Trimming the qname is implemented in Rsamtools 1.17.18 and should be available via biocLite() ~ noon tomorrow. 'qnamePrefixStart' and 'qnameSuffixEnd' fields have been added to the BamFile class. Currently the trimming is implemented for mate pairing only, not just reading records from a bam. Unique qnames aren't a problem in this sample file - just using it to demonstrate the output. fl <- system.file("extdata", "ex1.bam", package="Rsamtools") param <- ScanBamParam(what="qname") ## no trimming bf <- BamFile(fl, asMates=TRUE) >> scanBam(bf, param=param)[[1]]$qname[1:3] > [1] "EAS54_61:4:143:69:578" "EAS54_61:4:143:69:578" > [3] "EAS219_FC30151:7:51:1429:1043" ## trim prefix qnamePrefixEnd(bf) <- "_" >> scanBam(bf, param=param)[[1]]$qname[1:3] > [1] "61:4:143:69:578" "61:4:143:69:578" "FC30151:7:51:1429:1043" ## trim prefix and suffix qnameSuffixStart(bf) <- ":" >> scanBam(bf, param=param)[[1]]$qname[1:3] > [1] "61:4:143:69" "61:4:143:69" "FC30151:7:51:1429" Valerie On 05/08/14 12:17, Stefano Calza wrote: > Yes, I say that would be easier to use than regexp > > Stefano > > On 05/08/2014 08:59 PM, Valerie Obenchain wrote: >> Thanks for the SRA tips. >> >> It's starting to look like the modifications are an additional prefix >> or suffix separated by dot or slash (possibly underscore?). Maybe >> simply adding an option to trim the QNAME by the pre/post term >> separated by a given character would be sufficient. This allows >> flexibilty but prevents unwarranted QNAME mangling. >> >> Valerie >> >> >> On 05/08/14 10:56, Stefano Calza wrote: >>> Right this is how I got some other example. I think it would add the >>> files names, as from 2 SRA files (SRR1234 & SRR1235) my reads are named >>> STARTING with SRR1234 or SRR1235 for the two mates, followed by actual >>> read QNAME. >>> >>> Stefano >>> >>> On 05/08/2014 07:05 PM, James W. MacDonald wrote: >>>> Hi Valerie, >>>> >>>> You get something similar from the .sra files that you can download >>>> from the SRA, if they are paired data. If you use the SRA toolkit to >>>> convert to fastq (fastq-dump), it will spit out two fastq files, and >>>> the QNAME in each of the fastq files will be appended with a .1 for >>>> the first pairs and a .2 for the second pairs. >>>> >>>> As an example: >>>> >>>> zcat SRR833731_1.fastq.gz | head -n 1 >>>> @SRR833731.1.1 HWI-ST423:250:D0JRLACXX:8:1101:1473:1978 length=101 >>>> zcat SRR833731_2.fastq.gz | head -n 1 >>>> @SRR833731.1.2 HWI-ST423:250:D0JRLACXX:8:1101:1473:1978 length=101 >>>> >>>> >>>> Best, >>>> >>>> Jim >>>> >>>> >>>> >>>> On Thursday, May 08, 2014 12:03:29 PM, Stefano Calza wrote: >>>>> Thanks Valerie >>>>> >>>>> I have got this BAM files from different sources but they cannot be >>>>> distributed. >>>>> >>>>> Up to now I experienced twp different 'patterns' in QNAME. One is the >>>>> trailing value as we said (/1, /2). Another one is a leading string. >>>>> Eg. (made up QNAME) >>>>> >>>>> SRR1122.12345HTR >>>>> SRR1123.12345HTR >>>>> >>>>> So there must be removed SRR1122 and SRR1123) >>>>> >>>>> My little program actually uses a regex substitution, so the user can >>>>> decide what pattern to edit. This second one though it seems quit >>>>> unusual. >>>>> >>>>> Those with trailing values were downloaded by TCGA (if I recall >>>>> correctly the use a pipeline called MapSplice) >>>>> >>>>> >>>>> Regards >>>>> >>>>> Stefano >>>>> >>>>> On 05/08/2014 05:54 PM, Valerie Obenchain wrote: >>>>>> Hi Stefano, >>>>>> >>>>>> No, the current mate-pairing doesn't handle the trailing values. I >>>>>> will implement this and post back when it's done. >>>>>> >>>>>> For reference, where did you download your bam files or what >>>>>> application outputs QNAMEs in this format? I'd like to have some for >>>>>> test data. >>>>>> >>>>>> >>>>>> Thanks. >>>>>> Valerie >>>>>> >>>>>> >>>>>> On 05/08/14 08:14, Stefano Calza wrote: >>>>>>> Hi everybody >>>>>>> >>>>>>> >>>>>>> I am using GenomicAlignments package to read RNAseq pair-end >>>>>>> data. The >>>>>>> problem is that readGAlignmentPairsFromBam, after setting >>>>>>> asMates=TRUE >>>>>>> in BamFile, returns 0 mates. >>>>>>> >>>>>>> The reason is that mates have different QNAMEs. Eg: >>>>>>> >>>>>>> UNC15-SN850:240:D148CACXX:3:1308:19719:99367/1 >>>>>>> UNC15-SN850:240:D148CACXX:3:1308:19719:99367/2 >>>>>>> >>>>>>> that is the two mates have /1 or /2 at the end. >>>>>>> >>>>>>> I wrote a Python (and a cpp) program to fix it...but this takes >>>>>>> still >>>>>>> quite a substantial amount of time on big files. >>>>>>> >>>>>>> Does the mating algorithm allow for this? If so how? >>>>>>> >>>>>>> Regards >>>>>>> >>>>>>> Stefano >>>>>>> >>>>>>> _______________________________________________ >>>>>>> Bioconductor mailing list >>>>>>> Bioconductor at r-project.org >>>>>>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>>>>>> Search the archives: >>>>>>> http://news.gmane.org/gmane.science.biology.informatics.conductor >>>>>> >>>>>> >>>>> >>>>> _______________________________________________ >>>>> Bioconductor mailing list >>>>> Bioconductor at r-project.org >>>>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>>>> Search the archives: >>>>> http://news.gmane.org/gmane.science.biology.informatics.conductor >>>> >>>> -- >>>> James W. MacDonald, M.S. >>>> Biostatistician >>>> University of Washington >>>> Environmental and Occupational Health Sciences >>>> 4225 Roosevelt Way NE, # 100 >>>> Seattle WA 98105-6099 >>>> >>>> _______________________________________________ >>>> Bioconductor mailing list >>>> Bioconductor at r-project.org >>>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>>> Search the archives: >>>> http://news.gmane.org/gmane.science.biology.informatics.conductor >>> >>> _______________________________________________ >>> Bioconductor mailing list >>> Bioconductor at r-project.org >>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>> Search the archives: >>> http://news.gmane.org/gmane.science.biology.informatics.conductor >> >> >