Hi all, I want to visualize my copy number alteration results following annotating with Variant Effect Predictor (VEP) as a CNV plot.

The input of VEP had been generated by RgenomicRanges package in R. I found several significant deletions or duplications (qvalue<0.2)

Here is what I obtained from VEP:

#Uploaded_variation Location    Allele  Consequence IMPACT  SYMBOL  Gene    Feature_type    Feature BIOTYPE EXON    INTRON  HGVSc   HGVSp   cDNA_position   CDS_position    Protein_position    Amino_acids Codons  Existing_variation  DISTANCE    STRAND  FLAGS   SYMBOL_SOURCE   HGNC_ID TSL APPRIS  SIFT    PolyPhen    AF  AFR_AF  AMR_AF  EAS_AF  EUR_AF  SAS_AF  AA_AF   EA_AF   gnomAD_AF   gnomAD_AFR_AF   gnomAD_AMR_AF   gnomAD_ASJ_AF   gnomAD_EAS_AF   gnomAD_FIN_AF   gnomAD_NFE_AF   gnomAD_OTH_AF   gnomAD_SAS_AF   CLIN_SIG    SOMATIC PHENO   PUBMED  MOTIF_NAME  MOTIF_POS   HIGH_INF_POS    MOTIF_SCORE_CHANGE
11_66333072_deletion    11:66333071-66333838    deletion    coding_sequence_variant,intron_variant,feature_truncation   MODIFIER    CTSF    ENSG00000174080 Transcript  ENST00000310325 protein_coding  5/8/2013    5/8/2012    -   -   755-?   645-?   215-?   -   -   -   -   -1  -   HGNC    2531    -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -
11_66333072_deletion    11:66333071-66333838    deletion    coding_sequence_variant,intron_variant,feature_truncation   MODIFIER    CTSF    ENSG00000174080 Transcript  ENST00000524994 protein_coding  3/6/2009    3/6/2008    -   -   187-?   189-?   63-?    -   -   -   -   -1  cds_start_NF,cds_end_NF HGNC    2531    -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -
13_50135463_deletion    13:50135462-50141345    deletion    coding_sequence_variant,intron_variant,feature_truncation   MODIFIER    RCBTB1  ENSG00000136144 Transcript  ENST00000258646 protein_coding  1/2/2011    1/2/2010    -   -   115-?   71-?    24-?    -   -   -   -   -1  -   HGNC    18243   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -   -

I also tried to perform copy number alteration analysis on TCGA data using Gistic 2.0 in GenePattern. However stragely no amplification or deletion were detected.

Can you tell me why I did not get significant results when running gistic 2.0.

Regards

Nazanin

Credits to Tiago Silva; https://f1000research.com/articles/5-1542

Ignording VEP, with output from runGAIA(), which identifies recurrent somatic copy number alterations (sCNAs), you can generate a plot like this:

• Part I - download segmented sCNA data for any TCGA cohort from Broad Institute's FireBrowse server and identify recurrent sCNA regions in these with GAIA

• Part II - plot recurrent sCNA gains and losses from GAIA

• Part III - annotate the recurrent sCNA regions (this post, just below)

• Part IV - generate heatmap of recurrent sCNA regions over your cohort

Part II

run runGAIA

results <- runGAIA(cnv_obj, markers_obj, output_file_name="Tumor.asian.txt", aberrations=-1, chromosomes=-1, num_iterations=10, threshold=0.15)

tidy output

#Set qvalue threshold for plotting and annotation
threshold <- 0.15

#Convert the recurrent aberrations to numeric (GAIA saves it as text)
RecCNV <- t(apply(results, 1, as.numeric))
colnames(RecCNV) <- colnames(results)

#Add a new column for 'score'
RecCNV <- cbind(RecCNV, score=0)

#Determine the minimum Q value that's not equal to 0
minval <- format(min(RecCNV[RecCNV[,"q-value"]!=0, "q-value"]), scientific=FALSE)
minval <- substring(minval,1, nchar(minval)-1)

#Replace Q values of 0 with the minimum, non-zero value
RecCNV[RecCNV[,"q-value"]==0, "q-value"] <- as.numeric(minval)

#Set the score to equal -log base 10 of the Q value
RecCNV[,"score"] <- sapply(RecCNV[,"q-value"], function(x) -log10(as.numeric(x)))

create plot function

#Create a function for plotting the recurrent copy number variants
gaiaCNVplot <- function (calls, threshold=0.01, main="main") {
    Calls <- calls[order(calls[,"Region Start [bp]"]),]
    Calls <- Calls[order(Calls[,"Chromosome"]),]
    rownames(Calls) <- NULL
    Chromo <- Calls[,"Chromosome"]
    Gains <- apply(Calls,1,function(x) ifelse(x["Aberration Kind"]==1, x["score"], 0))
    Losses <- apply(Calls, 1,function(x) ifelse(x["Aberration Kind"]==0, x["score"], 0))
    plot(Gains, ylim=c(-max(Calls [,"score"]+2), max(Calls[,"score"]+2)), type="h", col="red2", xlab="Chromosome", ylab=expression("-log"[10]~italic(Q)~"value"), main=main, cex.main=4, xaxt="n", font=2, font.axis=2, font.lab=2, font.axis=2)
    points(-(Losses), type="h", col="forestgreen")
    abline(h= 0, cex=4)
    abline(h=-log10(threshold), col="black", cex=4, main="test", lty=6, lwd=2)
    abline(h=log10(threshold), col="black", cex=4, main="test", lty=6, lwd=2)
    uni.chr <- unique(Chromo)
    temp <- rep(0, length(uni.chr))

    for (i in 1:length(uni.chr)) {
        temp[i] <- max(which(uni.chr[i] == Chromo))
    }

    for (i in 1:length(temp)) {
        abline(v = temp[i], col = "black", lty = "dashed", )
    }

    nChroms <- length(uni.chr)

    begin <- c()

    for (d in 1:nChroms) {
        chrom <- sum(Chromo == uni.chr[d])
        begin <- append(begin, chrom)
    }

    temp2 <- rep(0, nChroms)

    for (i in 1:nChroms) {
        if (i == 1) {
            temp2[1] <- (begin[1] * 0.5)
        }
        else if (i > 1) {
            temp2[i] <- temp[i - 1] + (begin[i] * 0.5)
        }
    }

    uni.chr[uni.chr==23] <- "X"
    uni.chr[uni.chr==24] <- "Y"

    for (i in 1:length(temp)) {
        axis(1, at = temp2[i], labels = uni.chr[i], cex.axis = 1)
    }

    #legend("topright", y.intersp=0.8, c("Amplification"), pch=15, col=c("red2"), text.font=2)
    #legend("bottomright", y.intersp=0.8, c("Deletion"), pch=15, col=c("forestgreen"), text.font=2)
}

plot data

gaiaCNVplot(RecCNV, threshold, "A")

Kevin