CRISPResso version 2.3.1 [Command used]: /software/EasyBuild/Intel_Xeon_Platinum_8358_CPU__2.60GHz/software/crispresso2/2.3.1/bin/CRISPResso -o /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch --name Sample007 --exclude_bp_from_left 15 --needleman_wunsch_gap_open -20 --exclude_bp_from_right 15 --min_single_bp_quality 0 --conversion_nuc_to T --aln_seed_len 10 --min_paired_end_reads_overlap 10 --max_paired_end_reads_overlap None --needleman_wunsch_gap_extend -2 --quantification_window_size 1 --n_processes 6 --needleman_wunsch_gap_incentive 1 --prime_editing_gap_open_penalty -50 --flash_command None --verbosity 3 --amplicon_name Reference --plot_window_size 20 --quantification_window_center -3 --prime_editing_pegRNA_extension_quantification_window_size 5 --min_average_read_quality 0 --fastp_command fastp --prime_editing_pegRNA_scaffold_min_match_length 1 --max_rows_alleles_around_cut_to_plot 50 --amplicon_seq TAAACTACCAGAAGTATCAGTGCTAAAAGTATCCTTTTCTTTCCTACAGATTCCTCCTTATGGCCAACAAGGCCCCAGCGGGTATGGTCAGCAGGGCCAGACTCCATATTACAACCAGCAAAGTCCTCACCCCCAGCAGCAGCAGCCACCCTACTCTCAGCAACCACCATCCCAGACCCCTCATGCTCAACCTTCATATCAGCAGCAGCCTCAGTCTCAGCCACCACAGCTCCAGTCATCTCAGCCTCCATATTCCCAGCAGCCA --flexiguide_homology 80 --trimmomatic_command None --default_min_aln_score 60 --fastq_r1 Sample007_R1.fastq.gz --aln_seed_count 5 --aln_seed_min 2 --guide_seq GGACTTTGCTGGTTGTAATA --needleman_wunsch_aln_matrix_loc EDNAFULL --config_file None --min_bp_quality_or_N 0 --flexiguide_seq None --conversion_nuc_from C --min_frequency_alleles_around_cut_to_plot 0.2 --fastq_r2 Sample007_R2.fastq.gz --prime_editing_gap_extend_penalty 0 [Execution log]: Computing quantification windows CRISPRessoPro not installed Added 0 guides with flexible matching Original flexiguides: ['None'] Found guides: [] Mismatch locations: [] Processing sequences with fastp... Read1 before filtering: total reads: 9308 total bases: 1423509 Q20 bases: 1371810(96.3682%) Q30 bases: 1356685(95.3057%) Read2 before filtering: total reads: 9308 total bases: 1423486 Q20 bases: 1381845(97.0747%) Q30 bases: 1364735(95.8727%) Merged and filtered: total reads: 9138 total bases: 2314766 Q20 bases: 2248479(97.1363%) Q30 bases: 2226998(96.2083%) Filtering result: reads passed filter: 18616 reads failed due to low quality: 0 reads failed due to too many N: 0 reads corrected by overlap analysis: 730 bases corrected by overlap analysis: 1005 Duplication rate: 83.1758% Insert size peak (evaluated by paired-end reads): 254 Read pairs merged: 9138 % of original read pairs: 98.1736% % in reads after filtering: 100% JSON report: /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/fastp_report.json HTML report: /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/fastp_report.html fastp -i Sample007_R1.fastq.gz -I Sample007_R2.fastq.gz --merge --merged_out /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/oet.extendedFrags.fastq.gz --unpaired1 /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/out.notCombined_1.fastq.gz --unpaired2 /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/out.notCombined_2.fastq.gz --overlap_len_require 10 --thread 6 --json /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/fastp_report.json --html /mmfs1/projects/rrc_shared/common/practice_data/CRISPresso/gchlip2_20260708_work/crispresso_out/CRISPRessoBatch_on_crispresso_batch/CRISPResso_on_Sample007/fastp_report.html --disable_adapter_trimming --disable_trim_poly_g --disable_quality_filtering --disable_length_filtering fastp v0.23.4, time used: 1 seconds Done! Done! Aligning sequences... Processing reads; N_TOT_READS: 0 N_COMPUTED_ALN: 0 N_CACHED_ALN: 0 N_COMPUTED_NOTALN: 0 N_CACHED_NOTALN: 0 Finished reads; N_TOT_READS: 9138 N_COMPUTED_ALN: 1176 N_CACHED_ALN: 7925 N_COMPUTED_NOTALN: 15 N_CACHED_NOTALN: 22 Done! Quantifying indels/substitutions... Done! Calculating allele frequencies... Done! Saving processed data... Making Plots... Plotting read bar plot Plotting read class pie chart and bar plot Begin processing plots for amplicon Reference Plotting nucleotide quilt across amplicon Plotting nucleotide distribuition around sgRNA GGACTTTGCTGGTTGTAATA for Reference Plotting indel size distribution for Reference Plotting frequency deletions/insertions for Reference Plotting amplication modifications for Reference Plotting modification frequency for Reference Plotting quantification window locations for Reference Plotting position dependent indel for Reference Plotting allele distribution around cut for Reference Done! Done! Removing Intermediate files... Low number of total reads: <10000. Total reads: 9138. >=1.0% of reads have modifications at the start or end. Total reads: 9101, Irregular reads: 195. >=0.2% of substitutions were outside of the quantification window. Total substitutions: 3500, Substitutions outside window: 3500. Analysis Complete!