def test_sistr(variables):
metadata = MetadataObject()
method.runmetadata.samples = list()
fasta = os.path.join(variables.sequencepath, 'NC_003198.fasta')
metadata.name = os.path.split(fasta)[1].split('.')[0]
# Initialise the general and run categories
metadata.general = GenObject()
metadata.run = GenObject()
metadata.general.fastqfiles = list()
# Set the destination folder
outputdir = os.path.join(variables.sequencepath, metadata.name)
make_path(outputdir)
# Add the output directory to the metadata
metadata.general.outputdirectory = outputdir
metadata.general.logout = os.path.join(outputdir, 'out')
metadata.general.logerr = os.path.join(outputdir, 'err')
metadata.run.outputdirectory = outputdir
metadata.general.bestassemblyfile = True
# Initialise an attribute to store commands
metadata.commands = GenObject()
# Assume that all samples are Salmonella
metadata.general.referencegenus = 'Salmonella'
# Set the .fasta file as the best assembly
metadata.general.bestassemblyfile = fasta
method.runmetadata.samples.append(metadata)
method.sistr()
for sample in method.runmetadata.samples:
assert sample.sistr.cgmlst_genome_match == 'SAL_BA2732AA'
variable_update()
def test_sistr(variables):
metadata = MetadataObject()
method.runmetadata.samples = list()
fasta = os.path.join(variables.sequencepath, 'NC_003198.fasta')
metadata.name = os.path.split(fasta)[1].split('.')[0]
# Initialise the general and run categories
metadata.general = GenObject()
metadata.run = GenObject()
metadata.general.fastqfiles = list()
# Set the destination folder
outputdir = os.path.join(variables.sequencepath, metadata.name)
make_path(outputdir)
# Add the output directory to the metadata
metadata.general.outputdirectory = outputdir
metadata.run.outputdirectory = outputdir
metadata.general.bestassemblyfile = True
# Initialise an attribute to store commands
metadata.commands = GenObject()
# Assume that all samples are Salmonella
metadata.general.referencegenus = 'Salmonella'
# Set the .fasta file as the best assembly
metadata.general.bestassemblyfile = fasta
method.runmetadata.samples.append(metadata)
method.sistr()
for sample in method.runmetadata.samples:
assert sample.sistr.cgmlst_genome_match == 'SAL_BA2732AA'
variable_update()
def basic(self):
# Grab any .fastq files in the path
fastqfiles = glob(os.path.join(self.path, '*.fastq*'))
# Extract the base name of the globbed name + path provided
fastqnames = map(lambda x: os.path.split(x)[1], filer(fastqfiles))
# Iterate through the names of the fastq files
for fastqname in sorted(fastqnames):
# Set the name
metadata = MetadataObject()
metadata.name = fastqname
# Set the destination folder
outputdir = os.path.join(self.path, fastqname)
# Make the destination folder
make_path(outputdir)
# Get the fastq files specific to the fastqname
specificfastq = glob(
os.path.join(self.path, '{}*.fastq*'.format(fastqname)))
# Link the files to the output folder
try:
# Link the .gz files to :self.path/:filename
list(
map(
lambda x: os.symlink(
'../{}'.format(os.path.basename(x)), '{}/{}'.
format(outputdir, os.path.basename(x))),
specificfastq))
# Except os errors
except OSError as exception:
# If there is an exception other than the file exists, raise it
if exception.errno != errno.EEXIST:
raise
# Initialise the general and run categories
metadata.general = GenObject()
metadata.run = GenObject()
# Populate the .fastqfiles category of :self.metadata
metadata.general.fastqfiles = [
fastq for fastq in sorted(
glob(
os.path.join(outputdir, '{}*.fastq*'.format(
metadata.name)))) if 'trimmed' not in fastq
and 'normalised' not in fastq and 'corrected' not in fastq
and 'paired' not in fastq and 'unpaired' not in fastq
]
# Add the output directory to the metadata
metadata.general.outputdirectory = outputdir
metadata.general.logout = os.path.join(
self.path, metadata.name,
'{}_log_out.txt'.format(metadata.name))
metadata.general.logerr = os.path.join(
self.path, metadata.name,
'{}_log_err.txt'.format(metadata.name))
# Append the metadata to the list of samples
self.samples.append(metadata)
# Grab metadata from previous runs
previousmetadata = metadataReader.MetadataReader(self)
# Update self.samples (if required)
if previousmetadata.samples:
self.samples = previousmetadata.samples
# Run the read length method
self.readlength()
def createobject(self):
# Grab any .fastq files in the path
fastqfiles = glob(os.path.join(self.path, '*.fastq*'))
# Extract the base name of the globbed name + path provided
fastqnames = map(lambda x: os.path.split(x)[1], filer(fastqfiles))
# Iterate through the names of the fastq files
for fastqname in sorted(fastqnames):
# Set the name
metadata = MetadataObject()
metadata.name = fastqname
# Set the destination folder
outputdir = os.path.join(self.path, fastqname)
# Make the destination folder
make_path(outputdir)
# Get the fastq files specific to the fastqname
specificfastq = glob(
os.path.join(self.path, '{}*.fastq*'.format(fastqname)))
# Make relative symlinks to the files in :self.path
try:
for fastq in specificfastq:
# Get the basename of the file
fastqfile = os.path.split(fastq)[-1]
# Set the destination fastq path as the base name plus the destination folder
destinationfastq = os.path.join(outputdir, fastqfile)
# Symlink the files
os.symlink('../{}'.format(fastqfile), destinationfastq)
# Except os errors
except OSError as exception:
# If there is an exception other than the file exists, raise it
if exception.errno != errno.EEXIST:
raise
# Initialise the general and run categories
metadata.general = GenObject()
metadata.run = GenObject()
# Populate the .fastqfiles category of :self.metadata
metadata.general.fastqfiles = [
fastq for fastq in glob(
os.path.join(outputdir, '{}*.fastq*'.format(fastqname)))
if 'trimmed' not in fastq
]
# Add the output directory to the metadata
metadata.general.outputdirectory = outputdir
metadata.run.outputdirectory = outputdir
metadata.general.bestassemblyfile = True
metadata.general.trimmedcorrectedfastqfiles = metadata.general.fastqfiles
metadata.general.logout = os.path.join(
metadata.general.outputdirectory, 'logout')
metadata.general.logerr = os.path.join(
metadata.general.outputdirectory, 'logerr')
# Initialise an attribute to store commands
metadata.commands = GenObject()
# Append the metadata to the list of samples
self.samples.append(metadata)
# Define the start time
arguments.starttime = time.time()
# Find the files
fastas = sorted(glob(os.path.join(arguments.sequencepath, '*.fa*')))
# Create a metadata object
arguments.runmetadata = MetadataObject()
arguments.runmetadata.samples = list()
for fasta in fastas:
metadata = MetadataObject()
metadata.name = os.path.split(fasta)[1].split('.')[0]
# Initialise the general and run categories
metadata.general = GenObject()
metadata.run = GenObject()
# Set the destination folder
outputdir = os.path.join(arguments.sequencepath, metadata.name)
make_path(outputdir)
# Add the output directory to the metadata
metadata.general.outputdirectory = outputdir
metadata.run.outputdirectory = outputdir
metadata.general.bestassemblyfile = True
# Initialise an attribute to store commands
metadata.commands = GenObject()
# Assume that all samples are Salmonella
metadata.general.referencegenus = 'Salmonella'
# Set the .fasta file as the best assembly
metadata.general.bestassemblyfile = fasta
arguments.runmetadata.samples.append(metadata)
def parsesamplesheet(self):
"""Parses the sample sheet (SampleSheet.csv) to determine certain values
important for the creation of the assembly report"""
# Open the sample sheet
with open(self.samplesheet, "r") as samplesheet:
# Iterate through the sample sheet
samples, prev, header = False, 0, []
for count, line in enumerate(samplesheet):
# Remove new lines, and split on commas
# line = line.decode('utf-8') # Turn from bytes to string, since python3 is finicky.
data = line.rstrip().split(",")
if any(data):
if "[Settings]" in line:
samples = False
if not line.startswith(
"[") and not samples and not data == ['']:
# Grab an data not in the [Data] Section
setattr(self.header, data[0].replace(" ", ""),
"".join(data[1:]))
elif "[Data]" in line or "[Reads]" in line:
samples = True
elif samples and "Sample_ID" in line:
header.extend([
x.replace("_", "").replace(' ', "") for x in data
])
prev = count
elif header:
# Try and replicate the Illumina rules to create file names from "Sample_Name"
samplename = samplenamer(data)
# Create an object for storing nested static variables
strainmetadata = MetadataObject()
# Set the sample name in the object
strainmetadata.name = samplename
# Add the header object to strainmetadata
# strainmetadata.__setattr__("run", GenObject(dict(self.header)))
strainmetadata.run = GenObject(
copy.copy(self.header.datastore))
# Create the run object, so it will be easier to populate the object (eg run.SampleName = ...
# instead of strainmetadata.run.SampleName = ...
run = strainmetadata.run
# Capture Sample_ID, Sample_Name, I7_Index_ID, index1, I5_Index_ID, index2, Sample_Project
for idx, item in enumerate(data):
setattr(run, header[idx],
item) if item else setattr(
run, header[idx], "NA")
# Add the sample number
run.SampleNumber = count - prev
# Create the 'General' category for strainmetadata
strainmetadata.general = GenObject({
'outputdirectory':
os.path.join(self.path, samplename),
'pipelinecommit':
self.commit
})
strainmetadata.general.logout = os.path.join(
self.path, samplename,
'{}_log_out.txt'.format(samplename))
strainmetadata.general.logerr = os.path.join(
self.path, samplename,
'{}_log_err.txt'.format(samplename))
# Add the output directory to the general category
# Append the strainmetadata object to a list
self.samples.append(strainmetadata)
elif samples:
setattr(self.header, 'forwardlength', data[0]) \
if 'forwardlength' not in self.header.datastore else \
setattr(self.header, 'reverselength', data[0])
self.totalreads += int(data[0])
self.date = self.header.Date if "Date" in self.header.datastore else self.date
for sample in self.samples:
if 'InvestigatorName' not in sample.run.datastore:
sample.run.InvestigatorName = 'NA'