ups

2007-08-21 10:25:23 +00:00
parent 26ab6c3fe7
commit e06eeb6d17
3 changed files with 125 additions and 82 deletions
--- a/scripts/lpls/run_smoker.py
+++ b/scripts/lpls/run_smoker.py
@@ -11,41 +11,30 @@ import cx_stats
 from plots_lpls import plot_corrloads

 ######## DATA ##########
-# full smoker data
-DX = dataset.read_ftsv(open("../../data/smokers-full/Smokers.ftsv"))
-DY = dataset.read_ftsv(open("../../data/smokers-full/Yg.ftsv"))
-Y = DY.asarray().astype('d')
-# select subset genes by SAM
-rpy.r.library("siggenes")
-rpy.r.library("qvalue")
-data = DX.asarray().T
-# data = data[:100,:]
-rpy.r.assign("data", data)
-cl = dot(DY.asarray(), diag([1,2,3])).sum(1)
-rpy.r.assign("cl", cl)
-rpy.r.assign("B", 20)
-# Perform a SAM analysis.
-print "Starting SAM"
-sam = rpy.r('sam.out<-sam(data=data,cl=cl,B=B,rand=123)')
-print "SAM done"
-# Compute the q-values of the genes.
-qq = rpy.r('qobj<-qvalue(sam.out@p.value)')
-qvals = asarray(qq['qvalues'])
-# cut off
-cutoff = 0.05
-index = where(qvals<cutoff)[0]
+use_data='uma'
+if use_data=='smoker':
+    # full smoker data
+    DX = dataset.read_ftsv(open("../../data/smokers-full/Smokers.ftsv"))
+    DY = dataset.read_ftsv(open("../../data/smokers-full/Yg.ftsv"))
+    Y = DY.asarray().astype('d')
+    gene_ids = DX.get_identifiers('gene_ids', sorted=True)
+elif use_data=='scherf':
+    DX = dataset.read_ftsv(open("../../data/scherf/Scherf.ftsv"))
+    DY = dataset.read_ftsv(open("../../data/scherf/Yd.ftsv"))
+    Y = DY.asarray().astype('d')
+    gene_ids = DX.get_identifiers('gene_ids', sorted=True)
+elif use_data=='staunton':
+    pass
+elif use_data=='uma':
+    DX = dataset.read_ftsv(open("../../data/uma/X133.ftsv"))
+    DY = dataset.read_ftsv(open("../../data/uma/Yg133.ftsv"))
+    Y = DY.asarray().astype('d')
+    gene_ids = DX.get_identifiers('gene_ids', sorted=True)

-# Subset data
-X = DX.asarray()
-Xr = X[:,index]
-gene_ids = DX.get_identifiers('gene_ids', index)
-print "\nWorking on subset with %s genes " %len(gene_ids)
-#gene2ind = {}
-#for i, gene in enumerate(gene_ids):
-#    gene2ind[gene] = i
-
-### Build GO data ####
+# Use only subset defined on GO
+ontology = 'BP'
 print "\n\nFiltering genes by Go terms "
+
 gene2goterms = rpy_go.goterms_from_gene(gene_ids)
 all_terms = set()
 for t in gene2goterms.values():
@@ -55,61 +44,72 @@ print "\nNumber of go-terms: %s" %len(terms)
 # update genelist
 gene_ids = gene2goterms.keys()
 print "\nNumber of genes: %s" %len(gene_ids)
+
+# use subset based on SAM or IQR
+subset = 'm'
+if subset=='sam':
+    # select subset genes by SAM
+    rpy.r.library("siggenes")
+    rpy.r.library("qvalue")
+    data = DX.asarray().T
+    # data = data[:100,:]
+    rpy.r.assign("data", data)
+    cl = dot(DY.asarray(), diag([1,2,3])).sum(1)
+    rpy.r.assign("cl", cl)
+    rpy.r.assign("B", 20)
+    # Perform a SAM analysis.
+    print "Starting SAM"
+    sam = rpy.r('sam.out<-sam(data=data,cl=cl,B=B,rand=123)')
+    print "SAM done"
+    # Compute the q-values of the genes.
+    qq = rpy.r('qobj<-qvalue(sam.out@p.value)')
+    qvals = asarray(qq['qvalues'])
+    # cut off
+    cutoff = 0.001
+    index = where(qvals<cutoff)[0]
+    # Subset data
+    X = DX.asarray()
+    #Xr = X[:,index]
+    gene_ids = DX.get_identifiers('gene_ids', index)
+    print "\nWorking on subset with %s genes " %len(gene_ids)
+else:
+    # noimp (smoker data is prefiltered)
+    pass
+
+
 rpy.r.library("GOSim")
 # Go-term similarity matrix
 methods = ("JiangConrath","Resnik","Lin","CoutoEnriched","CoutoJiangConrath","CoutoResnik","CoutoLin")
-meth = methods[0]
+meth = methods[2]
 print "Term-term similarity matrix (method = %s)" %meth
-if meth=="CoutoEnriched":
-    rpy.r('setEnrichmentFactors(alpha=0.1,beta=0.5)')
+
 print "\nCalculating term-term similarity matrix"

-rpytmat1 = rpy.with_mode(rpy.NO_CONVERSION, rpy.r.getTermSim)(terms, method=meth,verbose=False)
-tmat1 = rpy.r.assign("haha", rpytmat1)
-
-# check if all terms where found
-nanindex = where(isnan(tmat1[:,0]))[0]
-if len(nanindex)>0:
-    raise valueError("NANs in tmat")
-
-# Z-matrix
-#Z, newind = rpy_go.genego_matrix(terms, tmat, gene_ids, terms,func=mean)
-#Z = Z.T
-Z = rpy_go.genego_sim(gene2goterms,gene_ids,terms,rpytmat1,go_term_sim="OA",term_sim=meth)
-
-
-#### do another
-#meth = methods[4]
-#rpytmat = rpy.with_mode(rpy.NO_CONVERSION, rpy.r.getTermSim)(terms, method=meth,verbose=False)
-#tmat = rpy.r.assign("haha", rpytmat)
-
-# check if all terms where found
-#nanindex = where(isnan(tmat[:,0]))[0]
-#if len(nanindex)>0:
-#    raise valueError("NANs in tmat")
-
-# Z-matrix
-#Z, newind = rpy_go.genego_matrix(terms, tmat, gene_ids, terms,func=mean)
-#Z = Z.T
-#Z = rpy_go.genego_sim(gene2goterms,gene_ids,terms,rpytmat,go_term_sim="OA",term_sim=meth)
-
-
+rpytmat = rpy.with_mode(rpy.NO_CONVERSION, rpy.r.getTermSim)(terms, method=meth,verbose=False)
+tmat = rpy.r.assign("haha", rpytmat)
+print "\n Calculating Z matrix"
+Z = rpy_go.genego_sim(gene2goterms,gene_ids,terms,rpytmat,go_term_sim="OA",term_sim=meth)

 # update data (X) matrix
-#newind = [gene2ind[gene] for gene in gene_ids]
 newind = DX.get_indices('gene_ids', gene_ids)
-Xr = X[:,newind]
-#new_gene_ids = asarray(gene_ids)[newind]
+Xr = DX.asarray()[:,newind]


 ######## LPLSR ########
 print "LPLSR ..."
 a_max = 5
 aopt = 3
-alpha=.4
-mean_ctr = [2, 0, 1]
+xz_alpha = .5
+w_alpha = .1
+mean_ctr = [2, 0, 2]
+
+# standardize Z?
+sdtz = False
+if sdtz:
+    Z = Z/Z.std(0)
+
 T, W, P, Q, U, L, K, B, b0, evx, evy, evz = nipals_lpls(Xr,Y,Z, a_max,
-                                                        alpha=alpha,
+                                                        alpha=xz_alpha,
                                                        mean_ctr=mean_ctr)

 # Correlation loadings
@@ -117,24 +117,22 @@ dx,Rx,rssx = correlation_loadings(Xr, T, P)
 dx,Ry,rssy = correlation_loadings(Y, T, Q)
 cadz,Rz,rssz = correlation_loadings(Z.T, W, L)
 # Prediction error
-rmsep , yhat, class_error = cv_lpls(Xr, Y, Z, a_max, alpha=alpha,mean_ctr=mean_ctr)
-alpha_check=True
+rmsep , yhat, class_error = cv_lpls(Xr, Y, Z, a_max, alpha=xz_alpha,mean_ctr=mean_ctr)
+alpha_check=False
 if alpha_check:
    Alpha = arange(0.01, 1, .1)
    Rmsep,Yhat, CE = [],[],[]
    for a in Alpha:
-        rmsep , yhat, ce = cv_lpls(Xr, Y, Z, a_max, alpha=alpha)
+        rmsep , yhat, ce = cv_lpls(Xr, Y, Z, a_max, alpha=xz_alpha,mean_ctr=mean_ctr)
        Rmsep.append(rmsep)
        Yhat.append(yhat)
        CE.append(ce)
    Rmsep = asarray(Rmsep)
    Yhat = asarray(Yhat)
    CE = asarray(CE)
-    
-

 # Significance Hotellings T
-Wx, Wz, Wy, = jk_lpls(Xr, Y, Z, aopt)
+Wx, Wz, Wy, = jk_lpls(Xr, Y, Z, aopt, mean_ctr=mean_ctr,alpha=w_alpha)
 Ws = W*apply_along_axis(norm, 0, T)
 tsqx = cx_stats.hotelling(Wx, Ws[:,:aopt])
 tsqz = cx_stats.hotelling(Wz, L[:,:aopt])
@@ -157,7 +155,8 @@ ylim([class_error.min()-.05, class_error.max()+.05])
 title('Classification accuracy')

 figure(3) # Hypoid correlations
-plot_corrloads(Rz, pc1=0, pc2=1, s=tsqz/10.0, c='b', zorder=5, expvar=evz, ax=None)
+tsqz_s = 250*tsqz/tsqz.max()
+plot_corrloads(Rz, pc1=0, pc2=1, s=tsqz_s, c='b', zorder=5, expvar=evz, ax=None)
 ax = gca()
 ylabels = DY.get_identifiers('_status', sorted=True)
 plot_corrloads(Ry, pc1=0, pc2=1, s=150, c='g', zorder=5, expvar=evy, ax=ax,labels=ylabels)