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authorzsloan2021-04-27 21:37:12 +0000
committerzsloan2021-04-27 21:37:12 +0000
commit75bcab50abcf29c8a5f98a9f17b37457ac433d3b (patch)
treed38d00b4bf5f5e0cadc5bb1a83a6fec0b4737ac6 /wqflask
parent1a7bb988ee360b3ef48e22e25b419c375dccb9fa (diff)
downloadgenenetwork2-75bcab50abcf29c8a5f98a9f17b37457ac433d3b.tar.gz
Stopped using the scanone function pointer when doing R/qtl mapping, since the results are not converted into a Python object in a way that preserves marker names (which is important because pseudomarkers can be added)
Instead the marker names are extracted from the scanone results using R immediately after they're generated, and then passed to process_rqtl_results
Diffstat (limited to 'wqflask')
-rw-r--r--wqflask/wqflask/marker_regression/rqtl_mapping.py39
1 files changed, 21 insertions, 18 deletions
diff --git a/wqflask/wqflask/marker_regression/rqtl_mapping.py b/wqflask/wqflask/marker_regression/rqtl_mapping.py
index 4117a0e5..f593ae91 100644
--- a/wqflask/wqflask/marker_regression/rqtl_mapping.py
+++ b/wqflask/wqflask/marker_regression/rqtl_mapping.py
@@ -78,6 +78,7 @@ def run_rqtl_geno(vals, samples, dataset, mapping_scale, method, model, permChec
cross_object = calc_genoprob(cross_object)
else:
cross_object = calc_genoprob(cross_object, step=5, stepwidth="max")
+
logger.info("after calc_genoprob");
pheno_string = sanitize_rqtl_phenotype(vals)
logger.info("phenostring done");
@@ -110,11 +111,13 @@ def run_rqtl_geno(vals, samples, dataset, mapping_scale, method, model, permChec
return process_pair_scan_results(result_data_frame)
else:
if do_control == "true" or cofactors != "":
- logger.info("Using covariate"); result_data_frame = scanone(cross_object, pheno = "the_pheno", addcovar = covars, model=model, method=method)
- ro.r('save.image(file = "/home/zas1024/gn2-zach/itp_cofactor_test.RData")')
+ ro.r(f"qtl_results = scanone(the_cross, pheno='the_pheno', addcovar=all_covars, model='{model}', method='{method}')")
+ result_data_frame = ro.r("qtl_results")
else:
- logger.info("No covariates"); result_data_frame = scanone(cross_object, pheno = "the_pheno", model=model, method=method)
+ ro.r(f"qtl_results = scanone(the_cross, pheno='the_pheno', model='{model}', method='{method}')")
+ result_data_frame = ro.r("qtl_results")
+ marker_names = np.asarray(ro.r("row.names(qtl_results)"))
if num_perm > 0 and permCheck == "ON": # Do permutation (if requested by user)
if len(perm_strata_list) > 0: #ZS: The strata list would only be populated if "Stratified" was checked on before mapping
cross_object, strata_ob = add_perm_strata(cross_object, perm_strata_list)
@@ -129,9 +132,10 @@ def run_rqtl_geno(vals, samples, dataset, mapping_scale, method, model, permChec
perm_data_frame = scanone(cross_object, pheno_col = "the_pheno", n_perm = num_perm, model=model, method=method)
perm_output, suggestive, significant = process_rqtl_perm_results(num_perm, perm_data_frame) # Functions that sets the thresholds for the webinterface
- return perm_output, suggestive, significant, process_rqtl_results(result_data_frame, dataset.group.species)
+
+ return perm_output, suggestive, significant, process_rqtl_results(marker_names, result_data_frame, dataset.group.species)
else:
- return process_rqtl_results(result_data_frame, dataset.group.species)
+ return process_rqtl_results(marker_names, result_data_frame, dataset.group.species)
def generate_cross_from_rdata(dataset):
rdata_location = locate(dataset.group.name + ".RData", "genotype/rdata")
@@ -144,7 +148,6 @@ def generate_cross_from_rdata(dataset):
""" % (rdata_location))
def generate_cross_from_geno(dataset, scale_units): # TODO: Need to figure out why some genofiles have the wrong format and don't convert properly
-
ro.r("""
trim <- function( x ) { gsub("(^[[:space:]]+|[[:space:]]+$)", "", x) }
getGenoCode <- function(header, name = 'unk'){
@@ -376,9 +379,8 @@ def process_pair_scan_results(result):
def process_rqtl_perm_results(num_perm, results):
perm_vals = []
- for line in str(results).split("\n")[1:(num_perm+1)]:
- #print("R/qtl permutation line:", line.split())
- perm_vals.append(float(line.split()[1]))
+ for item in results:
+ perm_vals.append(item)
perm_output = perm_vals
suggestive = np.percentile(np.array(perm_vals), 67)
@@ -386,20 +388,21 @@ def process_rqtl_perm_results(num_perm, results):
return perm_output, suggestive, significant
-def process_rqtl_results(result, species_name): # TODO: how to make this a one liner and not copy the stuff in a loop
+def process_rqtl_results(marker_names, results, species_name): # TODO: how to make this a one liner and not copy the stuff in a loop
qtl_results = []
- output = [tuple([result[j][i] for j in range(result.ncol)]) for i in range(result.nrow)]
- for i, line in enumerate(result.iter_row()):
+ for i, line in enumerate(results):
marker = {}
- marker['name'] = result.rownames[i]
- if species_name == "mouse" and output[i][0] == 20: #ZS: This is awkward, but I'm not sure how to change the 20s to Xs in the RData file
+ marker['name'] = marker_names[i]
+ if species_name == "mouse" and line[0] == 20:
marker['chr'] = "X"
else:
- marker['chr'] = output[i][0]
- marker['cM'] = output[i][1]
- marker['Mb'] = output[i][1]
- marker['lod_score'] = output[i][2]
+ try:
+ marker['chr'] = int(line[0])
+ except:
+ marker['chr'] = line[0]
+ marker['cM'] = marker['Mb'] = line[1]
+ marker['lod_score'] = line[2]
qtl_results.append(marker)
return qtl_results \ No newline at end of file