https://github.com/fenderglass/Ragout
Tip revision: a68b9dba9aa7570c0a8e3f579b662524ee919e2b authored by Mikhail Kolmogorov on 27 July 2018, 01:48:58 UTC
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Tip revision: a68b9db
blocks-dotplot.py
#!/usr/bin/env python2.7
#(c) 2013-2014 by Authors
#This file is a part of Ragout program.
#Released under the BSD license (see LICENSE file)
"""
This script generates dot-plots of given set of synteny blocks
for visual comparison.
"""
from __future__ import print_function
from Bio import SeqIO
from Bio.SeqRecord import SeqRecord
import os, sys
import subprocess
from collections import namedtuple
Block = namedtuple("Block", ["id", "start", "length", "genome_id", "chr_id"])
SeqInfo = namedtuple("SeqInfo", ["id", "length"])
GEPARD_DIR = "/home/mkolmogo/tools/gepard-1.30/"
EXEC = "./gepardcmd.sh"
MATRIX = "matrices/edna.mat"
GENOMES = ["C57B6J", "BALBcJ"]
def main():
if len(sys.argv) < 4:
print("Usage: dotplot.py coords_file output_dir fasta_references\n\n"
"A script for plotting synteny blocks for visual verification. "
"Probably, you don't want to use it.")
return
coords_file = sys.argv[1]
fasta = sys.argv[3:]
blocks = parse_coords_file(coords_file)
draw_dot_plot(blocks, fasta, sys.argv[2])
def draw_dot_plot(blocks, seq_files, out_dir):
seqs = {}
for file in seq_files:
for seq in SeqIO.parse(file, "fasta"):
seq_id = seq.id.split(" ")[0]
seqs[seq_id] = seq.seq
out_dir = os.path.abspath(out_dir)
os.chdir(GEPARD_DIR)
for block_id, blocklist in blocks.items():
blocklist = filter(lambda b: b.genome_id in GENOMES, blocklist)
if len(blocklist) < 2:
continue
"""
allBlocks = open(os.path.join(out_dir,
"blocks{0}.fasta".format(block_id)), "w")
for block in blocklist:
seq = seqs[block.chr_id][block.start : block.start + block.length]
if block.id < 0:
seq = seq.reverse_complement()
SeqIO.write(SeqRecord(seq, id=block.chr_id, description=""),
allBlocks, "fasta")
"""
block1, block2 = blocklist[0:2]
s1 = seqs[block1.chr_id]
s2 = seqs[block2.chr_id]
seq1 = s1[block1.start : block1.start + block1.length]
seq2 = s2[block2.start : block2.start + block2.length]
if block1.id < 0:
seq1 = seq1.reverse_complement()
if block2.id < 0:
seq2 = seq2.reverse_complement()
file1 = os.path.join(out_dir, "block{0}.{1}-1.fasta"
.format(block_id, block1.chr_id))
file2 = os.path.join(out_dir, "block{0}.{1}-2.fasta"
.format(block_id, block2.chr_id))
SeqIO.write(SeqRecord(seq1), file1, "fasta")
SeqIO.write(SeqRecord(seq2), file2, "fasta")
out_dot = os.path.join(out_dir, "block{0}-{1}-{2}.png"
.format(block_id, block1.chr_id, block2.chr_id))
cmdline = [EXEC, "-seq1", file1, "-seq2", file2, "-outfile",
out_dot, "-matrix", MATRIX, "-word", "10"]
subprocess.check_call(cmdline)
os.remove(file1)
os.remove(file2)
print(len(blocks))
def parse_coords_file(blocks_file):
group = [[]]
seq_info = {}
blocks_info = {}
line = [l.strip() for l in open(blocks_file) if l.strip()]
for l in line:
if l.startswith("-"):
group.append([])
else:
group[-1].append(l)
for l in group[0][1:]:
seq_num, seq_len, seq_id = l.split()
seq_num = int(seq_num)
seq_info[seq_num] = SeqInfo(seq_id, int(seq_len))
for g in [g for g in group[1:] if g]:
block_id = int(g[0].split()[1][1:])
blocks_info[block_id] = []
for l in g[2:]:
chr_num, bl_strand, bl_start, bl_end, bl_length = l.split()
chr_num = int(chr_num)
name_string = seq_info[chr_num].id
genome_id, chr_id = name_string.split(".", 1)
bl_start, bl_end = int(bl_start), int(bl_end)
if bl_strand == "-":
bl_start, bl_end = bl_end, bl_start
num_id = block_id if bl_strand == "+" else -block_id
blocks_info[block_id].append(Block(num_id, bl_start,
int(bl_length), genome_id,
chr_id))
return blocks_info
if __name__ == "__main__":
main()
