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Cole/fix assigning multiple qwc #37

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Feb 5, 2024
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8 changes: 6 additions & 2 deletions CRISPResso2/CRISPRessoCORE.py
Original file line number Diff line number Diff line change
Expand Up @@ -1837,7 +1837,7 @@ def get_prime_editing_guides(this_amp_seq, this_amp_name, ref0_seq, prime_edited
break

if clone_ref_name is not None:
for ref_name in ref_names:
for this_ref_idx, ref_name in enumerate(ref_names):
if clone_ref_name == ref_name:
continue
cut_points = refs[ref_name]['sgRNA_cut_points']
Expand Down Expand Up @@ -1962,8 +1962,12 @@ def get_prime_editing_guides(this_amp_seq, this_amp_name, ref0_seq, prime_edited

#quantification window coordinates override other options
if amplicon_quant_window_coordinates_arr[clone_ref_idx] != "":
if amplicon_quant_window_coordinates_arr[this_ref_idx] != "":
this_quant_window_coordinates = amplicon_quant_window_coordinates_arr[this_ref_idx]
else:
this_quant_window_coordinates = amplicon_quant_window_coordinates_arr[clone_ref_idx]
this_include_idxs = []
these_coords = amplicon_quant_window_coordinates_arr[clone_ref_idx].split("_")
these_coords = this_quant_window_coordinates.split("_")
for coord in these_coords:
coordRE = re.match(r'^(\d+)-(\d+)$', coord)
if coordRE:
Expand Down
7 changes: 4 additions & 3 deletions CRISPResso2/CRISPRessoShared.py
Original file line number Diff line number Diff line change
Expand Up @@ -285,8 +285,9 @@ def getCRISPRessoArgParser(parser_title="CRISPResso Parameters", required_params
help='If set, in the allele plots, the percentages will show the percentage as a percent of reads aligned to the assigned reference. Default behavior is to show percentage as a percent of all reads.',
action='store_true')
parser.add_argument('-qwc', '--quantification_window_coordinates', type=str,
help='Bp positions in the amplicon sequence specifying the quantification window. This parameter overrides values of the "--quantification_window_center", "--cleavage_offset", "--window_around_sgrna" or "--window_around_sgrna" values. Any indels/substitutions outside this window are excluded. Indexes are 0-based, meaning that the first nucleotide is position 0. Ranges are separted by the dash sign (e.g. "start-stop"), and multiple ranges can be separated by the underscore (_). ' +
'A value of 0 disables this filter. (can be comma-separated list of values, corresponding to amplicon sequences given in --amplicon_seq e.g. 5-10,5-10_20-30 would specify the 5th-10th bp in the first reference and the 5th-10th and 20th-30th bp in the second reference)',
help='Bp positions in the amplicon sequence specifying the quantification window. This parameter overrides values of the "--quantification_window_center", "--cleavage_offset", "--window_around_sgrna" or "--window_around_sgrna" values. Any indels/substitutions outside this window are excluded. Indexes are 0-based, meaning that the first nucleotide is position 0. Ranges are separted by the dash sign (e.g. "start-stop"), and multiple ranges can be separated by the underscore (_) (can be comma-separated list of values, corresponding to amplicon sequences given in --amplicon_seq e.g. 5-10,5-10_20-30 would specify the 6th-11th bp in the first reference and the 6th-11th and 21st-31st bp in the second reference). ' +
'A value of 0 disables this filter for a particular amplicon (e.g. 0,90-110 This would disable the quantification window for the first amplicon and specify the quantification window of 90-110 for the second).' +
'Note that if there are multiple amplicons provided, and only one quantification window coordinate is provided, the same quantification window will be used for all amplicons and be adjusted to account for insertions/deletions.',
default=None)
parser.add_argument('--annotate_wildtype_allele', type=str,
help='Wildtype alleles in the allele table plots will be marked with this string (e.g. **).',
Expand Down Expand Up @@ -1527,7 +1528,7 @@ def get_amplicon_info_for_guides(ref_seq, guides, guide_mismatches, guide_names,
# create mask of positions in which to include/exclude indels for the quantification window
# first, if exact coordinates have been given, set those
given_include_idxs = []
if quantification_window_coordinates is not None:
if quantification_window_coordinates is not None and quantification_window_coordinates != "0":
coordinate_include_idxs = []
theseCoords = str(quantification_window_coordinates).split("_")
for coord in theseCoords:
Expand Down
2 changes: 1 addition & 1 deletion README.md
Original file line number Diff line number Diff line change
Expand Up @@ -245,7 +245,7 @@ This should produce a folder called 'CRISPResso_on_base_editor'. Open the file c

-wc or --quantification_window_center or --cleavage_offset: Center of quantification window to use within respect to the 3' end of the provided sgRNA sequence. Remember that the sgRNA sequence must be entered without the PAM. For cleaving nucleases, this is the predicted cleavage position. The default is -3 and is suitable for the Cas9 system. For alternate nucleases, other cleavage offsets may be appropriate, for example, if using Cpf1 this parameter would be set to 1. For base editors, this could be set to -17. (default: -3)

-qwc or --quantification_window_coordinates: Bp positions in the amplicon sequence specifying the quantification window. This parameter overrides values of the "--quantification_window_center", "-- cleavage_offset", "--window_around_sgrna" or "-- window_around_sgrna" values. Any indels/substitutions outside this window are excluded. Indexes are 0-based, meaning that the first nucleotide is position 0. Ranges are separated by the dash sign like "start-stop", and multiple ranges can be separated by the underscore (\_). A value of 0 disables this filter. (can be comma-separated list of values, corresponding to amplicon sequences given in --amplicon_seq e.g. 5-10,5-10_20-30 would specify the 5th-10th bp in the first reference and the 5th-10th and 20th-30th bp in the second reference) (default: None)
-qwc or --quantification_window_coordinates: Bp positions in the amplicon sequence specifying the quantification window. This parameter overrides values of the "--quantification_window_center", "-- cleavage_offset", "--window_around_sgrna" or "-- window_around_sgrna" values. Any indels/substitutions outside this window are excluded. Indexes are 0-based, meaning that the first nucleotide is position 0. Ranges are separated by the dash sign like "start-stop", and multiple ranges can be separated by the underscore (\_). A value of 0 disables this filter. (can be comma-separated list of values, corresponding to amplicon sequences given in --amplicon_seq e.g. 5-10,5-10_20-30 would specify the 5th-10th bp in the first reference and the 5th-10th and 20th-30th bp in the second reference). Note that if there are multiple amplicons provided, and only one quantification window coordinate is provided, the same quantification window will be used for all amplicons and be adjusted to account for insertions/deletions. (default: None)

--exclude_bp_from_left: Exclude bp from the left side of the amplicon sequence for the quantification of the indels (default: 15)

Expand Down