txt",what="character")
-	peptides_txt_mapped_log2 = peptides_mapped_intensity
-  # Takes the log2 of the intensities.
-	for (i in intensity_columns) {
-		peptides_txt_mapped_log2[,i] = log2(subset(peptides_txt_mapped_log2, select = i))
-	}
-  #get the minimum from each column while ignoring the -Inf; get the min of these mins for the global min; breaks when there's only one intensity column
-	global_min = min(apply(peptides_txt_mapped_log2[,2:ncol(peptides_txt_mapped_log2)],2,function(x) {
-	  min(x[x != -Inf])
-	}))
-	peptides_txt_mapped_log2[peptides_txt_mapped_log2 == -Inf] <- 0
-  #uniprot accessions WITHOUT isoforms; it looks like only contaminants contain isoforms anyways
-	mapped_protein_uniprotonly = str_extract(peptides_txt_mapped_log2$Uniprot,"[OPQ][0-9][A-Z0-9]{3}[0-9]|[A-NR-Z][0-9]([A-Z][A-Z0-9]{2}[0-9]){1,2}")
-	mapped_protein_uniprot_accession = str_extract(peptides_txt_mapped_log2$Uniprot,"[OPQ][0-9][A-Z0-9]{3}[0-9](-[0-9]+)?|[A-NR-Z][0-9]([A-Z][A-Z0-9]{2}[0-9]){1,2}(-[0-9]+)?|[OPQ][0-9][A-Z0-9]{3}[0-9]|[A-NR-Z][0-9]([A-Z][A-Z0-9]{2}[0-9]){1,2}")
-	peptides_txt_mapped_log2$mapped_protein = mapped_protein_uniprotonly
-  # Runs the Tukey function returning completed table
-  peptides_txt_mapped_log2 = subset(peptides_txt_mapped_log2,mapped_protein %in% swissprot_fasta)
-	protein_intensities_tukeys = get_protein_values(peptides_txt_mapped_log2,intensity_columns)
-  protein_intensities_tukeys[protein_intensities_tukeys == 1] <- 0
-  write.table(protein_intensities_tukeys, "./tukeys_output.txt", row.names = FALSE, col.names = TRUE, quote = FALSE, sep = "\t")
-
-}
-
-map_peptides_proteins = function(peptides_in) {
-    #reverse sequences are blank but have a razor protein indicating that they are reverse; exclude these for now
-    peptides_in = subset(peptides_in,peptides_in$Proteins != "")
-    results_list = list()
-    k = 1
-    for (i in 1:nrow(peptides_in)) {
-        protein_names = peptides_in[i,"Proteins"]
-        protein_names_split = unlist(strsplit(protein_names,";"))
-        for (j in 1:length(protein_names_split)) {
-            peptides_mapped_proteins = data.frame(peptides_in[i,],mapped_protein=protein_names_split[j],stringsAsFactors=FALSE)
-            results_list[[k]] = peptides_mapped_proteins
-            k = k+1
-
-        }
-    }
-    return(rbindlist(results_list))
-}
-
-get_protein_values = function(mapped_peptides_in,intensity_columns_list) {
-  unique_mapped_proteins_list = unique(mapped_peptides_in$mapped_protein) # Gets list of all peptides listed.
-  # Generates a blank data frame with clomns of Intensities and rows of Uniprots.
-  Tukeys_df = data.frame(mapped_protein = unique_mapped_proteins_list, stringsAsFactors = FALSE )
-  for (q in intensity_columns_list) {Tukeys_df[,q] = NA}
-  for (i in 1:length(unique_mapped_proteins_list)) {
-    mapped_peptides_unique_subset = subset(mapped_peptides_in, mapped_protein == unique_mapped_proteins_list[i])
-    #calculate Tukey's Biweight from library(affy); returns a single numeric
-    #results_list[[i]] = data.frame(Protein=unique_mapped_proteins_list[i],Peptides_per_protein=nrow(mapped_peptides_unique_subset))
-    for (j in intensity_columns_list) {
-      #Populates with new Tukeys values.
-      Tukeys_df[i,j] = 2^(tukey.biweight(mapped_peptides_unique_subset[,j]))
-    }
-  }
-  return(Tukeys_df)
-}
-
-args <- commandArgs(trailingOnly = TRUE)
-main(args[1])
--- a/saint_preproc/tool_dependencies.xml	Tue Nov 10 13:13:22 2015 -0500
+++ /dev/null	Thu Jan 01 00:00:00 1970 +0000
@@ -1,6 +0,0 @@
-<?xml version="1.0"?>
-<tool_dependency>
-    <set_environment version="1.0">
-        <environment_variable name="INSTALL_RUN_PATH" action="set_to">$REPOSITORY_INSTALL_DIR</environment_variable>
-    </set_environment>-->
-</tool_dependency>
\ No newline at end of file