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Library Sequencing Data Processing Workflow File

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Figshare2025-10-29 更新2026-04-28 收录
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For each repair outcome category, sgRNA enrichment was evaluated by comparing outcome frequencies between individual sgRNAs and nontargeting controls using Fisher’s exact test. Both left-tailed (depletion) and right-tailed (enrichment) p-values were computed together with the corresponding log₂ fold change (log₂FC). sgRNAs with ≤10 reads or without detectable mutations were excluded.To derive gene-level significance, sgRNAs were ranked globally based on direction-specific p-values and log₂FCs. For depletion analysis, sgRNAs showing negative log₂FCs and smaller left-tailed p-values were prioritized, while inconsistent entries were penalized. The same strategy was mirrored for enrichment analysis. Robust Rank Aggregation (RRA) was applied to these ranked lists to compute gene-level RRA scores. Statistical significance was assessed through 20,000 random permutations to generate empirical p-value distributions.To integrate results from the sg3 and sg81 libraries, shared genes were retained, and combined log₂FC values were calculated using outcome-frequency–weighted averages. Corresponding one-tailed p-values were transformed into z-scores, merged by weighted averaging, and back-transformed into integrated p-values. Genes with |log₂FC| > 0.5 and combined p
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