Unconfigured Ad

Collapse
X
 
  • Filter
  • Time
  • Show
Clear All
new posts
  • gfmgfm
    Member
    • Jun 2010
    • 64

    SNP filtering

    I ran samtools pileup and varfilter on human capture Ilumina data.
    Does anyone has suggestions on how to filter the output in order to get reliable homozygous and heterozygous SNPs?
  • nickloman
    Senior Member
    • Jul 2009
    • 355

    #2
    I'd suggest looking at VarScan and playing with the settings.

    Comment

    • drio
      Senior Member
      • Oct 2008
      • 323

      #3
      pileup is deprecated. Use mpileup instead. It computes BAQ (check same link) and uses it for the SNP calling. It seems BAQ helps reduce false positives (check alignment example at the bottom in the link above).
      -drd

      Comment

      • gfmgfm
        Member
        • Jun 2010
        • 64

        #4
        Thanks a lot for the suggestion. I already tried VarScan. The problem is that it does not give columns with total coverage for the position, so it is difficult to decide whether it is a reliable heterozygous/homozygous SNP. For example here are two lines from an output of VarScan:
        1.chrM 16236 C A 0 35 100% 0 1 0 93 0.98
        2. chrM 16236 C T 0 275 100% 0 2 0 93 0.98

        I thought that in order to distinguish b/w reliable homozygous/heterozygous SNPs, I need to know the ratio of the "A" coverage (line 1) relative to the total coverage for that position. I would also like to know what is the ratio between the most frequent nucleotide to the second frequent nucleotide.
        without this info how can I tell, for example in line 1, if it is a reliable SNP and what kind of SNP?

        Comment

        • gfmgfm
          Member
          • Jun 2010
          • 64

          #5
          drio, thanks a lot for the reply. I looked at the mpileup. If I have already results and conclusions from pileup results - is it OK to use them?

          Comment

          • drio
            Senior Member
            • Oct 2008
            • 323

            #6
            As soon as you used reasonable filters (check protocol in FAQ for a starting point) yes. pileup has been used with great level of success in various papers.
            -drd

            Comment

            • gfmgfm
              Member
              • Jun 2010
              • 64

              #7
              ok, thanks.

              Comment

              • bioman1
                Member
                • May 2012
                • 80

                #8
                Varscan SNV

                Dear all,
                I am new to NGS analysis. I have used bowtie (ver:bowtie-0.12.7) for aligning reference sequence (fastq format) with two paired end files of illumina reads (fastq format). Then I used SAM tools (ver:samtools-0.1.18) and made a 'mpileup' file. Then I have used Varscan (ver:.v2.2.11) for variant calling. I used "pileup2snp' command (with default parameters) to determine SNV and for heterozygosity & homozygosity.

                1. The output gives in colums and I have below as rows for easy reading
                Output:
                Chrom:gi|53564564|gb|JH556356.3
                Position:1781287
                Ref:T
                Cons:Y
                Reads1:7
                Reads2:2
                VarFreq:22.22%
                Strands1:2
                Strands2:2
                Qual1:27
                Qual2:26
                Pvalue:0.98
                MapQual1:1
                MapQual2:1
                Reads1Plus:5
                Reads1Minus:2
                Reads2Plus:1
                Reads2Minus:1
                VarAllele:c


                2. Any any one can tell me how identify SNV (how many of them are heterzygous & homozygous) with the above output ?. I have searched this forum, I could not find any help.

                Comment

                • soban
                  Junior Member
                  • Nov 2011
                  • 5

                  #9
                  SNP Filtering

                  Dear Fellows,
                  I am new to NGS technologies, i ran BWA for mapping my reads then i used GATK-Tool for SNP-Calling, now i want to filter the SNPs, i dont know how to proceed further, please name some tools to filter the SNPs, also how to use that one?.
                  Last edited by soban; 02-07-2013, 02:49 AM.

                  Comment

                  Latest Articles

                  Collapse

                  • SEQadmin2
                    Advanced Sequencing Platforms Tackle Neuroscience’s Toughest Genomics Problems
                    by SEQadmin2



                    Genomics studies in neuroscience face a special challenge due to the brain’s complexity and scarcity of samples. Mapping changes in cell type and state using conventional next-generation sequencing methods remains challenging. Advances in technologies like single-cell sequencing, spatial transcriptomics, and long-read sequencing have opened the door to deeper studies of the brain and diseases like Alzheimer’s, amyotrophic lateral sclerosis (ALS), and schizophrenia.
                    ...
                    07-09-2026, 11:10 AM
                  • SEQadmin2
                    Cancer Drug Resistance: The Lingering Barrier to Rising Survival
                    by SEQadmin2



                    Cancer survival rates have significantly increased in the last few decades in the United States, reaching a combined 70% 5-year survival rate by 2021. Behind this number, there are years of research to find new therapies, drug targets, and early detection methods. But there is one core challenge that keeps slowing down these advances, and it’s about drug resistance.

                    There is no single reason why many patients don’t respond to treatment as expected. Cancer is...
                    07-08-2026, 05:17 AM
                  • GATTACAT
                    Reply to Nine Things a Sample Prep Scientist Thinks About Before Sequencing
                    by GATTACAT
                    Love this - good data definitely starts from good input, and poor input can only give relatively poor data. I particularly like the mention of Nanodrop/absorbance based methods for quantification. It's such a toss up if you'll get an accurate reading or what amounts to a randomly generated number, and a lot of library/sequencing related issues can be traced back to poor quant.
                    07-01-2026, 11:43 AM

                  ad_right_rmr

                  Collapse

                  News

                  Collapse

                  Topics Statistics Last Post
                  Started by SEQadmin2, Today, 10:26 AM
                  0 responses
                  9 views
                  0 reactions
                  Last Post SEQadmin2  
                  Started by SEQadmin2, 07-09-2026, 10:04 AM
                  0 responses
                  24 views
                  0 reactions
                  Last Post SEQadmin2  
                  Started by SEQadmin2, 07-08-2026, 10:08 AM
                  0 responses
                  16 views
                  0 reactions
                  Last Post SEQadmin2  
                  Started by SEQadmin2, 07-07-2026, 11:05 AM
                  0 responses
                  33 views
                  0 reactions
                  Last Post SEQadmin2  
                  Working...