Hi Martin, thanks for your suggestion, GappedAlignments looks promising and together with MD tag as Michael suggested, I should get what I want, I will go through your source code carefully later. I tried your sample code, that actually looks pretty cool with shiny and responsive too. Is that going to be in some of your packages? btw, I am also experimenting with shiny recently and writing a package focusing on quality control of variants and visualization of vcf files using ggbio, I guess I can learn and get some great ideas from your example code, thanks a lot! Tengfei On Fri, Mar 1, 2013 at 12:40 PM, Martin Morgan <mtmorgan@fhcrc.org> wrote: > On 3/1/2013 5:03 AM, Michael Lawrence wrote: > >> You should check out the GappedReads object from ShortRead. It extends >> GappedAlignments to hold the read sequence information in a DNAStringSet. >> You could then take the genome() identifier and auto-lookup the BSgenome. >> Or if the SAM MD tag is present in the GappedAlignments, you could use >> that >> for the mismatches. >> > > I think it's better to use readGappedAlignments with > ScanBamParam(what="seq") to get a GappedAlignments object with a 'seq' > metadata column (also any tags in the bam file); the most interesting > functionality that might come with a GappedReads (qnarrow, narrow, which > alter the cigar and potentially underlying sequence) are not implemented on > GappedReads (the class was introduced before GappedAlignments supported > additional metadata columns). > > Probably live to regret it but there is > > https://gist.github.com/**mtmorgan/4067179<https: gist.github.com="" mtmorgan="" 4067179=""> > > which uses the cigar to make a view onto a DNAStringSet of aligned reads. > There are some crude visualizations in there. It seems to have problems > with reads with (long) N's. The current implementation collapses reads into > single lines the way genome browsers do (losing information on individual > reads), but this could be changed easily I think by making lvls in line 29 > just a vector along the input ranges. One can also create a parallel view > of 'qual', allowing overlaying of sequence and quality info. > > I played around last night with wrapping this in shiny (biocLite("shiny")) > > ============== > cigarview/ui.R > ============== > library(shiny) > bamFilepath <- file.choose() > bamFile <- open(BamFile(bamFilepath)) > > seqnames <- seqlevels(bamFile) > names(seqnames) <- seqnames > start <- 1248187 # min(start(seqinfo)) > end <- 1300264 # max(end(seqinfo)) > > shinyUI(pageWithSidebar( > > headerPanel("Cigar Viewer"), > > sidebarPanel( > textInput("bamFile", "BAM file:", bamFilepath), > selectInput("seqname", "Seqname:", seqnames, "5"), > numericInput("start", "Global start:", start), > numericInput("end", "Global end:", end), > > h4("View (relative to global coordinates)"), > numericInput("viewStart", "Start:", 1), > numericInput("viewWidth", "Width:", 1000) > ), > > mainPanel( > plotOutput("pileup") > ) > > )) > > ================== > cigarview/server.R > ================== > library(shiny) > library(Rsamtools) > library(RColorBrewer) > source("../4067179/cigarAlign.**R") > > shinyServer(function(input, output) { > > aln <- reactive({ > which <- GRanges(input$seqname, > IRanges(input$start, input$end)) > param <- ScanBamParam(which=which, what="seq") > cigarAlign(input$bamFile, param=param, pad=TRUE) > }) > > output$pileup <- renderPlot({ > variantplot2(subviews(aln(), input$viewStart, > width=input$viewWidth)) > }) > > }) > > > and then shiny::runApp("./cigarview"); changing the 'view' parameters is > basically usable for interactive exploration within the region of global > start / end coordinates. > > Martin > > > >> Michael >> >> >> On Thu, Feb 28, 2013 at 9:43 PM, Tengfei Yin <yintengfei@gmail.com> >> wrote: >> >> >>> >>> On Thu, Feb 28, 2013 at 11:08 PM, Michael Lawrence < >>> lawrence.michael@gene.com> wrote: >>> >>> >>>> >>>> >>>> On Thu, Feb 28, 2013 at 11:46 AM, Tengfei Yin <yintengfei@gmail.com>>>> >wrote: >>>> >>>> On Thu, Feb 28, 2013 at 11:46 AM, Julian Gehring >>>>> <julian.gehring@gmail.com>**wrote: >>>>> >>>>> Hi, >>>>>> >>>>>> Is there a good way to visualize aligned reads with mismatch bases >>>>>> >>>>> (SNPs) >>>>> >>>>>> along the genome (similar to what one knows from the standard genome >>>>>> browsers)? >>>>>> >>>>>> 'ggbio' came to my mind with which plotting a pile of reads is >>>>>> straight >>>>>> forward. However, overlaying the mismatched bases for each reads >>>>>> >>>>> seems not >>>>> >>>>>> that easy any more. >>>>>> >>>>>> >>>>> Hi Julian, >>>>> >>>>> You are right, currently ggbio only supports summary of mismatch >>>>> showing >>>>> as >>>>> coverage plot and barchart(?stat_mismatch), but looks like what you >>>>> want >>>>> is >>>>> detailed short reads alignments visualization with mismatch bases >>>>> showing >>>>> right on the reads, . It's possible, but not easy to do it >>>>> manually...you >>>>> have to have two GRanges objects, one for alignment one for SNP, and >>>>> plot >>>>> them layer by layer, the tricky part is assigning each reads fixed >>>>> stepping >>>>> level, so snp can be plotted on the right position. I will NOT >>>>> recommend >>>>> you to do this, it's probably not worth taking time doing it. I need to >>>>> implement this features in some easy way. >>>>> >>>>> The tricky part is that there are different modes, 1. show reads as >>>>> gray >>>>> rectangle, and color mismatch as segment >>>>> >>>> >>>> >>>> Are you talking about single-read detail for #1 above or what we get >>>> from >>>> stat_mismatch? >>>> >>>> >>> The single-read detail, not summary mismatch from stat_mismatch(). so for >>> example, one 75bp reads shown as one rectangle filled with gray color, >>> and >>> use vertical colored segment indicated mismatched position on this reads >>> if >>> any. >>> >>> >>> >>>> >>>> 2. show SNP as nucleotide text, >>>>> A/C/T/G.., 3. show sequence detail for each alignment. those depends >>>>> on >>>>> zoomed level and even coverage, and I guess most time you don't want to >>>>> see >>>>> bases for every reads... >>>>> >>>>> >>>>> I think #3 is really important for any sort of diagnosis of alignment >>>> issues, and I would find this very useful. Right now, I'm using IGV for >>>> this, but ggbio would be a lot more flexible. This is probably my #1 top >>>> missing feature from ggbio. >>>> >>>> >>> Got it, those features are indeed important but missing, I will keep this >>> in mind. >>> >>> I was thinking about generalize it into visualization of DNAStringSet >>> first, but mismatch is not that general, require BSgenome and raw bam >>> files >>> at the same time to get mismatched information. So we may extend the list >>> returned by scanBam(), and create a GRanges or vector with equal length >>> of >>> short reads numbers for particular region which storing mismatch position >>> and nucleotide. I am trying to think about a more general data structure, >>> not only for visualization purpose, but also for command line analysis, >>> for >>> example, people can simply retrieve mismatch information for any single >>> short read from specific data structure. >>> >>> and Julian, sorry that I don't have any working example right now, I will >>> let you know when this feature is ready to test. >>> >>> Tengfei >>> >>> >>>> >>>> >>>> Just curious for future ggbio development, are those modes want you >>>>> want? >>>>> are you just using bam files here? no VCF files involved right? >>>>> Because >>>>> you mentioned 'snp', I think what you mean is mismatch? >>>>> >>>>> ps: I cannot speak for other tools, and only thing I know, in SRAdb >>>>> package, looks like it could fire your data in IGV.. >>>>> >>>>> Thanks >>>>> >>>>> Tengfei >>>>> >>>>> >>>>> Does someone of you have a good way to do this or found another >>>>>> >>>>> solution >>>>> >>>>>> that works for R/bioc? >>>>>> >>>>>> Best wishes >>>>>> Julian >>>>>> >>>>>> ______________________________****_________________ >>>>>> Bioconductor mailing list >>>>>> Bioconductor@r-project.org >>>>>> https://stat.ethz.ch/mailman/****listinfo/bioconductor<https: stat.ethz.ch="" mailman="" **listinfo="" bioconductor=""> >>>>>> < >>>>>> >>>>> https://stat.ethz.ch/mailman/**listinfo/bioconductor<https: sta="" t.ethz.ch="" mailman="" listinfo="" bioconductor=""> >>>>> > >>>>> >>>>>> Search the archives: http://news.gmane.org/gmane.** >>>>>> science.biology.informatics.****conductor< >>>>>> >>>>> http://news.gmane.org/gmane.**science.biology.informatics.**cond uctor<http: news.gmane.org="" gmane.science.biology.informatics.conducto="" r=""> >>>>> > >>>>> >>>>>> >>>>>> >>>>> >>>>> >>>>> -- >>>>> Tengfei Yin >>>>> MCDB PhD student >>>>> 1620 Howe Hall, 2274, >>>>> Iowa State University >>>>> Ames, IA,50011-2274 >>>>> >>>>> [[alternative HTML version deleted]] >>>>> >>>>> ______________________________**_________________ >>>>> Bioconductor mailing list >>>>> Bioconductor@r-project.org >>>>> https://stat.ethz.ch/mailman/**listinfo/bioconductor<https: sta="" t.ethz.ch="" mailman="" listinfo="" bioconductor=""> >>>>> Search the archives: >>>>> http://news.gmane.org/gmane.**science.biology.informatics.**cond uctor<http: news.gmane.org="" gmane.science.biology.informatics.conducto="" r=""> >>>>> >>>>> >>>> >>>> >>> >>> -- >>> Tengfei Yin >>> MCDB PhD student >>> 1620 Howe Hall, 2274, >>> Iowa State University >>> Ames, IA,50011-2274 >>> >>> >>> >>> >> [[alternative HTML version deleted]] >> >> ______________________________**_________________ >> Bioconductor mailing list >> Bioconductor@r-project.org >> https://stat.ethz.ch/mailman/**listinfo/bioconductor<https: stat.e="" thz.ch="" mailman="" listinfo="" bioconductor=""> >> Search the archives: http://news.gmane.org/gmane.** >> science.biology.informatics.**conductor<http: news.gmane.org="" gmane="" .science.biology.informatics.conductor=""> >> >> > > -- > Dr. Martin Morgan, PhD > Fred Hutchinson Cancer Research Center > 1100 Fairview Ave. N. > PO Box 19024 Seattle, WA 98109 > -- Tengfei Yin MCDB PhD student 1620 Howe Hall, 2274, Iowa State University Ames, IA,50011-2274 [[alternative HTML version deleted]]