You may alreadly have minimap2
and samtools
if you performed analysis of Oxford Nanopore sequencing data. You can use which minimap2
and which samtools
to check the full path to the two executable files. Please note that minimap2
should be v2.22 or later.
Once you installed the above tools, you can use the following commands to install NanoRepeat (we recommend creating an new conda environment to avoid dependency issues):
conda create -n nanorepeat python=3.8
conda activate nanorepeat
git clone https://github.com/WGLab/NanoRepeat.git
cd NanoRepeat
pip install .
If you want to install a stable version from Python Package Index (PyPI):
conda create -n nanorepeat python=3.8
conda activate nanorepeat
pip install NanoRepeat
Notice: If you want to install NanoRepeat from a PyPI mirror, please check if the version in the mirror is update to date.
NanoRepeat can quantify STRs from targeted sequencing or whole-genome sequencing data. We will demonstrate the usage of NanoRepeat using an example data set, which can be downloaded using the following commands.
wget https://github.com/WGLab/NanoRepeat/releases/download/v1.3/NanoRepeat_v1.3_example_data.tar.bz2
tar xjf NanoRepeat_v1.3_example_data.tar.bz2
After unzipping the file, you will see a NanoRepeat_v1.3_example_data
folder and there are two subfolders: HG002
and HTT_amplicon
. In this section, we will use the data under the HG002
folder.
$ ls -1 ./NanoRepeat_v1.3_example_data/HG002/
GRCh37_chr1.fasta
GRCh37_chr1.fasta.fai
HG002_GRCh37_example_regions.bed
hg002_Q20.20210805_3flowcells.hs37d5.example_regions.bam
hg002_Q20.20210805_3flowcells.hs37d5.example_regions.bam.bai
You can use the following command to run NanoRepeat:
nanoRepeat.py \
-i path/to/NanoRepeat_v1.3_example_data/HG002/hg002_Q20.20210805_3flowcells.hs37d5.example_regions.bam \
-t bam \
-d ont_q20 \
-r path/to/NanoRepeat_v1.3_example_data/HG002/GRCh37_chr1.fasta \
-b path/to/NanoRepeat_v1.3_example_data/HG002/HG002_GRCh37_example_regions.bed \
-c 4 \
--samtools path/to/samtools \
--minimap2 path/to/minimap2 \
-o ./nanorepeat_output/HG002
-i
specifies the input file, which can be in fasta
, fastq
or bam
format. In this case our input file is hg002_Q20.20210805_3flowcells.hs37d5.example_regions.bam
. It is a subset of an Oxford Nanopore whole-genome sequencing dataset of the NIST/GIAB HG002 (GM24385/NA24385) genome. The sequencing data was from the Oxford Nanopore Technologies Benchmark Datasets and reads from 15 example STR regions in chr1
were extracted. These regions were selected because they overlap with the HG002 SV benchmark set and are heterozygous (i.e., two alleles have different repeat sizes).
-t
specifies the input file type. There are four valid values: bam, cram, fastq or fasta. In this case the input file is in a bam file.
-d
specifies the data type. There are five valid values: ont_q20
, ont_sup
, ont
, hifi
, and clr
. ont_q20
is for Oxford Nanopore sequencing with Q20+ chemistry (such as R10 flowcells). ont_sup
is for Oxford Nanopore sequencing with R9 flowcells and basecalled in super accuracy mode. ont
is for Oxford Nanopore sequencing with R9 flowcells and basecalled in fast mode or high accuracy mode. hifi
is for PacBio HiFi/CCS reads. clr
is for PacBio Continuous Long Reads (CLR) reads. Default value: ont
.
-r
specifies the reference genome file in FASTA
format. In this case, GRCh37_chr1.fasta
is chr1 of the GRCh37/hg19 reference genome. We used GRCh37 instead of GRCh38 because the HG002 SV benchmark set is based on GRCh37.
-b
specifies the information of the tandem repeat regions that you are interested in. It is a tab-delimited text file in BED format. There are four required columns: chromosome
, start_position
, end_position
, repeat_unit_sequence
. In our case, HG002_GRCh37_example_regions.bed
contains 15 STR regions in chr1 of GRCh37. The first 5 rows of the HG002_GRCh37_example_regions.bed
are shown below.
1 | 4599903 | 4599930 | TTTAG |
---|---|---|---|
1 | 7923034 | 7923187 | TATTG |
1 | 8321418 | 8321465 | TTCC |
1 | 14459872 | 14459935 | AAAG |
1 | 20934886 | 20934920 | GTTTT |
IMPORTANT NOTICE
-
Please note that in BED format, all chromosome positions start from 0.
start_position
is self-inclusive butend_position
is NOT self-inclusive. Tip: If you have 1-based positons, simply decrease the value ofstart_position
by 1 and no changes forend_position
-
NanoRepeat assumes that the seqeunce between
start_position
andend_position
are all repeats of the motif specified in the fourth column. There should be neither non-repeat sequences nor other repeat motifs betweenstart_position
andend_position
. If a region contains two consecutive repeats, you can specify them in two rows.
-c
specifies the number of CPU cores for alignment.
-o
specifies the output prefix. Please include the path to the output directory and prefix of output file names. In our case, the output prefix is ./nanorepeat_output/HG002
, which means the output directory is ./nanorepeat_output/
and the prefix of output file names is HG002
.
--samtools
and --minimap2
specifies the path to the two software tools. The two arguments are optional if samtools
and minimap2
and be found in your environment.
If you run NanoRepeat sucessfully, you will see 90 output files (six files per region). Output files of a single repeat region look like this:
HG002.1-7923034-7923187-TATTG.allele1.fastq
HG002.1-7923034-7923187-TATTG.allele2.fastq
HG002.1-7923034-7923187-TATTG.hist.png
HG002.1-7923034-7923187-TATTG.phased_reads.txt
HG002.1-7923034-7923187-TATTG.repeat_size.txt
HG002.1-7923034-7923187-TATTG.summary.txt
HG002.1-7923034-7923187-TATTG.allele1.fastq
and HG002.1-7923034-7923187-TATTG.allele2.fastq
are reads of each allele.
HG002.1-7923034-7923187-TATTG.hist.png
is a histogram showing the repeat size distribution. Each allele has a different color.
HG002.1-7923034-7923187-TATTG.phased_reads.txt
shows the phasing results. First 10 lines of the HG002.1-7923034-7923187-TATTG.phased_reads.txt
are shown below.
$ head HG002.1-7923034-7923187-TATTG.phased_reads.txt
##RepeatRegion=1-7923034-7923187-TATTG
#Read_Name Allele_ID Phasing_Confidence Repeat_Size
746edfa7-715f-4e97-913e-ef73ed97135f 1 HIGH 14.0
d6355053-0ed2-438e-8469-28cabeb2aedf 1 HIGH 17.0
513a749a-6ffc-47c4-a499-9f9222e93abf 1 HIGH 17.0
fc8dc377-8772-4dc0-922d-ad694deec8d7 1 HIGH 17.0
cd847c0e-9fbf-4abf-8f0a-ea938026ef41 1 HIGH 17.0
f53bc376-69b4-4118-87e1-59379c640408 1 HIGH 17.0
9b70cd2a-c1df-447a-a7aa-b5ab8046115e 1 HIGH 17.0
6a9b6f5b-d59d-4dde-9adb-8e6ac91cc6e4 1 HIGH 17.0
The columns of the *.phased_reads.txt
file:
Column | Description |
---|---|
1 | Read_Name |
2 | Allele_ID |
3 | Phasing_Confidence (two values: HIGH or LOW) |
4 | Repeat_Size |
HG002.1-7923034-7923187-TATTG.repeat_size.txt
is the estimated repeat sizes of ALL reads. This file is similar to the *.phased_reads.txt
file but it also includes reads that may be removed in the phasing process (e.g. reads considered as noisy reads or outliers)
$ head HG002.1-7923034-7923187-TATTG.repeat_size.txt
##Repeat_Region=1-7923034-7923187-TATTG
#Read_Name Repeat_Size
746edfa7-715f-4e97-913e-ef73ed97135f 14.0
d6355053-0ed2-438e-8469-28cabeb2aedf 17.0
dadaf0a0-8797-47ca-a21b-259928edca7e 48.0
513a749a-6ffc-47c4-a499-9f9222e93abf 17.0
07f65d31-4023-4d86-beba-76fb88f2cf45 48.0
4e66c3d0-6f15-4ff7-a8a8-d5c95d57e73d 48.0
fc8dc377-8772-4dc0-922d-ad694deec8d7 17.0
cd847c0e-9fbf-4abf-8f0a-ea938026ef41 17.0
HG002.1-7923034-7923187-TATTG.summary.txt
gives the quantification of the repeat size. It has the following information: 1) repeat region; 2) number of detected alleles; 3) repeat size of each allele; 4) number of reads of each allele; 5) number of removed reads.
$ cat HG002.1-7923034-7923187-TATTG.summary.txt
Repeat_Region=1-7923034-7923187-TATTG Method=GMM Num_Alleles=2 Num_Removed_Reads=0 Allele1_Num_Reads=33 Allele1_Repeat_Size=17 Allele2_Num_Reads=19 Allele2_Repeat_Size=48
Sometimes two STRs are next to each other. For example, in exon-1 of the human HTT gene, there are two adjacent STRs: CAG
and CCG
. The sequence structure is: (CAG)m-CAA-CAG-CCG-CCA-(CCG)n. NanoRepeat can jointly quantify the two STRs and provide phased results. In our experience, looking at both repeats help generate better quantification results.
We will demonstrate the joint quantification using the same example dataset (described in the above section). If you have not downloaded the dataset, you can execute following commands.
wget https://github.com/WGLab/NanoRepeat/releases/download/v1.3/NanoRepeat_v1.3_example_data.tar.bz2
tar xjf NanoRepeat_v1.3_example_data.tar.bz2
After unzipping the file, you will see a NanoRepeat_v1.2_example_data
folder and there are two subfolders: HG002
and HTT_amplicon
. In this section, we will use the data under the HTT_amplicon
folder.
The input fastq file is here: ./NanoRepeat_v1.2_example_data/HTT_amplicon/HTT_amplicon.fastq.gz
.
The reference fasta file is here: ./NanoRepeat_v1.2_example_data/HTT_amplicon/GRCh38_chr4.0_4Mb.fasta
.
You can use the following command to run NanoRepeat-joint
:
nanoRepeat-joint.py \
-i ./NanoRepeat_v1.3_example_data/HTT_amplicon/HTT_amplicon.fastq.gz \
-r ./NanoRepeat_v1.3_example_data/HTT_amplicon/GRCh38_chr4.0_4Mb.fasta \
-1 chr4:3074876:3074933:CAG:200 \
-2 chr4:3074946:3074966:CCG:20 \
-o ./joint_quantification_output/HTT \
-c 4
-1
and -2
specify the two repeat regions. The format of -1
and -2
is chrom:start_position:end_position:repeat_unit:max_size
. The start and end positions are 0-based (the first base on the chromosome is numbered 0). The start position is self-inclusive but the end position is non-inclusive, which is the same as the BED format. For example, a region of the first 100 bases of chr1 is denoted as chr1:0:100
. max_size
is the max repeat length that we consider. Please set max_size
to be a reasonal number. If max_size
is too large (e.g. well beyond the max possible number), the speed of joint quantification might be slow.
If you run NanoRepeat sucessfully, you will see the following files in the ./joint_quantification_output
folder.
HTT.allele1.fastq
HTT.allele2.fastq
HTT.chr4-3074876-3074933-CAG.hist.png
HTT.chr4-3074946-3074966-CCG.hist.png
HTT.hist2d.png
HTT.phased_reads.txt
HTT.repeat_size.txt
HTT.scatter.png
HTT.summary.txt
HTT.allele1.fastq
and HTT.allele2.fastq
are the reads assigned to each allele.
HTT.chr4-3074876-3074933-CAG.hist.png
is a histogram showing the repeat size distribution of the first repeat (chr4-3074876-3074933-CAG).
HTT.chr4-3074946-3074966-CCG.hist.png
is a histogram showing the repeat size distribution of the second repeat (chr4-3074946-3074966-CCG).
HTT.hist2d.png
is a two-dimensional histogram showing the joint distribution of the two repeats.
HTT.scatter.png
is a scatter plot showing the joint distribution of the two repeats. The dotted lines indicates the 95% equi-probability surface of the Gaussian mixture models.
HTT.phased_reads.txt
shows the phasing results. The first line is the path to the input FASTQ file. Lines 2-9 of the HTT.phased_reads.txt
file are shown below (as a table).
#Read_Name | Allele_ID | Phasing_Confidence | chr4-3074876-3074933-CAG.Repeat_Size | chr4-3074946-3074966-CCG.Repeat_Size |
---|---|---|---|---|
ONT_read330 | 1 | HIGH | 13.5 | 8 |
ONT_read1284 | 1 | HIGH | 17 | 11.5 |
ONT_read579 | 1 | HIGH | 16 | 10 |
ONT_read838 | 1 | HIGH | 15.5 | 10 |
ONT_read520 | 1 | LOW | 25 | 13 |
ONT_read1066 | 1 | HIGH | 17.5 | 10 |
ONT_read1059 | 1 | HIGH | 16 | 10.5 |
ONT_read526 | 1 | HIGH | 17 | 10 |
The *summary.txt
file gives the quantification of the repeat sizes. It has the following information:
- input file
- number of alleles
- number of reads for each allele
- quantification of repeat sizes of each allele
The content of HTT.summary.txt
is shown below:
Input_FASTQ | path/to/HTT_amplicon.fastq.gz |
---|---|
Method | 2D-GMM |
Num_Alleles | 2 |
Num_Removed_Reads | 0 |
Allele1_Num_Reads | 733 |
Allele1_chr4-3074876-3074933-CAG.Repeat_Size | 17 |
Allele1_chr4-3074946-3074966-CCG.Repeat_Size | 10 |
Allele2_Num_Reads | 856 |
Allele2_chr4-3074876-3074933-CAG.Repeat_Size | 55 |
Allele2_chr4-3074946-3074966-CCG.Repeat_Size | 7 |
If you use NanoRepeat, please cite:
Fang L, Monteys AM, Dürr A, Keiser M, Cheng C, Harapanahalli A, et al. Haplotyping SNPs for allele-specific gene editing of the expanded huntingtin allele using long-read sequencing. Human Genetics and Genomics Advances. 2023;4(1):100146. DOI: https://doi.org/10.1016/j.xhgg.2022.100146.
BibTeX format:
@article{FANG2023100146,
title = {Haplotyping SNPs for allele-specific gene editing of the expanded huntingtin allele using long-read sequencing},
journal = {Human Genetics and Genomics Advances},
volume = {4},
number = {1},
pages = {100146},
year = {2023},
issn = {2666-2477},
doi = {https://doi.org/10.1016/j.xhgg.2022.100146},
url = {https://www.sciencedirect.com/science/article/pii/S266624772200063X},
author = {Li Fang and Alex Mas Monteys and Alexandra Dürr and Megan Keiser and Congsheng Cheng and Akhil Harapanahalli and Pedro Gonzalez-Alegre and Beverly L. Davidson and Kai Wang},
keywords = {Huntington’s disease, long-read sequencing, CRISPR, SNP, repeat detection}
}
NanoRepeat can accuratly quantify simple repeats but cannot handle mixed repeats of different motifs (i.e. a mixture of GCCA
and AAATT
), but imperfect repeats of approximately the same motif are OK.
If you need any help from us, you are welcome to raise an issue at the issue page. You can also contact Dr. Li Fang ([email protected]) or Dr. Kai Wang ([email protected]).