Worked Example: PCA on SNPs data from a vcf file Part 1 - Data Preparation

Introduction

In this worked example you will replicate a PCA on a published dataset.

The example is split into 2 Parts:

• Part 1: Data Preparation (this file)
• Part 2: Data analysis with PCA

In this Data Preparation phase, you will do the following things:

1. Load the SNP genotypes in .vcf format (vcfR::read.vcfR())
2. Extract the genotypes into an R-compatible format (vcfR::extract.gt())
3. Rotate the data into the standard R analysis format (t())
4. Remove individuals (rows) from the data set that have >50% NAs (using a function I wrote)
5. Remove SNPs (columns) that are fixed
6. Impute remaining NAs (using a for() loop)
7. Save the prepared data as a .csv file for the next step (write.csv())

Biological background

This worked example is based on a paper in the journal Molecular Ecology from 2017 by Jennifer Walsh titled Subspecies delineation amid phenotypic, geographic and genetic discordance in a songbird.

The study investigated variation between two bird species in the genus Ammodramus: A. nenlsoni and A. caudacutus.

The species A. nenlsoni has been divided into 3 sub-species: A. n. nenlsoni, A.n. alterus, and A n. subvirgatus. The other species, A. caudacutus, has been divided into two subspecies, A.c. caudacutus and A.c. diversus.

The purpose of this study was to investigate to what extent these five subspecies recognized by taxonomists are supported by genetic data. The author’s collected DNA from 75 birds (15 per subspecies) and genotyped 1929 SNPs. They then analyzed the data with Principal Components Analysis (PCA), among other genetic analyzes.

This tutorial will work through all of the steps necessary to re-analyze Walsh et al.s data

Tasks

In the code below all code is provided. Your tasks will be to do 2 things:

1. Give a meaningful title to all sections marked “TODO: TITLE”
2. Write 1 to 2 sentences describing what is being done and why in all sections marked “TODO: EXPLAIN”

Preliminaries

Load the vcfR and other packages with library().

library(vcfR)    

## 
##    *****       ***   vcfR   ***       *****
##    This is vcfR 1.13.0 
##      browseVignettes('vcfR') # Documentation
##      citation('vcfR') # Citation
##    *****       *****      *****       *****

library(vegan)

## Loading required package: permute

## Loading required package: lattice

## This is vegan 2.6-4

library(ggplot2)
library(ggpubr)

Make sure that your working directory is set to the location of the file all_loci.vcf.

getwd()

## [1] "/Users/BradAngstadt/Downloads"

list.files()

##  [1] "07-mean_imputation.docx"             
##  [2] "07-mean_imputation.html"             
##  [3] "07-mean_imputation.Rmd"              
##  [4] "08-PCA_worked.html"                  
##  [5] "08-PCA_worked.Rmd"                   
##  [6] "09-PCA_worked_example-SNPs-part1.Rmd"
##  [7] "all_loci.vcf"                        
##  [8] "Amy"                                 
##  [9] "bird_snps_remove_NAs.html"           
## [10] "bird_snps_remove_NAs.Rmd"            
## [11] "removing_fixed_alleles.html"         
## [12] "removing_fixed_alleles.Rmd"          
## [13] "rsconnect"                           
## [14] "SNPs_cleaned.csv"                    
## [15] "walsh2017morphology (1).csv"         
## [16] "walsh2017morphology.csv"

list.files(pattern = "vcf")

## [1] "all_loci.vcf"

Data preparation

TODO: upload vcf file

TODO: Have R convert the vcf file to something R can use and we can manipulate. opens it in R

snps <- vcfR::read.vcfR("all_loci.vcf", convertNA  = TRUE)

## Scanning file to determine attributes.
## File attributes:
##   meta lines: 8
##   header_line: 9
##   variant count: 1929
##   column count: 81
## 
Meta line 8 read in.
## All meta lines processed.
## gt matrix initialized.
## Character matrix gt created.
##   Character matrix gt rows: 1929
##   Character matrix gt cols: 81
##   skip: 0
##   nrows: 1929
##   row_num: 0
## 
Processed variant 1000
Processed variant: 1929
## All variants processed

TODO: fatures to numbers

TODO: R takes the snp proteins and converts them to numbers so we can do math.

snps_num <- vcfR::extract.gt(snps, 
           element = "GT",
           IDtoRowNames  = F,
           as.numeric = T,
           convertNA = T,
           return.alleles = F)

TODO: Transpose

TODO: Flips the axis so individuals are rows with genes as columns. Makes R happy

snps_num_t <- t(snps_num) 

TODO: makes a Data frame so we can remove or add features

snps_num_df <- data.frame(snps_num_t) 

TODO: NA finder function

TODO: Creates a function to tell us where NAs are and how many there are in each row.

find_NAs <- function(x){
  NAs_TF <- is.na(x)
  i_NA <- which(NAs_TF == TRUE)
  N_NA <- length(i_NA)
  
  cat("Results:",N_NA, "NAs present\n.")
  return(i_NA)
}

TODO: Uses for() to repeat function for each row and print out how many NAs after assigning a vector to save the values.

# N_rows
# number of rows (individuals)
N_rows <- nrow(snps_num_t)

# N_NA
# vector to hold output (number of NAs)
N_NA   <- rep(x = 0, times = N_rows)

# N_SNPs
# total number of columns (SNPs)
N_SNPs <- ncol(snps_num_t)

# the for() loop
for(i in 1:N_rows){
  
  # for each row, find the location of
  ## NAs with snps_num_t()
  i_NA <- find_NAs(snps_num_t[i,]) 
  
  # then determine how many NAs
  ## with length()
  N_NA_i <- length(i_NA)
  
  # then save the output to 
  ## our storage vector
  N_NA[i] <- N_NA_i
}

## Results: 28 NAs present
## .Results: 20 NAs present
## .Results: 28 NAs present
## .Results: 24 NAs present
## .Results: 23 NAs present
## .Results: 63 NAs present
## .Results: 51 NAs present
## .Results: 38 NAs present
## .Results: 34 NAs present
## .Results: 24 NAs present
## .Results: 48 NAs present
## .Results: 21 NAs present
## .Results: 42 NAs present
## .Results: 78 NAs present
## .Results: 45 NAs present
## .Results: 21 NAs present
## .Results: 42 NAs present
## .Results: 34 NAs present
## .Results: 66 NAs present
## .Results: 54 NAs present
## .Results: 59 NAs present
## .Results: 52 NAs present
## .Results: 47 NAs present
## .Results: 31 NAs present
## .Results: 63 NAs present
## .Results: 40 NAs present
## .Results: 40 NAs present
## .Results: 22 NAs present
## .Results: 60 NAs present
## .Results: 48 NAs present
## .Results: 961 NAs present
## .Results: 478 NAs present
## .Results: 59 NAs present
## .Results: 26 NAs present
## .Results: 285 NAs present
## .Results: 409 NAs present
## .Results: 1140 NAs present
## .Results: 600 NAs present
## .Results: 1905 NAs present
## .Results: 25 NAs present
## .Results: 1247 NAs present
## .Results: 23 NAs present
## .Results: 750 NAs present
## .Results: 179 NAs present
## .Results: 433 NAs present
## .Results: 123 NAs present
## .Results: 65 NAs present
## .Results: 49 NAs present
## .Results: 192 NAs present
## .Results: 433 NAs present
## .Results: 66 NAs present
## .Results: 597 NAs present
## .Results: 1891 NAs present
## .Results: 207 NAs present
## .Results: 41 NAs present
## .Results: 268 NAs present
## .Results: 43 NAs present
## .Results: 110 NAs present
## .Results: 130 NAs present
## .Results: 90 NAs present
## .Results: 271 NAs present
## .Results: 92 NAs present
## .Results: 103 NAs present
## .Results: 175 NAs present
## .Results: 31 NAs present
## .Results: 66 NAs present
## .Results: 64 NAs present
## .Results: 400 NAs present
## .Results: 192 NAs present
## .Results: 251 NAs present
## .Results: 69 NAs present
## .Results: 58 NAs present
## .

TODO: Make a histogram of NA frequency for each gene, 50% is the max amount of NAs in a gene we want

# 50% of N_SNPs
cutoff50 <- N_SNPs*0.5

hist(N_NA)            
abline(v = cutoff50, 
       col = 2, 
       lwd = 2, 
       lty = 2)

TODO: Calculates NA percentage and creates a save without genes above the 50%

percent_NA <- N_NA/N_SNPs*100

# Call which() on percent_NA
i_NA_50percent <- which(percent_NA > 50) 

snps_num_t02 <- snps_num_t[-i_NA_50percent, ]

TODO: Name engineering

TODO: remove unnecessary parts of samples so they are easier to read and view

row_names <- row.names(snps_num_t02) # Key

row_names02 <- gsub("sample_","",row_names)

sample_id <- gsub("^([ATCG]*)(_)(.*)",
                  "\\3",
                  row_names02)
pop_id <- gsub("[01-9]*",    
               "",
               sample_id)

table(pop_id)  

## pop_id
## Alt Cau Div Nel Sub 
##  15  12  15  15  11

TODO: Invariant removal

TODO: Writes a function to omit invariant columns and applies it to reduce load and give better values later

invar_omit <- function(x){
  cat("Dataframe of dim",dim(x), "processed...\n")
  sds <- apply(x, 2, sd, na.rm = TRUE)
  i_var0 <- which(sds == 0)
 
  
  cat(length(i_var0),"columns removed\n")
  
  if(length(i_var0) > 0){
     x <- x[, -i_var0]
  }
  
  ## add return()  with x in it
  return(x)                      
}


snps_no_invar <- invar_omit(snps_num_t02) 

## Dataframe of dim 68 1929 processed...
## 591 columns removed

TODO: mean imputation

TODO: replaces NAs with means of that column and creates new objects

snps_noNAs <- snps_no_invar

N_col <- ncol(snps_no_invar)
for(i in 1:N_col){
  
  # get the current column
  column_i <- snps_noNAs[, i]
  
  # get the mean of the current column
  mean_i <- mean(column_i, na.rm = TRUE)
  
  # get the NAs in the current column
  NAs_i <- which(is.na(column_i))
  
  # record the number of NAs
  N_NAs <- length(NAs_i)

  # replace the NAs in the current column
  column_i[NAs_i] <- mean_i
  
  # replace the original column with the
  ## updated columns
  snps_noNAs[, i] <- column_i
  
}

Save the data

Save the data as a .csv file which can be loaded again later.

write.csv(snps_noNAs, file = "SNPs_cleaned.csv",
          row.names = F)

Check for the presence of the file with list.files()

list.files(pattern = ".csv")

## [1] "SNPs_cleaned.csv"            "walsh2017morphology (1).csv"
## [3] "walsh2017morphology.csv"

Next steps:

In Part 2, we will re-load the SNPs_cleaned.csv file and carry an an analysis with PCA.