diff dante_gff_to_dna.py @ 0:a5f1638b73be draft

Uploaded
author petr-novak
date Wed, 26 Jun 2019 08:01:42 -0400
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--- /dev/null	Thu Jan 01 00:00:00 1970 +0000
+++ b/dante_gff_to_dna.py	Wed Jun 26 08:01:42 2019 -0400
@@ -0,0 +1,186 @@
+#!/usr/bin/env python3
+
+import argparse
+import configuration
+import time
+import os
+from collections import defaultdict
+from Bio import SeqIO
+import textwrap
+
+t_nt_seqs_extraction = time.time()
+
+
+def str2bool(v):
+    if v.lower() in ('yes', 'true', 't', 'y', '1'):
+        return True
+    elif v.lower() in ('no', 'false', 'f', 'n', '0'):
+        return False
+    else:
+        raise argparse.ArgumentTypeError('Boolean value expected')
+
+
+def check_file_start(gff_file):
+    count_comment = 0
+    with open(gff_file, "r") as gff_all:
+        line = gff_all.readline()
+        while line.startswith("#"):
+            line = gff_all.readline()
+            count_comment += 1
+    return count_comment, line
+
+
+def extract_nt_seqs(DNA_SEQ, DOM_GFF, OUT_DIR, CLASS_TBL, EXTENDED):
+    ''' Extract nucleotide sequences of protein domains found by DANTE from input DNA seq.
+		Sequences are saved in fasta files separately for each transposon lineage.
+		Sequences extraction is based on position of Best_Hit alignment reported by LASTAL.
+		The positions can be extended (optional) based on what part of database domain was aligned (Best_Hit_DB_Pos attribute).
+		The strand orientation needs to be considered in extending and extracting the sequence itself
+	'''
+    [count_comment, first_line] = check_file_start(DOM_GFF)
+    unique_classes = get_unique_classes(CLASS_TBL)
+    files_dict = defaultdict(str)
+    domains_counts_dict = defaultdict(int)
+    allSeqs = SeqIO.to_dict(SeqIO.parse(DNA_SEQ, 'fasta'))
+    with open(DOM_GFF, "r") as domains:
+        for comment_idx in range(count_comment):
+            next(domains)
+        seq_id_stored = first_line.split("\t")[0]
+        allSeqs = SeqIO.to_dict(SeqIO.parse(DNA_SEQ, 'fasta'))
+        seq_nt = allSeqs[seq_id_stored]
+        for line in domains:
+            seq_id = line.split("\t")[0]
+            dom_type = line.split("\t")[8].split(";")[0].split("=")[1]
+            elem_type = line.split("\t")[8].split(";")[1].split("=")[1]
+            strand = line.split("\t")[6]
+            align_nt_start = int(line.split("\t")[8].split(";")[3].split(":")[
+                -1].split("-")[0])
+            align_nt_end = int(line.split("\t")[8].split(";")[3].split(":")[
+                -1].split("-")[1].split("[")[0])
+            if seq_id != seq_id_stored:
+                seq_id_stored = seq_id
+                seq_nt = allSeqs[seq_id_stored]
+            if EXTENDED:
+                ## which part of database sequence was aligned
+                db_part = line.split("\t")[8].split(";")[4].split("=")[1]
+                ## datatabse seq length
+                dom_len = int(db_part.split("of")[1])
+                ## start of alignment on database seq
+                db_start = int(db_part.split("of")[0].split(":")[0])
+                ## end of alignment on database seq
+                db_end = int(db_part.split("of")[0].split(":")[1])
+                ## number of nucleotides missing in the beginning
+                dom_nt_prefix = (db_start - 1) * 3
+                ## number of nucleotides missing in the end
+                dom_nt_suffix = (dom_len - db_end) * 3
+                if strand == "+":
+                    dom_nt_start = align_nt_start - dom_nt_prefix
+                    dom_nt_end = align_nt_end + dom_nt_suffix
+                ## reverse extending for - strand
+                else:
+                    dom_nt_start = align_nt_start - dom_nt_suffix
+                    dom_nt_end = align_nt_end + dom_nt_prefix
+                ## correction for domain after extending having negative starting positon
+                dom_nt_start = max(1, dom_nt_start)
+            else:
+                dom_nt_start = align_nt_start
+                dom_nt_end = align_nt_end
+            full_dom_nt = seq_nt.seq[dom_nt_start - 1:dom_nt_end]
+            ## for - strand take reverse complement of the extracted sequence
+            if strand == "-":
+                full_dom_nt = full_dom_nt.reverse_complement()
+            full_dom_nt = str(full_dom_nt)
+            ## report when domain classified to the last level and no Ns in extracted seq
+            if elem_type in unique_classes and "N" not in full_dom_nt:
+                # lineages reported in separate fasta files
+                if not elem_type in files_dict:
+                    files_dict[elem_type] = os.path.join(
+                        OUT_DIR, "{}.fasta".format(elem_type.split("|")[
+                            -1].replace("/", "_")))
+                with open(files_dict[elem_type], "a") as out_nt_seq:
+                    out_nt_seq.write(">{}:{}-{}|{}[{}]\n{}\n".format(
+                        seq_nt.id, dom_nt_start, dom_nt_end, dom_type,
+                        elem_type, textwrap.fill(full_dom_nt,
+                                                 configuration.FASTA_LINE)))
+                domains_counts_dict[elem_type] += 1
+    return domains_counts_dict
+
+
+def get_unique_classes(CLASS_TBL):
+    ''' Get all the lineages of current domains classification table to check if domains are classified to the last level.
+		Only the sequences of unambiguous and completely classified domains will be extracted.
+	'''
+    unique_classes = []
+    with open(CLASS_TBL, "r") as class_tbl:
+        for line in class_tbl:
+            line_class = "|".join(line.rstrip().split("\t")[1:])
+            if line_class not in unique_classes:
+                unique_classes.append(line_class)
+    return unique_classes
+
+
+def write_domains_stat(domains_counts_dict, OUT_DIR):
+    ''' Report counts of domains for individual lineages
+	'''
+    total = 0
+    with open(
+            os.path.join(OUT_DIR,
+                         configuration.EXTRACT_DOM_STAT), "w") as dom_stat:
+        for domain, count in domains_counts_dict.items():
+            dom_stat.write(";{}:{}\n".format(domain, count))
+            total += count
+        dom_stat.write(";TOTAL:{}\n".format(total))
+
+
+def main(args):
+
+    DNA_SEQ = args.input_dna
+    DOM_GFF = args.domains_gff
+    OUT_DIR = args.out_dir
+    CLASS_TBL = args.classification
+    EXTENDED = args.extended
+
+    if not os.path.exists(OUT_DIR):
+        os.makedirs(OUT_DIR)
+
+    domains_counts_dict = extract_nt_seqs(DNA_SEQ, DOM_GFF, OUT_DIR, CLASS_TBL,
+                                          EXTENDED)
+    write_domains_stat(domains_counts_dict, OUT_DIR)
+
+    print("ELAPSED_TIME_EXTRACTION = {} s\n".format(time.time() -
+                                                    t_nt_seqs_extraction))
+
+
+if __name__ == "__main__":
+
+    # Command line arguments
+    parser = argparse.ArgumentParser()
+    parser.add_argument('-i',
+                        '--input_dna',
+                        type=str,
+                        required=True,
+                        help='path to input DNA sequence')
+    parser.add_argument('-d',
+                        '--domains_gff',
+                        type=str,
+                        required=True,
+                        help='GFF file of protein domains')
+    parser.add_argument('-cs',
+                        '--classification',
+                        type=str,
+                        required=True,
+                        help='protein domains classification file')
+    parser.add_argument('-out',
+                        '--out_dir',
+                        type=str,
+                        default=configuration.EXTRACT_OUT_DIR,
+                        help='output directory')
+    parser.add_argument(
+        '-ex',
+        '--extended',
+        type=str2bool,
+        default=True,
+        help=
+        'extend the domains edges if not the whole datatabase sequence was aligned')
+    args = parser.parse_args()
+    main(args)