Last updated: 2021-07-29

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Follow outlined GenomicPredictionChecklist and previous pipeline to process cassavabase data for ultimate genomic prediction.

Below we will clean and format training data.

  • Inputs: “Raw” field trial data
  • Expected outputs: “Cleaned” field trial data

[User input] Cassavabase download

Downloaded all IITA field trials.

  1. Cassavabase search wizard:

  2. Selected all IITA trials currently available. Make a list. Named it ALL_IITA_TRIALS_2021May04.

  3. Go to Manage –> Download here. Download phenotypes (plot-basis only) and meta-data as CSV using the corresponding boxes / drop-downs.

  4. Store flatfiles, unaltered in directory data/DatabaseDownload_2021May04/.

rm(list=ls())
library(tidyverse); library(magrittr);
source(here::here("code","gsFunctions.R"))

Read DB data.

dbdata<-readDBdata(phenotypeFile = here::here("data/DatabaseDownload_2021May04"
                                              ,"2021-05-04T193557phenotype_download.csv"),
                  metadataFile = here::here("data/DatabaseDownload_2021May04"
                                              ,"2021-05-04T194847metadata_download.csv"))

Group and select trials to analyze

Make TrialType Variable

dbdata<-makeTrialTypeVar(dbdata) 
dbdata %>% 
  count(TrialType) %>% rmarkdown::paged_table()

Trials NOT included

Looking at the studyName’s of trials getting NA for TrialType, which can’t be classified at present.

Here is the list of trials I am not including.

dbdata %>% filter(is.na(TrialType)) %$% unique(studyName) %>% 
  write.csv(.,file = here::here("output","IITA_trials_NOT_identifiable.csv"), row.names = F)

Wrote to disk a CSV in the output/ sub-directory.

Should any of these trials have been included?

Especially among the following new trials (post 2018):

dbdata %>% 
  filter(is.na(TrialType),
         as.numeric(studyYear)>2018) %$% unique(studyName)

Remove unclassified trials

dbdata %<>% 
    filter(!is.na(TrialType)) 
dbdata %>% 
    group_by(programName) %>% 
    summarize(N=n()) %>% rmarkdown::paged_table()
#   May 2021:   524390 (now including a ~200K plot seedling nursery) plots
## Dec 2020: 475097 plots (~155K are seedling nurseries which will be excluded from most analyses)

Traits and TraitAbbreviations

Making a table of abbreviations for renaming. Since July 2019 version: added chromometer traits (L, a, b) and added branching levels count (BRLVLS) at IYR’s request.

traitabbrevs<-tribble(~TraitAbbrev,~TraitName,
        "CMD1S","cassava.mosaic.disease.severity.1.month.evaluation.CO_334.0000191",
        "CMD3S","cassava.mosaic.disease.severity.3.month.evaluation.CO_334.0000192",
        "CMD6S","cassava.mosaic.disease.severity.6.month.evaluation.CO_334.0000194",
        "CMD9S","cassava.mosaic.disease.severity.9.month.evaluation.CO_334.0000193",
        "CGM","Cassava.green.mite.severity.CO_334.0000033",
        "CGMS1","cassava.green.mite.severity.first.evaluation.CO_334.0000189",
        "CGMS2","cassava.green.mite.severity.second.evaluation.CO_334.0000190",
        "DM","dry.matter.content.percentage.CO_334.0000092",
        "PLTHT","plant.height.measurement.in.cm.CO_334.0000018",
        "BRNHT1","first.apical.branch.height.measurement.in.cm.CO_334.0000106",
        "BRLVLS","branching.level.counting.CO_334.0000079",
        "SHTWT","fresh.shoot.weight.measurement.in.kg.per.plot.CO_334.0000016",
        "RTWT","fresh.storage.root.weight.per.plot.CO_334.0000012",
        "RTNO","root.number.counting.CO_334.0000011",
        "TCHART","total.carotenoid.by.chart.1.8.CO_334.0000161",
        "LCHROMO","L.chromometer.value.CO_334.0002065",
        "ACHROMO","a.chromometer.value.CO_334.0002066",
        "BCHROMO","b.chromometer.value.CO_334.0002064",
        "NOHAV","plant.stands.harvested.counting.CO_334.0000010")
traitabbrevs %>% rmarkdown::paged_table()

Run function renameAndSelectCols() to rename columns and remove everything unecessary

dbdata<-renameAndSelectCols(traitabbrevs,indata=dbdata,customColsToKeep = c("TrialType","observationUnitName"))

QC Trait values

dbdata<-dbdata %>% 
  mutate(CMD1S=ifelse(CMD1S<1 | CMD1S>5,NA,CMD1S),
         CMD3S=ifelse(CMD3S<1 | CMD3S>5,NA,CMD3S),
         CMD6S=ifelse(CMD6S<1 | CMD6S>5,NA,CMD6S), 
         CMD9S=ifelse(CMD9S<1 | CMD9S>5,NA,CMD9S),
         CGM=ifelse(CGM<1 | CGM>5,NA,CGM),
         CGMS1=ifelse(CGMS1<1 | CGMS1>5,NA,CGMS1),
         CGMS2=ifelse(CGMS2<1 | CGMS2>5,NA,CGMS2),
         DM=ifelse(DM>100 | DM<=0,NA,DM),
         RTWT=ifelse(RTWT==0 | NOHAV==0 | is.na(NOHAV),NA,RTWT),
         SHTWT=ifelse(SHTWT==0 | NOHAV==0 | is.na(NOHAV),NA,SHTWT),
         RTNO=ifelse(RTNO==0 | NOHAV==0 | is.na(NOHAV),NA,RTNO),
         NOHAV=ifelse(NOHAV==0,NA,NOHAV),
         NOHAV=ifelse(NOHAV>42,NA,NOHAV),
         RTNO=ifelse(!RTNO %in% 1:10000,NA,RTNO))

Post-QC traits

Harvest index

dbdata<-dbdata %>% 
    mutate(HI=RTWT/(RTWT+SHTWT))

Unit area traits

I anticipate this will not be necessary as it will be computed before or during data upload.

For calculating fresh root yield:

  1. PlotSpacing: Area in \(m^2\) per plant. plotWidth and plotLength metadata would hypothetically provide this info, but is missing for vast majority of trials. Therefore, use info from Fola.
  2. maxNOHAV: Instead of ExpectedNOHAV. Need to know the max number of plants in the area harvested. For some trials, only the inner (or “net”) plot is harvested, therefore the PlantsPerPlot meta-variable will not suffice. Besides, the PlantsPerPlot information is missing for the vast majority of trials. Instead, use observed max(NOHAV) for each trial. We use this plus the PlotSpacing to calc. the area over which the RTWT was measured. During analysis, variation in the actual number of plants harvested will be accounted for.
dbdata<-dbdata %>% 
    mutate(PlotSpacing=ifelse(programName!="IITA",1,
                              ifelse(studyYear<2013,1,
                              ifelse(TrialType %in% c("CET","GeneticGain","ExpCET"),1,0.8))))
maxNOHAV_byStudy<-dbdata %>% 
  group_by(programName,locationName,studyYear,studyName,studyDesign) %>% 
  summarize(MaxNOHAV=max(NOHAV, na.rm=T)) %>% 
  ungroup() %>% 
  mutate(MaxNOHAV=ifelse(MaxNOHAV=="-Inf",NA,MaxNOHAV))

write.csv(maxNOHAV_byStudy %>% arrange(studyYear),file=here::here("output","maxNOHAV_byStudy.csv"), row.names = F)
# I log transform yield traits 
# to satisfy homoskedastic residuals assumption 
# of linear mixed models
dbdata<-left_join(dbdata,maxNOHAV_byStudy) %>% 
  mutate(RTWT=ifelse(NOHAV>MaxNOHAV,NA,RTWT),
         SHTWT=ifelse(NOHAV>MaxNOHAV,NA,SHTWT),
         RTNO=ifelse(NOHAV>MaxNOHAV,NA,RTNO),
         HI=ifelse(NOHAV>MaxNOHAV,NA,HI),
         FYLD=RTWT/(MaxNOHAV*PlotSpacing)*10,
         DYLD=FYLD*(DM/100),
         logFYLD=log(FYLD),
         logDYLD=log(DYLD),
         logTOPYLD=log(SHTWT/(MaxNOHAV*PlotSpacing)*10),
         logRTNO=log(RTNO),
         PropNOHAV=NOHAV/MaxNOHAV) 
# remove non transformed / per-plot (instead of per area) traits
dbdata %<>% select(-RTWT,-SHTWT,-RTNO,-FYLD,-DYLD)

Season-wide mean disease severity

# [NEW AS OF APRIL 2021]
## VERSION with vs. without CBSD
## Impervious to particular timepoints between 1, 3, 6 and 9 scores

# Without CBSD (West Africa)
dbdata<-dbdata %>% 
  mutate(MCMDS=rowMeans(.[,colnames(.) %in% c("CMD1S","CMD3S","CMD6S","CMD9S")], na.rm = T)) %>% 
  select(-any_of(c("CMD1S","CMD3S","CMD6S","CMD9S")))

# With CBSD (East Africa)
# dbdata<-dbdata %>% 
#   mutate(MCMDS=rowMeans(.[,colnames(.) %in% c("CMD1S","CMD3S","CMD6S","CMD9S")], na.rm = T),
#          MCBSDS=rowMeans(.[,colnames(.) %in% c("CBSD1S","CBSD3S","CBSD6S","CBSD9S")], na.rm = T)) %>% 
#   select(-any_of(c("CMD1S","CMD3S","CMD6S","CMD9S","CBSD1S","CBSD3S","CBSD6S","CBSD9S")))

[User input] Assign genos to phenos

This step is mostly copy-pasted from previous processing of IITA- and IITA-specific data.

Uses 4 flat files, which are available e.g. here. Specifically, IITA_GBStoPhenoMaster_33018.csv, GBSdataMasterList_31818.csv and IITA_GBStoPhenoMaster_40318.csv and chr1_RefPanelAndGSprogeny_ReadyForGP_72719.fam. I copy them to the data/ sub-directory for the current analysis.

In addition, DArT-only samples are now expected to also have phenotypes. Therefore, checking for matches in new flatfiles, deposited in the data/ (see code below).

library(tidyverse); library(magrittr)
gbs2phenoMaster<-dbdata %>% 
  select(germplasmName) %>% 
  distinct %>% 
  left_join(read.csv(here::here("data","NRCRI_GBStoPhenoMaster_40318.csv"), 
                     stringsAsFactors = F)) %>% 
  mutate(FullSampleName=ifelse(grepl("C2a",germplasmName,ignore.case = T) & 
                                 is.na(FullSampleName),germplasmName,FullSampleName)) %>% 
  filter(!is.na(FullSampleName)) %>% 
  select(germplasmName,FullSampleName) %>% 
  bind_rows(dbdata %>% 
              select(germplasmName) %>% 
              distinct %>% 
              left_join(read.csv(here::here("data","IITA_GBStoPhenoMaster_33018.csv"), 
                                 stringsAsFactors = F)) %>% 
              filter(!is.na(FullSampleName)) %>% 
              select(germplasmName,FullSampleName)) %>% 
  bind_rows(dbdata %>% 
              select(germplasmName) %>% 
              distinct %>% 
              left_join(read.csv(here::here("data","GBSdataMasterList_31818.csv"), 
                                 stringsAsFactors = F) %>% 
                          select(DNASample,FullSampleName) %>% 
                          rename(germplasmName=DNASample)) %>% 
              filter(!is.na(FullSampleName)) %>% 
              select(germplasmName,FullSampleName)) %>% 
  bind_rows(dbdata %>% 
              select(germplasmName) %>% 
              distinct %>% 
              mutate(germplasmSynonyms=ifelse(grepl("^UG",germplasmName,ignore.case = T),
                                              gsub("UG","Ug",germplasmName),germplasmName)) %>% 
              left_join(read.csv(here::here("data","GBSdataMasterList_31818.csv"), 
                                 stringsAsFactors = F) %>% 
                          select(DNASample,FullSampleName) %>% 
                          rename(germplasmSynonyms=DNASample)) %>% 
              filter(!is.na(FullSampleName)) %>% 
              select(germplasmName,FullSampleName)) %>%  
  bind_rows(dbdata %>% 
              select(germplasmName) %>% 
              distinct %>% 
              mutate(germplasmSynonyms=ifelse(grepl("^TZ",germplasmName,
                                                    ignore.case = T),
                                              gsub("TZ","",germplasmName),germplasmName)) %>% 
              left_join(read.csv(here::here("data","GBSdataMasterList_31818.csv"), 
                                 stringsAsFactors = F) %>% 
                          select(DNASample,FullSampleName) %>% 
                          rename(germplasmSynonyms=DNASample)) %>% 
              filter(!is.na(FullSampleName)) %>%
              select(germplasmName,FullSampleName)) %>% 
  distinct %>% 
  left_join(read.csv(here::here("data","GBSdataMasterList_31818.csv"), 
                     stringsAsFactors = F) %>% 
              select(FullSampleName,OrigKeyFile,Institute) %>% 
              rename(OriginOfSample=Institute)) %>% 
  mutate(OrigKeyFile=ifelse(grepl("C2a",germplasmName,ignore.case = T),
                            ifelse(is.na(OrigKeyFile),"LavalGBS",OrigKeyFile),
                            OrigKeyFile),
         OriginOfSample=ifelse(grepl("C2a",germplasmName,ignore.case = T),
                               ifelse(is.na(OriginOfSample),"NRCRI",OriginOfSample),
                               OriginOfSample))

## NEW: check for germName-DArT name matches
germNamesWithoutGBSgenos<-dbdata %>% 
  select(programName,germplasmName) %>% 
  distinct %>% 
  left_join(gbs2phenoMaster) %>% 
  filter(is.na(FullSampleName)) %>% 
  select(-FullSampleName)
## NEW: check for germName-DArT name matches
germNamesWithoutGBSgenos<-dbdata %>% 
  select(programName,germplasmName) %>% 
  distinct %>% 
  left_join(gbs2phenoMaster) %>% 
  filter(is.na(FullSampleName)) %>% 
  select(-FullSampleName)

germNamesWithDArT<-germNamesWithoutGBSgenos %>% 
  inner_join(read.table(here::here("data","chr1_RefPanelAndGSprogeny_ReadyForGP_72719.fam"), 
                        header = F, stringsAsFactors = F)$V2 %>% 
               grep("TMS16|TMS17|TMS18|TMS19|TMS20",.,value = T, ignore.case = T) %>% 
               tibble(dartName=.) %>% 
               separate(dartName,c("germplasmName","dartID"),"_",extra = 'merge',remove = F)) %>% 
  group_by(germplasmName) %>% 
  slice(1) %>% 
  ungroup() %>% 
  rename(FullSampleName=dartName) %>% 
  mutate(OrigKeyFile="DArTseqLD", OriginOfSample="IITA") %>% 
  select(-dartID)
print(paste0(nrow(germNamesWithDArT)," germNames with DArT-only genos"))

# first, filter to just program-DNAorigin matches
germNamesWithGenos<-dbdata %>% 
  select(programName,germplasmName) %>% 
  distinct %>% 
  left_join(gbs2phenoMaster) %>% 
  filter(!is.na(FullSampleName))
print(paste0(nrow(germNamesWithGenos)," germNames with GBS genos"))

# program-germNames with locally sourced GBS samples
germNamesWithGenos_HasLocalSourcedGBS<-germNamesWithGenos %>% 
  filter(programName==OriginOfSample) %>% 
  select(programName,germplasmName) %>% 
  semi_join(germNamesWithGenos,.) %>% 
  group_by(programName,germplasmName) %>% # select one DNA per germplasmName per program
  slice(1) %>% ungroup() 
print(paste0(nrow(germNamesWithGenos_HasLocalSourcedGBS)," germNames with local GBS genos"))

# the rest (program-germNames) with GBS but coming from a different breeding program
germNamesWithGenos_NoLocalSourcedGBS<-germNamesWithGenos %>% 
  filter(programName==OriginOfSample) %>% 
  select(programName,germplasmName) %>% 
  anti_join(germNamesWithGenos,.) %>% 
  # select one DNA per germplasmName per program
  group_by(programName,germplasmName) %>% 
  slice(1) %>% ungroup() 
print(paste0(nrow(germNamesWithGenos_NoLocalSourcedGBS)," germNames without local GBS genos"))

genosForPhenos<-bind_rows(germNamesWithGenos_HasLocalSourcedGBS,
                        germNamesWithGenos_NoLocalSourcedGBS) %>% 
  bind_rows(germNamesWithDArT)

print(paste0(nrow(genosForPhenos)," total germNames with genos either GBS or DArT"))

dbdata %<>% 
    left_join(genosForPhenos) 

# Create a new identifier, GID
## Equals the value SNP data name (FullSampleName) 
## else germplasmName if no SNP data
dbdata %<>% 
  mutate(GID=ifelse(is.na(FullSampleName),germplasmName,FullSampleName))
# # going to check against SNP data
# snps<-readRDS(file=url(paste0("ftp://ftp.cassavabase.org/marnin_datasets/NGC_BigData/",
#                               "DosageMatrix_RefPanelAndGSprogeny_ReadyForGP_73019.rds")))
# rownames_snps<-rownames(snps); rm(snps); gc()
# # current matches to SNP data
# dbdata %>%
#   distinct(GID,germplasmName,FullSampleName) %>%
#   semi_join(tibble(GID=rownames_snps)) %>% nrow() # 10707
# dbdata %>%
#   distinct(GID,germplasmName,FullSampleName) %>%
#   semi_join(tibble(GID=rownames_snps)) %>%
#   filter(grepl("TMS13|2013_",GID,ignore.case = F)) %>% nrow() # 2424 TMS13
# dbdata %>%
#   distinct(GID,germplasmName,FullSampleName) %>%
#   semi_join(tibble(GID=rownames_snps)) %>%
#   filter(grepl("TMS14",GID,ignore.case = F)) %>% nrow() # 2236 TMS14
# dbdata %>%
#   distinct(GID,germplasmName,FullSampleName) %>%
#   semi_join(tibble(GID=rownames_snps)) %>%
#   filter(grepl("TMS15",GID,ignore.case = F)) %>% nrow() # 2287 TMS15
# dbdata %>%
#   distinct(GID,germplasmName,FullSampleName) %>%
#   semi_join(tibble(GID=rownames_snps)) %>%
#   filter(grepl("TMS18",GID,ignore.case = F)) %>% nrow() # 2401 TMS18

[User input] Choose locations

WARNING: User input required! If I had preselected locations before downloading, this wouldn’t have been necessary.

Based on previous locations used for IITA analysis, but adding based on list of locations used in IYR’s trial list data/2019_GS_PhenoUpload.csv: “Ago-Owu” wasn’t used last year.

dbdata %<>% 
  filter(locationName %in% c("Abuja","Ago-Owu","Ibadan","Ikenne","Ilorin","Jos","Kano",
                             "Malam Madori","Mokwa","Ubiaja","Umudike","Warri","Zaria"))
nrow(dbdata) # [1] 479588

Output “cleaned” file

saveRDS(dbdata,file=here::here("output","IITA_CleanedTrialData_2021May10.rds"))

Detect experimental designs

The next step is to check the experimental design of each trial. If you are absolutely certain of the usage of the design variables in your dataset, you might not need this step.

Examples of reasons to do the step below:

  • Some trials appear to be complete blocked designs and the blockNumber is used instead of replicate, which is what most use.
  • Some complete block designs have nested, incomplete sub-blocks, others simply copy the “replicate” variable into the “blockNumber variable”
  • Some trials have only incomplete blocks but the incomplete block info might be in the replicate and/or the blockNumber column

One reason it might be important to get this right is that the variance among complete blocks might not be the same among incomplete blocks. If we treat a mixture of complete and incomplete blocks as part of the same random-effect (replicated-within-trial), we assume they have the same variance.

Also error variances might be heterogeneous among different trial-types (blocking scheme available) and/or plot sizes (maxNOHAV).

Start with cleaned data from previous step.

rm(list=ls()); gc()
library(tidyverse); library(magrittr);
source(here::here("code","gsFunctions.R"))
dbdata<-readRDS(here::here("output","IITA_CleanedTrialData_2021May10.rds"))
dbdata %>% head %>% rmarkdown::paged_table()

Detect designs

dbdata<-detectExptDesigns(dbdata)
dbdata %>% 
    count(programName,CompleteBlocks,IncompleteBlocks) %>% rmarkdown::paged_table()

Output file

saveRDS(dbdata,file=here::here("output","IITA_ExptDesignsDetected_2021May10.rds"))

Next step

  1. Get BLUPs combining all trial data: Combine data from all trait-trials to get BLUPs for downstream genomic prediction. Fit mixed-model to multi-trial dataset and extract BLUPs, de-regressed BLUPs and weights. Include two rounds of outlier removal.

sessionInfo()