Python get_salmon_fraglen_file Examples

Programming Language: Python

Namespace/Package Name: bcbio.pipeline.datadict

Method/Function: get_salmon_fraglen_file

Examples at hotexamples.com: 5

Python get_salmon_fraglen_file - 5 examples found. These are the top rated real world Python examples of bcbio.pipeline.datadict.get_salmon_fraglen_file extracted from open source projects. You can rate examples to help us improve the quality of examples.

Example #1

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def run_salmon_bam(data):
    samplename = dd.get_sample_name(data)
    work_dir = dd.get_work_dir(data)
    salmon_dir = os.path.join(work_dir, "salmon", samplename)
    gtf_file = dd.get_gtf_file(data)
    bam_file = dd.get_transcriptome_bam(data)
    out_file = salmon_quant_bam(bam_file, salmon_dir, gtf_file, data)
    data = dd.set_salmon(data, out_file)
    data = dd.set_salmon_dir(data, salmon_dir)
    data = dd.set_salmon_fraglen_file(data, _get_fraglen_file(salmon_dir))
    data = dd.update_summary_qc(data, "salmon", base=dd.get_salmon_fraglen_file(data))
    return [[data]]

Example #2

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File: salmon.py Project: chapmanb/bcbio-nextgen

def run_salmon_bam(data):
    samplename = dd.get_sample_name(data)
    work_dir = dd.get_work_dir(data)
    salmon_dir = os.path.join(work_dir, "salmon", samplename)
    gtf_file = dd.get_gtf_file(data)
    bam_file = dd.get_transcriptome_bam(data)
    fasta_file = dd.get_ref_file(data)
    out_file = salmon_quant_bam(bam_file, salmon_dir, gtf_file, fasta_file, data)
    data = dd.set_salmon(data, out_file)
    data = dd.set_salmon_dir(data, salmon_dir)
    data = dd.set_salmon_fraglen_file(data, _get_fraglen_file(salmon_dir))
    data = dd.update_summary_qc(data, "salmon", base=dd.get_salmon_fraglen_file(data))
    return [[data]]

Example #3

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File: salmon.py Project: yyxql/bcbio-nextgen

def run_salmon_reads(data):
    data = utils.to_single_data(data)
    files = dd.get_input_sequence_files(data)
    if bam.is_bam(files[0]):
        files = fastq.convert_bam_to_fastq(files[0], data["dirs"]["work"],
                                           data, data["dirs"], data["config"])
    samplename = dd.get_sample_name(data)
    work_dir = dd.get_work_dir(data)
    salmon_dir = os.path.join(work_dir, "salmon", samplename)
    gtf_file = dd.get_gtf_file(data)
    if len(files) == 2:
        fq1, fq2 = files
    else:
        fq1, fq2 = files[0], None
    fasta_file = dd.get_ref_file(data)
    out_file = salmon_quant_reads(fq1, fq2, salmon_dir, gtf_file, fasta_file, data)
    data = dd.set_salmon(data, out_file)
    data = dd.set_salmon_dir(data, salmon_dir)
    data = dd.set_salmon_fraglen_file(data, _get_fraglen_file(salmon_dir))
    data = dd.update_summary_qc(data, "salmon", base=dd.get_salmon_fraglen_file(data))
    return [[data]]

Example #4

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def estimate_fragment_size(data):
    filename = dd.get_salmon_fraglen_file(data)
    if not file_exists(filename):
        return None
    flen = parse_fragment_length_file(filename)
    return float(np.sum(np.multiply(flen, range(len(flen)))))

Example #5

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File: salmon.py Project: vladsaveliev/bcbio-nextgen

def estimate_fragment_size(data):
    filename = dd.get_salmon_fraglen_file(data)
    if not file_exists(filename):
        return None
    flen = parse_fragment_length_file(filename)
    return float(np.sum(np.multiply(flen, range(len(flen)))))