Hi,
I am trying to phase genotyping data (Plink format file) for imputation later. But I have an alignment problem between my data and the reference data set , because of it the most of my SNPs are excluded ...
Is there any thing to do to avoid losing data ?
Edit June 7, 2020:
The code below is for pre-phasing with SHAPEIT2. For phased imputation using the output of SHAPEIT2 and ultimate production of phased VCFs, see my answer here: A: ERROR: You must specify a valid interval for imputation using the -int argument,
So, the steps are usually:
Thanks - good to know that there is now a GRCh38 version of that data! - I utilise GRCh37, here: Produce PCA bi-plot for 1000 Genomes Phase III - Version 2
If your Illumina microarray is a special design, then it may only target very specific regions and have minimal overlap.
Otherwise, as mentioned, the use of SHAPEIT involves a 3 step process:
-check)check)for chr in X {1..22}; do
plink --bfile MyData --chr "${chr}" --make-bed --out temp
if [ "${chr}" != "X" ]
then
srun --mem=8 --cpus-per-task=4 --partition=serial \
shapeit \
-check \
-B temp \
-M library/1000GP_Phase3/genetic_map_chr"${chr}"_combined_b37.txt \
--input-ref library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".hap.gz library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".legend.gz library/1000GP_Phase3/1000GP_Phase3.sample \
--output-log Prephased/MyData_chr"${chr}"_alignments \
-T 8 ;
fi
done ;
rm temp.* ;
This should generate files with extensions _alignments.snp.strand.exclude. Use these in the next step via --exclude-snp:
for chr in X {1..22}; do
plink --bfile MyData --chr "${chr}" --make-bed --out temp
if [ "${chr}" != "X" ]
then
srun --mem=8 --cpus-per-task=4 --partition=serial \
shapeit \
-check \
-B temp \
-M library/1000GP_Phase3/genetic_map_chr"${chr}"_combined_b37.txt \
--input-ref library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".hap.gz library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".legend.gz library/1000GP_Phase3/1000GP_Phase3.sample \
--exclude-snp Prephased/MyData_chr"${chr}"_alignments.snp.strand.exclude \
-T 8 ;
fi
done ;
rm temp.* ;
This should now run to completion and not return any error.
NB - this does not actually remove the variants from your data. It just excludes them when SHAPEIT is trying to determine the alignment between your data and the reference. If this command runs to completion without error, then you can proceed to the next step, #3
Here, we again instruct SHAPEIT to not include the problematic variants. Ultimately, these will therefore be lost from the dataset from this point.
for chr in X {1..22}; do
plink --bfile MyData --chr "${chr}" --make-bed --out temp
if [ "${chr}" != "X" ]
then
srun --mem=12 --cpus-per-task=8 --partition=serial \
shapeit \
-B temp \
-M library/1000GP_Phase3/genetic_map_chr"${chr}"_combined_b37.txt \
--input-ref library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".hap.gz library/1000GP_Phase3/1000GP_Phase3_chr"${chr}".legend.gz library/1000GP_Phase3/1000GP_Phase3.sample \
--exclude-snp Prephased/GSA_QCd_chr"${chr}"_alignments.snp.strand.exclude \
-O Prephased/MyData_chr"${chr}"_1KGphased \
-T 8 ;
fi
done ;
rm temp.* ;
Hi Kevin,
Thanks so much for your time and examples. I have a question about Step 1 . I get both
ERROR: Reference and Main panels are not well aligned:
and
ERROR: Duplicate site pos=5961743 ref=T alt=TCAAAA
the later inhibits the production of a .snp.strand.exclude file for the chromosome. Are both errors expected? I'm assuming no since in Step 2 errors are still thrown since some files cannot be opened (they weren't ever made). I'm using the same reference data, for example, 1000GP_Phase3_chr${i}.legend.gz and my study data is in the GRCh37 build.
Thank you!
Thank you for your extremely useful guide on pre-phasing using SHAPEITv2. I have about 1300 trios that I am pre-phasing and I run into very high (>5-10%) rates of Mendelian errors with all of them. I have already checked for kinship using KING and they are definitely correctly annotated parenthoods. Sharing a snippet of my log file at step 2. Do you think this is expected? Or is there a way to solve this? They arise whether I use a reference panel or not.
Additionally, I have filtered to remove duplicates, and only include biallelic SNPs with missingness rate <10% as QC.
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version 2.3.6
Have you tried to flip the SNPs that are discordant between your data and your reference (e.g.: --flip function in PLINK) and see if fewer SNPs are excluded?
thank you I will try this
What is the source of the data that you are imputing, and what is the reference panel? Also, can you share the command(s) that you are using? I have recently completed 2 imputations - for each, I ran 3 separate SHAPEIT commands in order to ensure that the data was correctly pre-phased.
Hi Kevin, It's a genotyping data from Illumina chip, Its 37 buit but I did the liftover to 38. Firstly I run the check command with shapeit to compare my data to reference panel (1000 genomes) and this step infom me that a lot of SNPs (for example for chr1 more 30000 will be excluded...) Thank you for your help
I see - thank you! From where did you obtain the 1000 Genomes data? - most data that is available is GRCh37.
This link : http://ftp.1000genomes.ebi.ac.uk/vol1/ftp/data_collections/1000_genomes_project/release/20190312_biallelic_SNV_and_INDEL/