一个人全基因组完整数据分析脚本
人全基因组分析一直是整个测序行业最重要的内容之一,随着各种测序仪性能的快速提升,人全基因组测序价格越来越便宜,周期越来越低,可以预见,即将有越来越多的人全基因组被测序出来。这里我们将系统介绍一个完整的人全基因组分析案例,人全基因组分析可以大致分为四个过程。
1、从DNA到fastq;
2、从fastq到bam;
3、从bam到vcf;
4、从vcf到pdf;
一、从DNA到fastq
从DNA到fastq也就是测序的过程,对于人全基因组的测序,要分清楚几个问题?
1、选择哪种测序平台?
2、需要提供多少样品?
3、需要多少测序量?
目前illumina的hiseq平台和bgiseq都可以完成人的全基因组测序,三代测序依然成本较大;如果想进行个人的全基因组测序,可以抽取10ml左右静脉血液即可;人的基因组大小是3G数据量,按照当前测序片段长度,例如双末端150bp,需要测序30倍数据,也就是90G数据;这里我们有一对完整的人全基因组测序原始数据;
-rwxr-xr-x 1 wangtong wangtong 24G 9月 19 22:51 180586B_4607-DNA_S33_L003_R1_001.fastq.gz
-rwxr-xr-x 1 wangtong wangtong 25G 9月 19 23:29 180586B_4607-DNA_S33_L003_R2_001.fastq.gz
二、分析准备工作
得到数据之后就可以开始进行分析;不过需要先进行一些准备工作,例如下载软件和数据库;
1、下载软件
#bwa:
https://jaist.dl.sourceforge.net/project/bio-bwa/bwa-0.7.17.tar.bz2
#samtools:
https://github.com/samtools/samtools/releases/download/1.8/samtools-1.8.tar.bz2
#GATK4:
https://github.com/broadinstitute/gatk/releases/download/4.0.2.1/gatk-4.0.2.1.zip
#bcftools:
https://github.com/samtools/bcftools/releases/download/1.8/bcftools-1.8.tar.bz2
#SNPeff:
https://jaist.dl.sourceforge.net/project/snpeff/snpEff_latest_core.zip
#lumpuy:
https://github.com/arq5x/lumpy-sv
#cnvnator:
https://github.com/abyzovlab/CNVnator/releases
2、下载数据库
lftp ftp.broadinstitute.org/bundle -u gsapubftp-anonymous
cd hg38
mirros hg38
下载完数据,放到hg38/目录下;
├── 1000G_omni2.5.hg38.vcf.gz
├── 1000G_omni2.5.hg38.vcf.gz.tbi
├── 1000G_phase1.snps.high_confidence.hg38.vcf.gz
├── 1000G_phase1.snps.high_confidence.hg38.vcf.gz.tbi
├── Axiom_Exome_Plus.genotypes.all_populations.poly.hg38.vcf.gz
├── Axiom_Exome_Plus.genotypes.all_populations.poly.hg38.vcf.gz.tbi
├── dbsnp_146.hg38.vcf.gz
├── dbsnp_146.hg38.vcf.gz.tbi
├── hapmap_3.3_grch38_pop_stratified_af.vcf.gz
├── hapmap_3.3_grch38_pop_stratified_af.vcf.gz.tbi
├── hapmap_3.3.hg38.vcf.gz
├── hapmap_3.3.hg38.vcf.gz.tbi
├── Homo_sapiens_assembly38.fasta
├── Mills_and_1000G_gold_standard.indels.hg38.vcf.gz
├── Mills_and_1000G_gold_standard.indels.hg38.vcf.gz.tbi
└── wgs_calling_regions.hg38.interval_list
三、从fastq到bam
测序数据,软件,数据库有了之后就可以开始进行分析了。接下来的工作就是将测序的到的fastq文件,比对到参考序列,得到bam格式文件,需要对bam进行很多步处理。
1、原始数据质控;
mkdir rawdata_qc
fastqc -f fastq -o rawdata_qc 180586B_4607-DNA_S33_L003_R1_001.fastq.gz 180586B_4607-DNA_S33_L003_R2_001.fastq.gz
2、数据过滤;
fastp -i 180586B_4607-DNA_S33_L003_R1_001.fastq.gz -I 180586B_4607-DNA_S33_L003_R2_001.fastq.gz -o wgs_clean.1.fq.gz -O wgs_clean.2.fq.gz -z 4 -q 20 -u 30 -n 6 -w 4 -h clean.html
f
3、参考序列建立索引;
bwa index -p Homo_sapiens_assembly38 -a bwtsw Homo_sapiens_assembly38.fasta
gatk CreateSequenceDictionary -R Homo_sapiens_assembly38.fasta -O Homo_sapiens_assembly38.dict
4、bwa mem比对;
bwa mem -t 4 -M -Y -R “@RG\tID:Sample1\tPL:ILLUMINA\tLB:Lib1\tSM:Sample1” hg38/Homo_sapiens_assembly38 wgs_clean.1.fq.gz wgs_clean.2.fq.gz >Sample1.sam
time gatk SortSam -I Sample1.sam -O Sample1.sorted.bam -SO coordinate --CREATE_INDEX true
#也可以利用samtools进行排序
#samtools sort -@ 4 -o Sample1.sorted.bam Sample1.sam
#rm -rf Sample1.sam
5、标记duplication;
gatk MarkDuplicates -I Sample1.sorted.bam -M Sample1.markdup_metrics.txt -O Sample1.sorted.markdup.bam
samtools index Sample1.sorted.markdup.bam
#rm -rf Sample1.sorted.bam
6、碱基较正BQSR
#加time命令计时
time gatk BaseRecalibrator
-R hg38/Homo_sapiens_assembly38.fasta
-I Sample1.sorted.markdup.bam
–known-sites hg38/1000G_phase1.snps.high_confidence.hg38.vcf.gz
–known-sites hg38/Mills_and_1000G_gold_standard.indels.hg38.vcf.gz
–known-sites hg38/dbsnp_146.hg38.vcf.gz
-O Sample1.sorted.markdup.recal_data.table >bqsr.log
time gatk ApplyBQSR
–bqsr-recal-file Sample1.sorted.markdup.recal_data.table
-R hg38/Homo_sapiens_assembly38.fasta
-I Sample1.sorted.markdup.bam
-O Sample1.sorted.markdup.BQSR.bam
time samtools index Sample1.sorted.markdup.BQSR.bam
#rm -rf Sample1.sorted.markdup.bam
四、从bam到vcf
经过对bam一系列的处理,最终得到了经过排序,去除duplication以及bqsr之后的bam文件,接下来就可以使用gatk进行变异检测,输入文件为Sample1.sorted.markdup.BQSR.bam;
1、利用gatk得到vcf文件
time gatk HaplotypeCaller
–emit-ref-confidence GVCF
-R hg38/Homo_sapiens_assembly38.fasta
-I Sample1.sorted.markdup.BQSR.bam
-O Sample1.HC.g.vcf.gz
time gatk GenotypeGVCFs
-R hg38/Homo_sapiens_assembly38.fasta
-V Sample1.HC.g.vcf.gz
-O Sample1.HC.vcf.gz
2、利用VQSR方法过滤SNP结果
time gatk VariantRecalibrator
-R hg38/Homo_sapiens_assembly38.fasta
-V Sample1.HC.vcf.gz
–resource hapmap,known=false,training=true,truth=true,prior=15.0:hg38/hapmap_3.3.hg38.vcf.gz
–resource omni,known=false,training=true,truth=false,prior=12.0:hg38/1000G_omni2.5.hg38.vcf.gz
–resource 1000G,known=false,training=true,truth=false,prior=10.0:hg38/1000G_phase1.snps.high_confidence.hg38.vcf.gz
–resource dbsnp,known=true,training=false,truth=false,prior=2.0:hg38/dbsnp_146.hg38.vcf.gz
-an QD -an MQ -an MQRankSum -an ReadPosRankSum -an FS -an SOR -an DP
-mode SNP
-O Sample1.HC.snps.recal
–tranches-file Sample1.HC.snps.tranches
–rscript-file Sample1.HC.snps.plots.R
time gatk ApplyVQSR
-R hg38/Homo_sapiens_assembly38.fasta
-V Sample1.HC.vcf.gz
-O Sample1.HC.snps.VQSR.vcf.gz
–recal-file Sample1.HC.snps.recal
–tranches-file Sample1.HC.snps.tranches
-mode SNP
3、利用VQSR处理InDel
time gatk VariantRecalibrator
-R hg38/Homo_sapiens_assembly38.fasta
-V Sample1.HC.snps.VQSR.vcf.gz
–max-gaussians 4
–resource mills,known=false,training=true,truth=true,prior=12.0:hg38/Mills_and_1000G_gold_standard.indels.hg38.vcf.gz
–resource dbsnp,known=true,training=false,truth=false,prior=2.0:hg38/dbsnp_146.hg38.vcf.gz
-an QD -an DP -an FS -an SOR -an ReadPosRankSum -an MQRankSum
-mode INDEL
-O Sample1.HC.snps.indel.recal
–tranches-file Sample1.HC.snps.indel.tranches
–rscript-file Sample1.HC.snps.indel.plots.R
time gatk ApplyVQSR
-R hg38/Homo_sapiens_assembly38.fasta
-V Sample1.HC.snps.VQSR.vcf.gz
-O Sample1.HC.snps.indel.VQSR.vcf.gz
–truth-sensitivity-filter-level 99.0
–tranches-file Sample1.HC.snps.indel.tranches
–recal-file Sample1.HC.snps.indel.recal
-mode INDEL
最终,得到的Sample1.HC.snps.indel.VQSR.vcf.gz既是需要的文件。
4、统计结果
#统计突变数目
bcftools stats Sample1.HC.snps.indel.VQSR.vcf.gz > view.stats
plot-vcfstats view.stats -p output
五、其余突变检测
除了利用gatk找SNP和小的InDel之外,还可以利用lumpy找SV突变,CNVnator找CNV突变;
1、利用lumpy检测SV突变
samtools view -b -F 1294 Sample1.sorted.bam | samtools sort - > Sample1.discordants.sorted.bam
samtools view -h Sample1.sorted.bam | /ifs1/Software/biosoft/lumpy-sv-master/scripts/extractSplitReads_BwaMem -i stdin | samtools view -Sb - | samtools sort -> Sample1.splitters.sorted.bam
lumpyexpress -B Sample1.sorted.bam -S Sample1.discordants.sorted.bam -D Sample1.splitters.sorted.bam -o Sample1.lumpu.sv.vcf
2、利用delly检测SV突变
#SV检测
delly call -g hg38/Homo_sapiens_assembly38.fasta -o Sample1.delly.sv.bcf -n Sample1.sorted.bam
#过滤结果
delly filter -f germline -p -q 20 Sample1.delly.sv.bcf -o Sample1.delly.sv.filter.bcf
3、利用CNVnator检测CNV突变
#1.提取mapping信息
/ifs1/Software/biosoft/CNVnator/cnvnator -root Sample1.root -tree Sample1.sorted.bam -unique
#2.生成质量分布图HISTOGRAM
/ifs1/Software/biosoft/CNVnator/cnvnator -root Sample1.root -his 100 -d hg38/Homo_sapiens_assembly38.fasta
#3.生成统计结果
/ifs1/Software/biosoft/CNVnator/cnvnator -root Sample1.root -stat 100
#4.RD信息分割partipition
/ifs1/Software/biosoft/CNVnator/cnvnator -root Sample1.root -partition 100
#5.变异检出
/ifs1/Software/biosoft/CNVnator/cnvnator -root Sample1.root -call 100 > Sample1.cnvnator.vcf
六、从vcf到pdf
该阶段主要是对的到的突变vcf文件Sample1.HC.snps.indel.VQSR.vcf.gz,与各种数据库进行比对注释,得到注释结果之后,利用LaTex或者html语言进行标记,最终生成PDF文档报告。
1、利用SNPeff进行注释
#列出所有数据库
java -jar /ifs1/Software/biosoft/snpEff/snpEff.jar databases | less
#筛选人基因组数据库
java -jar /ifs1/Software/biosoft/snpEff/snpEff.jar databases |grep “Homo”
java -jar /ifs1/Software/biosoft/snpEff/snpEff.jar -i vcf -o vcf GRCh38.86 Sample1.HC.snps.indel.VQSR.vcf.gz >Sample1.snpeff.vcf
2、利用Annovar进行注释
#利用annovar进行注释
#1 装换格式
/ifs1/Software/biosoft/annovar/convert2annovar.pl -format vcf4old Sample1.HC.snps.indel.VQSR.vcf.gz >Sample1.annovar.input
#2 进行注释
/ifs1/Software/biosoft/annovar/annotate_variation.pl -buildver hg38 --geneanno --outfile Sample1.anno Sample1.annovar.input /ifs1/Software/biosoft/annovar/humandb/
3、与Clinvar数据库注释
#clinvar数据库注释
#perl annotate_variation.pl -downdb -webfrom annovar clinvar_20180603 -buildver hg38 humandb/
/ifs1/Software/biosoft/annovar/convert2annovar.pl -format vcf4old Sample1.HC.snps.indel.VQSR.vcf.gz >Sample1.annovar.input
/ifs1/Software/biosoft/annovar/annotate_variation.pl --filter -buildver hg38 --outfile Sample1.clinvar.anno Sample1.annovar.input -dbtype clinvar_20180603 /ifs1/Software/biosoft/annovar/humandb/
其他一些常用数据库:
HGMD:https://www.qiagenbioinformatics.com/hgmd-resources/
SNPedia:https://www.snpedia.com/
PhramGKB: https://www.pharmgkb.org/
七、突变结果可视化
很多时候,为了更加精细化的查看突变结果,可以利用IGV可视化变异结果。Integrative Genomics Viewer 交互式基因组浏览器,它是一种高性能的可视化工具,用来交互式地探索大型综合基因组数据。它支持各种数据类型,包括array-based的和下一代测序的数据和基因注释。
1、下载安装
下载地址:http://software.broadinstitute.org/software/igv/home
需要Java:
2、输入文件:
参考基因组
bam文件
snp vcf文件
indel vcf文件
1360
被折叠的 条评论
为什么被折叠?
到【灌水乐园】发言
