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library(tidyverse) |
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library(GEOquery) |
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count_parent_dir = "~/htcf_lts/downloaded_data/mahendrawada_2024/GSE236948_RAW" |
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counts_files = list.files(count_parent_dir, ".txt.gz") |
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names(counts_files) = str_extract(counts_files, "GSM\\d+") |
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genomic_features = arrow::read_parquet("~/code/hf/yeast_genome_resources/brentlab_features.parquet") |
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test_count_df = read_tsv(file.path(count_parent_dir, counts_files[[1]]), col_names = c('orig_locus_tag', 'count')) |
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find_matching_locus <- function(target, genomic_df) { |
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match_idx <- which(str_detect(genomic_df$alias, fixed(target))) |
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if (length(match_idx) == 0) { |
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return(tibble(locus_tag = NA_character_, chr = NA_character_, |
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start = NA_real_, end = NA_real_, strand = NA_character_)) |
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} else if (length(match_idx) > 1) { |
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message(paste("Multiple matches for", target, "- taking first")) |
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match_idx <- match_idx[1] |
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} |
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genomic_df %>% |
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slice(match_idx) %>% |
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select(locus_tag, chr, start, end, strand) |
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} |
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alias_matched_locus_tags <- test_count_df %>% |
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mutate(target_locus_tag = case_when( |
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orig_locus_tag == "LSR1" ~ "YNCB0019C", |
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orig_locus_tag == "SCR1" ~ "YNCE0024W", |
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orig_locus_tag == "snR18" ~ "YNCA0003W", |
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orig_locus_tag == "snR19" ~ "YNCN0005C", |
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orig_locus_tag == "snR3" ~ "YNCJ0030W", |
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orig_locus_tag == "snR39" ~ "YNCG0014C", |
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orig_locus_tag == "snR4" ~ "YNCE0019W", |
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orig_locus_tag == "snR5" ~ "YNCO0028W", |
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orig_locus_tag == "snR6" ~ "YNCL0006W", |
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orig_locus_tag == "snR8" ~ "YNCO0026W", |
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.default = orig_locus_tag)) %>% |
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left_join(genomic_features, |
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by = c('target_locus_tag' = 'locus_tag')) %>% |
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filter(is.na(chr), str_detect(target_locus_tag, "^__", negate=TRUE)) %>% |
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select(orig_locus_tag, target_locus_tag) %>% |
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mutate(target_locus_tag = str_replace_all(target_locus_tag, "\\(|\\)", "_")) %>% |
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mutate(match_info = map(target_locus_tag, ~find_matching_locus(.x, genomic_features))) %>% |
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unnest(match_info) %>% |
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select(orig_locus_tag, locus_tag) |
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locus_tag_map = test_count_df %>% |
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mutate(locus_tag = case_when( |
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orig_locus_tag == "LSR1" ~ "YNCB0019C", |
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orig_locus_tag == "SCR1" ~ "YNCE0024W", |
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orig_locus_tag == "snR18" ~ "YNCA0003W", |
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orig_locus_tag == "snR19" ~ "YNCN0005C", |
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orig_locus_tag == "snR3" ~ "YNCJ0030W", |
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orig_locus_tag == "snR39" ~ "YNCG0014C", |
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orig_locus_tag == "snR4" ~ "YNCE0019W", |
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orig_locus_tag == "snR5" ~ "YNCO0028W", |
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orig_locus_tag == "snR6" ~ "YNCL0006W", |
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orig_locus_tag == "snR8" ~ "YNCO0026W", |
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.default = orig_locus_tag)) %>% |
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filter(locus_tag %in% genomic_features$locus_tag) %>% |
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select(-count) %>% |
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bind_rows(alias_matched_locus_tags) %>% |
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left_join(select(genomic_features, locus_tag, symbol)) %>% |
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dplyr::rename(target_locus_tag = locus_tag, |
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target_symbol = symbol) |
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gse_soft <- getGEO("GSE236947", GSEMatrix = FALSE) |
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samples <- lapply(GSMList(gse_soft), function(gsm) { |
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meta <- Meta(gsm) |
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data.frame( |
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gsm_id = meta$geo_accession, |
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title = meta$title, |
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sra = { |
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rel <- meta$relation |
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sra_rel <- rel[grep("SRA", rel)] |
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if(length(sra_rel) > 0) sub(".*term=", "", sra_rel[1]) else NA |
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}, |
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genotype = ifelse(!is.null(meta$characteristics_ch1), |
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{ |
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char_lines <- meta$characteristics_ch1 |
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genotype_line <- char_lines[grep("genotype:", char_lines)] |
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if(length(genotype_line) > 0) { |
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sub("genotype: ", "", genotype_line[1]) |
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} else { |
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NA |
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} |
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}, |
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NA), |
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growth_protocol = ifelse(!is.null(meta$growth_protocol), |
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paste(meta$growth_protocol, collapse = " "), |
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NA), |
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treatment_protocol = ifelse(!is.null(meta$treatment_protocol), |
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paste(meta$treatment_protocol, collapse = " "), |
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NA), |
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stringsAsFactors = FALSE |
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) |
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}) |
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metadata <- do.call(rbind, samples) %>% |
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as_tibble() %>% |
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dplyr::rename(sra_accession = sra) %>% |
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mutate(title = str_replace(title, "FHK2", "FKH2")) %>% |
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mutate(title = str_replace(title, "Gal4", "GAL4")) |
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stopifnot(nrow(metadata) == length(counts_files)) |
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metadata_parsed <- metadata %>% |
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mutate( |
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timepoint = str_extract(title, "_(10|30|60|120)_"), |
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timepoint = as.integer(str_remove_all(timepoint, "_")), |
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has_degron_system = str_detect(treatment_protocol, "DMSO|IAA"), |
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degron_treatment = case_when( |
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str_detect(title, "_DMSO_") ~ "DMSO", |
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str_detect(title, "_3IAA_") ~ "IAA", |
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TRUE ~ NA_character_ |
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), |
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has_degron_tag = str_detect(genotype, "IAA7|mini-N-deg|mini-degron"), |
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degron_variant = case_when( |
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str_detect(genotype, "mini-N-deg") ~ "mini_N_terminal_IAA7", |
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str_detect(genotype, "IAA7") ~ "full_or_short_IAA7", |
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TRUE ~ NA_character_ |
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), |
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has_ostir1 = str_detect(genotype, "pGPD1-OSTIR"), |
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tf_mnase_fusion = str_extract(genotype, "[A-Z0-9]+(?=-MNase)"), |
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regulator_symbol = str_extract(title, "^[A-Z0-9]+(?=_)"), |
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strain_type = case_when( |
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!is.na(regulator_symbol) ~ "degron_experiment", |
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!is.na(tf_mnase_fusion) ~ "mnase_fusion", |
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TRUE ~ "parent_strain" |
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), |
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env_condition = case_when( |
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str_detect(title, "_SM_") ~ "SM", |
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str_detect(title, "_no_gal_") ~ "no_galactose", |
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str_detect(title, "_gal_") ~ "galactose", |
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str_detect(title, "_raf_") ~ "raffinose", |
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str_detect(title, "_37") | str_detect(title, "heat") ~ "heat_shock_37C", |
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TRUE ~ "standard_30C" |
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), |
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is_wt_control = str_detect(title, "^WT_"), |
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replicate = str_extract(title, "(?<=_)[ABC](?=_)"), |
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experiment_type = case_when( |
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has_degron_system & degron_treatment %in% c("DMSO", "IAA") & regulator_symbol == "WT" ~ "wt_degron_control", |
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has_degron_system & degron_treatment %in% c("DMSO", "IAA") & regulator_symbol != "WT" ~ "degron", |
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!has_degron_system & !is.na(tf_mnase_fusion) ~ "mnase_fusion_rnaseq", |
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!has_degron_system & is_wt_control ~ "wt_baseline", |
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TRUE ~ "other" |
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)) |
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metadata_parsed_grouped = metadata_parsed %>% |
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group_by(experiment_type) |
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metadata_parsed_split = metadata_parsed_grouped %>% |
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group_split(.keep=FALSE) |
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names(metadata_parsed_split) = group_keys(metadata_parsed_grouped)$experiment_type |
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metadata_parsed_split$degron = metadata_parsed_split$degron %>% |
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replace_na(list(timepoint = 30)) |
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get_counts_add_meta = function(gsmid){ |
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df = read_tsv( |
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file.path(count_parent_dir, |
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counts_files[[gsmid]]), |
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col_names = c('orig_locus_tag', 'count')) |
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counts_meta = df %>% |
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filter(str_detect(orig_locus_tag, "^__")) %>% |
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mutate(orig_locus_tag = str_remove(orig_locus_tag, "__")) %>% |
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dplyr::rename(tmp = orig_locus_tag) %>% |
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pivot_wider(names_from = tmp, values_from = count) %>% |
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mutate(gsm_id = gsmid) %>% |
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dplyr::relocate(gsm_id) |
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counts_df = df %>% |
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filter(str_detect(orig_locus_tag, "^__", negate=TRUE)) %>% |
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left_join(locus_tag_map) %>% |
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mutate(gsm_id = gsmid) %>% |
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select(gsm_id, target_locus_tag, target_symbol, orig_locus_tag, count) |
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list( |
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meta = counts_meta, |
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counts = counts_df |
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) |
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} |
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counts_parsed_list = map(metadata_parsed_split, ~{ |
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temp_list = map(.x$gsm_id, get_counts_add_meta) |
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list( |
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meta = map_df(temp_list, "meta") %>% |
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left_join(select(.x, gsm_id, sra_accession), by = "gsm_id") %>% |
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dplyr::relocate(sra_accession, gsm_id), |
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counts = map_df(temp_list, "counts") %>% |
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left_join(select(.x, gsm_id, sra_accession), by = "gsm_id") %>% |
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dplyr::relocate(sra_accession) %>% |
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dplyr::select(-gsm_id) |
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) |
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}) |
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counts_common_cols = c('sra_accession', 'gsm_id', 'replicate', |
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'no_feature', 'ambiguous', 'too_low_aQual', |
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'alignment_not_unique') |
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final_metadata_columns = list( |
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degron = c('degron_treatment', 'degron_variant', |
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'regulator_symbol', 'env_condition', |
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'timepoint'), |
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mnase_fusion_rnaseq = c('sra_accession', 'gsm_id', 'regulator_symbol', 'env_condition'), |
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wt_baseline = c('env_condition'), |
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wt_degron_control = c('degron_treatment') |
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) |
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metadata_with_counts_meta = map(names(metadata_parsed_split), ~{ |
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metadata_parsed_split[[.x]] %>% |
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left_join(counts_parsed_list[[.x]]$meta) %>% |
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select(all_of(c(final_metadata_columns[[.x]], counts_common_cols))) %>% |
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dplyr::relocate(sra_accession, gsm_id) %>% |
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dplyr::rename(gsm_accession = gsm_id) |
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}) |
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names(metadata_with_counts_meta) = names(metadata_parsed_split) |
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set_names_grouping_col_list = list( |
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wt_baseline = 'env_condition', |
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wt_degron_control = 'degron_treatment', |
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degron = c('degron_treatment', 'env_condition', |
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'regulator_symbol', 'timepoint'), |
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mnase_fusion_rnaseq = c('regulator_symbol', 'env_condition')) |
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prev_largest_sample_id = 0 |
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metadata_with_counts_meta_with_sample_id = metadata_with_counts_meta |
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for(n in names(set_names_grouping_col_list)){ |
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metadata_with_counts_meta_with_sample_id[[n]] = metadata_with_counts_meta[[n]] %>% |
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group_by(!!!syms(set_names_grouping_col_list[[n]])) %>% |
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mutate(sample_id = cur_group_id() + prev_largest_sample_id) %>% |
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arrange(sample_id) |
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prev_largest_sample_id = max(metadata_with_counts_meta_with_sample_id[[n]]$sample_id) |
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} |
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metadata_with_counts_meta_with_sample_id$mnase_fusion_rnaseq = |
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metadata_with_counts_meta_with_sample_id$mnase_fusion_rnaseq %>% |
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left_join(select(genomic_features, symbol, locus_tag) %>% |
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dplyr::rename(regulator_symbol = symbol, |
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regulator_locus_tag = locus_tag)) %>% |
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dplyr::relocate(sra_accession, gsm_accession, |
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regulator_locus_tag, regulator_symbol) |
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metadata_with_counts_meta_with_sample_id$degron = |
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metadata_with_counts_meta_with_sample_id$degron %>% |
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mutate(regulator_symbol = str_replace(regulator_symbol, "YNR063W", "PUL4")) %>% |
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left_join(select(genomic_features, symbol, locus_tag) %>% |
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dplyr::rename(regulator_symbol = symbol, |
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regulator_locus_tag = locus_tag)) %>% |
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dplyr::relocate(sra_accession, gsm_accession, |
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regulator_locus_tag, regulator_symbol) |
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for(n in names(metadata_with_counts_meta_with_sample_id)){ |
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meta = list( |
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path = file.path("/home/chase/code/hf/mahendrawada_2025", |
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paste0(n, "_counts_meta.parquet")), |
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data = metadata_with_counts_meta_with_sample_id[[n]] |
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) |
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counts = list( |
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path = file.path("/home/chase/code/hf/mahendrawada_2025", |
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paste0(n, "_counts.parquet")), |
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data = counts_parsed_list[[n]]$counts |
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) |
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arrow::write_parquet( |
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meta$data, |
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meta$path, |
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compression = "zstd", |
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write_statistics = TRUE) |
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arrow::write_parquet( |
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counts$data, |
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counts$path, |
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chunk_size = 7036, |
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compression = "zstd", |
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write_statistics = TRUE, |
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use_dictionary = c( |
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sra_accession = TRUE)) |
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} |
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