Last updated: 2022-04-06
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Knit directory: Serreze-T1D_Workflow/
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Unstaged changes:
Modified: analysis/4.1.1_qtl.analysis_binary_ici.vs.eoi_snpsqc_dis_no-x_updated.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici.vs.pbs_snpsqc_dis_no-x_updated.Rmd
Note that any generated files, e.g. HTML, png, CSS, etc., are not included in this status report because it is ok for generated content to have uncommitted changes.
There are no past versions. Publish this analysis with wflow_publish()
to start tracking its development.
load("data/e_snpg_samqc_5.batches.RData")
gm <- get(load("data/gm_samqc_5.batches.RData"))
gm
Object of class cross2 (crosstype "bc")
Total individuals 308
No. genotyped individuals 308
No. phenotyped individuals 308
No. with both geno & pheno 308
No. phenotypes 1
No. covariates 6
No. phenotype covariates 0
No. chromosomes 20
Total markers 133716
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13
10159 10172 7987 7736 7778 7911 7548 6561 6823 6472 7276 6226 6177
14 15 16 17 18 19 X
6082 5421 5075 5161 4682 3612 4857
It can also be useful to look at the proportion of missing genotypes by marker. Markers with a lot of missing data were likely difficult to call, and so the genotypes that were called may contain a lot of errors.
pmis_mar <- n_missing(gm, "marker", "proportion")*100
save(pmis_mar, file = "data/percent_missing_marker_5.batches.RData")
par(mar=c(5.1,0.6,0.6, 0.6))
hist(pmis_mar, breaks=seq(0, 100, length=201),
main="", yaxt="n", ylab="", xlab="Percent missing genotypes")
rug(pmis_mar)
pdf(file = "output/Percent_missing_genotype_data_per_marker_5.batches.pdf")
par(mar=c(5.1,0.6,0.6, 0.6))
hist(pmis_mar, breaks=seq(0, 100, length=201),
main="", yaxt="n", ylab="", xlab="Percent missing genotypes")
rug(pmis_mar)
dev.off()
quartz_off_screen
2
count | |
---|---|
pmis_mar_5 | 3362 |
pmis_mar_10 | 2360 |
pmis_mar_15 | 1840 |
pmis_mar_25 | 1208 |
pmis_mar_50 | 334 |
pmis_mar_75 | 65 |
total_snps | 133716 |
g <- do.call("cbind", gm$geno[1:19])
#fg <- do.call("cbind", gm$founder_geno[1:19])
#g <- g[,colSums(g)!=0]
#fg <- fg[,colSums(fg==0)==0]
#fgn <- colSums(g==2)
gf_mar <- t(apply(g, 2, function(a) table(factor(a, 1:2))/sum(a != 0)))
gn_mar <- t(apply(g, 2, function(a) table(factor(a, 1:2))))
gf_mar <- gf_mar[gf_mar[,2] != "NaN",]
MAF <- apply(gf_mar, 1, function(x) min(x))
MAF <- as.data.frame(MAF)
MAF$index <- 1:nrow(gf_mar)
gf_mar_maf <- merge(gf_mar,as.data.frame(MAF), by="row.names")
gf_mar_maf <- gf_mar_maf[order(gf_mar_maf$index),]
pdf(file = "output/genotype_frequency_marker_5.batches.pdf")
par(mar=c(5.1,0.6,0.6, 0.6))
hist(gf_mar_maf$MAF, breaks=seq(0, 1, length=201),
main="", yaxt="n", ylab="", xlab="MAF")
rug(gf_mar_maf$MAF)
dev.off()
quartz_off_screen
2
par(mar=c(5.1,0.6,0.6, 0.6))
hist(gf_mar_maf$MAF, breaks=seq(0, 1, length=201),
main="", yaxt="n", ylab="", xlab="MAF")
rug(gf_mar_maf$MAF)
gfmar <- NULL
gfmar$gfmar_mar_0 <- sum(gf_mar_maf$MAF==0)
gfmar$gfmar_mar_1 <- sum(gf_mar_maf$MAF< 0.01)
gfmar$gfmar_mar_5 <- sum(gf_mar_maf$MAF< 0.05)
gfmar$gfmar_mar_10 <- sum(gf_mar_maf$MAF< 0.10)
gfmar$gfmar_mar_15 <- sum(gf_mar_maf$MAF< 0.15)
gfmar$gfmar_mar_25 <- sum(gf_mar_maf$MAF< 0.25)
gfmar$gfmar_mar_50 <- sum(gf_mar_maf$MAF<= 0.50)
gfmar$total_snps <- nrow(as.data.frame(gf_mar_maf))
gfmar <- t(as.data.frame(gfmar))
gfmar <- as.data.frame(gfmar)
gfmar$count <- gfmar$V1
gfmar[c(2)] %>%
kable(escape = F,align = c("ccccccccc"),linesep ="\\hline") %>%
kable_styling(full_width = F) %>%
kable_styling("striped", full_width = F) %>%
row_spec(8 ,bold=T,color= "white",background = "black")
count | |
---|---|
gfmar_mar_0 | 84737 |
gfmar_mar_1 | 91037 |
gfmar_mar_5 | 95845 |
gfmar_mar_10 | 96139 |
gfmar_mar_15 | 96351 |
gfmar_mar_25 | 97125 |
gfmar_mar_50 | 128857 |
total_snps | 128857 |
save(gf_mar, file = "data/genotype_freq_marker_5.batches.RData")
errors_mar <- colSums(e>2)/n_typed(gm, "marker")*100
grayplot(pmis_mar, errors_mar,
xlab="Proportion missing", ylab="Proportion genotyping errors")
pdf(file = "output/genotype_error_marker_5.batches.pdf")
grayplot(pmis_mar, errors_mar,
xlab="Proportion missing", ylab="Proportion genotyping errors")
dev.off()
quartz_off_screen
2
save(errors_mar, file = "data/genotype_errors_marker_5.batches.RData")
Markers with higher rates of missing genotypes tend to show higher errors rates.
#Missingness
length(pmis_mar[pmis_mar >= 10])
[1] 2360
high_miss <- find_markerpos(gm, names(pmis_mar[pmis_mar >= 10]))
high_miss$id <- rownames(high_miss)
high_miss_df <- as.data.frame(pmis_mar[pmis_mar >= 10])
high_miss_df$index = 1: nrow(high_miss_df)
high_miss_df$id <- rownames(high_miss_df)
high_miss_bad <- merge(high_miss,high_miss_df, by=c("id"),all=T)
names(high_miss_bad)[5] <- c("high_miss")
names(high_miss_bad)[1] <- c("marker")
high_miss_bad <- high_miss_bad[order(high_miss_bad$index),]
#Monomorphic/Low Frequency markers
#low_freq_df <- as.data.frame(gf_mar)
count <- rowSums(gf_mar <= 0.01)
#count <- as.data.frame(count)
low_freq_df <- merge(as.data.frame(gf_mar),as.data.frame(count), by="row.names",all=T)
low_freq_df[is.na(low_freq_df)] <- ''
low_freq_df <- low_freq_df[low_freq_df$count == 1,]
rownames(low_freq_df) <- low_freq_df$Row.names
#low_freq_df$id <- rownames(low_freq_df)
#low_freq_df$index = 1: nrow(low_freq_df)
low_freq <- find_markerpos(gm, rownames(low_freq_df))
low_freq$id <- rownames(low_freq)
nrow(low_freq)
[1] 91075
low_freq_bad <- merge(low_freq,low_freq_df, by="row.names",all=T)
#names(low_freq_bad)[5] <- c("AA_freq")
#names(low_freq_bad)[6] <- c("AB_freq")
#names(low_freq_bad)[7] <- c("BB_freq")
names(low_freq_bad)[1] <- c("marker")
#low_freq_bad <- low_freq_bad[order(low_freq_bad$index),]
##Genotyping Error
length(errors_mar[errors_mar > 5])
[1] 10754
error_markers_names <- names(errors_mar[errors_mar > 5])
error_markers_names <- error_markers_names[complete.cases(error_markers_names)]
error_markers <- find_markerpos(gm, error_markers_names)
error_markers$id <- rownames(error_markers)
#rne <- rownames(as.data.frame(errors_mar))
error_mars_df <- as.data.frame(errors_mar[errors_mar > 5])
error_mars_df <- error_mars_df[complete.cases(error_mars_df$"errors_mar[errors_mar > 5]"),]
error_mars_df <- as.data.frame(error_mars_df)
#error_mars_df$id = rownames(error_mars_df)
error_mars_df$index = 1: nrow(error_mars_df)
#error_markers_bad <- merge(error_markers,error_mars_df, by=c("id"),all=T)
error_markers_bad <- cbind(error_markers,error_mars_df)
names(error_markers_bad)[5] <- c("error_mars")
names(error_markers_bad)[4] <- c("marker")
error_markers_bad <- error_markers_bad[order(error_markers_bad$index),]
### merge all
bad_markers <- rbind(high_miss_bad[c("marker","chr","gmap","pmap")], low_freq_bad[c("marker","chr","gmap","pmap")], error_markers_bad[c("marker","chr","gmap","pmap")])
#nrow(bad_markers)
duplicate <- bad_markers[duplicated(bad_markers),]
bad_markers <- bad_markers[!duplicated(bad_markers),]
nrow(bad_markers)
[1] 99179
save(bad_markers, file = "data/bad_markers_all_5.batches.RData")
Only removing markers that are missing in at least 10% of the samples
#missing in at least 10% of the samples
gm_allqc2 <- drop_markers(gm_samqc, high_miss_bad$marker)
gm_allqc <- drop_nullmarkers(gm_allqc2)
gm_allqc
Object of class cross2 (crosstype "bc")
Total individuals 308
No. genotyped individuals 308
No. phenotyped individuals 308
No. with both geno & pheno 308
No. phenotypes 1
No. covariates 6
No. phenotype covariates 0
No. chromosomes 20
Total markers 131356
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16
9956 9987 7848 7586 7609 7736 7399 6458 6713 6385 7143 6110 6082 5966 5346 5015
17 18 19 X
5080 4605 3562 4770
save(gm_allqc, file = "data/gm_allqc_5.batches_mis.RData")
sessionInfo()
R version 3.6.2 (2019-12-12)
Platform: x86_64-apple-darwin15.6.0 (64-bit)
Running under: macOS Catalina 10.15.7
Matrix products: default
BLAS: /Library/Frameworks/R.framework/Versions/3.6/Resources/lib/libRblas.0.dylib
LAPACK: /Library/Frameworks/R.framework/Versions/3.6/Resources/lib/libRlapack.dylib
locale:
[1] en_AU.UTF-8/en_AU.UTF-8/en_AU.UTF-8/C/en_AU.UTF-8/en_AU.UTF-8
attached base packages:
[1] stats graphics grDevices utils datasets methods base
other attached packages:
[1] fst_0.9.2 knitr_1.33 kableExtra_1.1.0 mclust_5.4.6
[5] ggrepel_0.8.2 ggplot2_3.3.5 qtlcharts_0.11-6 qtl2_0.22
[9] broman_0.70-4 workflowr_1.6.2
loaded via a namespace (and not attached):
[1] Rcpp_1.0.7 assertthat_0.2.1 rprojroot_1.3-2 digest_0.6.27
[5] utf8_1.2.1 R6_2.5.0 backports_1.2.1 RSQLite_2.2.7
[9] evaluate_0.14 httr_1.4.1 highr_0.9 pillar_1.6.1
[13] rlang_1.0.2 rstudioapi_0.13 data.table_1.14.0 blob_1.2.1
[17] rmarkdown_2.1 qtl_1.46-2 webshot_0.5.2 readr_1.3.1
[21] stringr_1.4.0 bit_4.0.4 munsell_0.5.0 compiler_3.6.2
[25] httpuv_1.5.2 xfun_0.24 pkgconfig_2.0.3 htmltools_0.5.1.1
[29] tidyselect_1.1.2 tibble_3.1.2 fansi_0.5.0 viridisLite_0.4.0
[33] crayon_1.4.1 dplyr_1.0.8 withr_2.4.2 later_1.0.0
[37] grid_3.6.2 gtable_0.3.0 lifecycle_1.0.1 DBI_1.1.1
[41] git2r_0.26.1 magrittr_2.0.1 scales_1.1.1 cli_3.0.0
[45] stringi_1.7.2 cachem_1.0.5 fs_1.4.1 promises_1.1.0
[49] xml2_1.3.1 ellipsis_0.3.2 generics_0.0.2 vctrs_0.3.8
[53] tools_3.6.2 bit64_4.0.5 glue_1.4.2 purrr_0.3.4
[57] hms_0.5.3 parallel_3.6.2 fastmap_1.1.0 yaml_2.2.1
[61] colorspace_2.0-2 rvest_0.3.5 memoise_2.0.0