So this error happens here, no? res = RangedData(IRanges(start=position(ar),width=width(ar)), strand=strand(ar),space=ar at chromosome) If this is the case the problem is not in nucleR, maybe there are some rows in a strange format in the AlignedRead (could be due the multiple format changes) that may avoid the conversion to the RangedData. Maybe I can detect them and skip those cases, but I would need to see what's happening in that odd case. Let me know if there's something I can do. Regards, Oscar El 03/11/2011 13:58, Stefanie Ververs escribi?: > Hi Oscar, > > thanks for your quick answer - I think I would have contacted you, if > there were no answers on the bioconductor-mailinglist. > > I just tried the workaround as you suggested, but I got the same error > again: > Fehler in solveUserSEW0(start = start, end = end, width = width) : > solving row 16512893: range cannot be determined from the supplied > arguments (too many NAs) > Calls: RangedData -> is -> IRanges -> solveUserSEW0 -> .Call > > I'll think about how to show you the data (it's hosted and processed > with Galaxy, so it might be possible to share it.) > > Regards, > > Steffi > > On 03.11.2011 13:16, Oscar Flores wrote: >> Hi Stefanie, >> >> I'm the developer of nucleR, so let's see if I can help you ;) >> >> After the processing, processReads converts the input data to a >> RangedData >> object for a easier manipulation later, so this error is occurs at >> the last >> step of the call, but data can be messed in previous steps. It's >> hard to tell what is happening without having a look to the input data, >> which I guess is huge... >> >> I would like to have a look to the raw data, but I know it is difficult >> to send it if it's not in a public repository. Maybe you can contact me >> directly about that (oflores at mmb.pcb.ub.es)... >> >> Meanwhile, if you want to try a workaround, you can directly convert the >> imported reads to RangedData format (which is the other format supported >> by processReads): >> >> (being "ar" your imported AlignedReads object) >> >> res = RangedData(IRanges(start=position(ar),width=width(ar)), >> strand=strand(ar),space=ar at chromosome) >> >> reads_pair = processReads(res, type="paired", fragmentLen=fragment_len) >> >> This should work, but will be nice to have a look to your data >> to fix a possible problem in the AlignedReads method. >> >> Regards, >> >> Oscar >> >> _______________________________________________ >> 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 > -- Oscar Flores Computer Engineer - PhD Student Molecular Modelling& Bioinformatics Group Institute for Research in Biomedicine (IRB Barcelona) Parc Cient?fic de Barcelona

On 07.11.2011 19:52, Martin Morgan wrote: > On 11/07/2011 02:53 AM, Stefanie Ververs wrote: >> Hi Martin, >> >> I just ran my script with another dataset but got the same error (even >> if on a different line). >> I read the description of readAligned and ScanBamParam, but I still >> don't get how to provide this parameters to readAligned. (I see that I >> can create an object/instance of ScanBamParam, but then? Is it something >> like "alignedReads <- readAligned(dir, pattern=filename, type="BAM", >> param=myScanBamParamObject)? There is no example and I am *really* new > > yes, for example > > dir <- system.file("extdata", package="Rsamtools") > param <- ScanBamParam(simpleCigar=TRUE,, reverseComplement=TRUE) > aln <- readAligned(dir, "ex1.bam$", type="BAM", param=param) I tried this: /param <- ScanBamParam(simpleCigar=TRUE, reverseComplement=TRUE) alignedReads <- readAligned(dir, pattern=filename, type="BAM", param=param)/ and got a warning: /Warnmeldung: UserArgumentMismatch using 'qname' 'flag' 'rname' 'strand' 'pos' 'mapq' 'seq' 'qual' for 'bamWhat(param)' / (I did not test with more arguments by now.) > >> to R, sorry ;) Then I would try parsing the file with more specified >> arguments.. >> >> I got some more information about my file/dataset: >> >> 17709538 + 0 in total (QC-passed reads + QC-failed reads) >> 0 + 0 duplicates >> 120774 + 0 mapped (0.68%:-nan%) >> 17709538 + 0 paired in sequencing >> 8854769 + 0 read1 >> 8854769 + 0 read2 >> 120774 + 0 properly paired (0.68%:-nan%) >> 120774 + 0 with itself and mate mapped >> 0 + 0 singletons (0.00%:-nan%) >> 0 + 0 with mate mapped to a different chr >> 0 + 0 with mate mapped to a different chr (mapQ>=5) >> >> >> And the error is (this time) in row /120775./ >> /(Fehler in solveUserSEW0(start = start, end = end, width = width) : >> solving row 120775: range cannot be determined from the supplied >> arguments (too many NAs) >> Calls: RangedData -> is -> IRanges -> solveUserSEW0 -> .Call/) > > Again it appears to be the last record. Can you provide a simpler > example? For instance, from your original message you said that you > input the data as I got some smaller input file and will try to use it for NucleR, too. By now: > > alignedReads <- readAligned(dir, pattern=filename, type="BAM") > > but that the error occurred at > > reads_pair = processReads(nucleosome_htseq, type="paired", > fragmentLen=fragment_len) > > but there is no obvious connection between 'alignedReads' and the > arguments to 'processReads'. Also, what is the output of This was because of copying and changing some names, alignedReads and nucleosome_htseq are the same. (I checked and ran again, still the same error.) > > idx = is.na(position(alignedReads)) & is.na(width(alignedReads)) > sum(idx) > > ? If sum(idx) != 0, then try using alignedReads[!idx]. And finally, after sum(idx) is 0. > > library(ShortRead) > library(nucleR) > > what is the result of > > sessionInfo() > > ? /The sessionInfo-Output: R version 2.13.2 (2011-09-30) Platform: x86_64-pc-linux-gnu (64-bit) locale: [1] LC_CTYPE=de_DE.UTF-8 LC_NUMERIC=C [3] LC_TIME=de_DE.UTF-8 LC_COLLATE=de_DE.UTF-8 [5] LC_MONETARY=C LC_MESSAGES=de_DE.UTF-8 [7] LC_PAPER=de_DE.UTF-8 LC_NAME=C [9] LC_ADDRESS=C LC_TELEPHONE=C [11] LC_MEASUREMENT=de_DE.UTF-8 LC_IDENTIFICATION=C attached base packages: [1] stats graphics grDevices utils datasets methods base other attached packages: [1] nucleR_0.99.4 Biobase_2.12.2 ShortRead_1.10.4 [4] Rsamtools_1.4.3 lattice_0.19-33 Biostrings_2.20.4 [7] GenomicRanges_1.4.8 IRanges_1.10.6 loaded via a namespace (and not attached): [1] grid_2.13.2 hwriter_1.3/ > >> >> >> >> On 03.11.2011 14:39, Martin Morgan wrote: >>> On 11/03/2011 06:14 AM, Oscar Flores wrote: >>>> So this error happens here, no? >>>> >>>> res = RangedData(IRanges(start=position(ar),width=width(ar)), >>>> strand=strand(ar),space=ar@chromosome) >>> >>> better to use the accessor chromosome(ar). The error >>> >>> > Fehler in solveUserSEW0(start = start, end = end, width = width) : >>> > solving row 16512893: range cannot be determined from the supplied >>> > arguments (too many NAs) >>> >>> suggests that position(ar)[16512893] and / or width(ar)[16512893] is >>> NA. You could filter these out, e.g., ar[!is.na(position(ar)) & >>> !is.na(position(ar))] or identify why these are read in in the first >>> place using the 'param' argument as described on ?readAligned. >>> >>> Martin >>> >>>> >>>> If this is the case the problem is not in nucleR, maybe there are some >>>> rows in a strange format in the AlignedRead (could be due the multiple >>>> format changes) that may avoid the conversion to the RangedData. >>>> Maybe I >>>> can detect them and skip those cases, but I would need to see what's >>>> happening in that odd case. >>>> >>>> Let me know if there's something I can do. >>>> >>>> Regards, >>>> >>>> Oscar >>>> >>>> >>>> El 03/11/2011 13:58, Stefanie Ververs escribió: >>>>> Hi Oscar, >>>>> >>>>> thanks for your quick answer - I think I would have contacted you, if >>>>> there were no answers on the bioconductor-mailinglist. >>>>> >>>>> I just tried the workaround as you suggested, but I got the same >>>>> error >>>>> again: >>>>> Fehler in solveUserSEW0(start = start, end = end, width = width) : >>>>> solving row 16512893: range cannot be determined from the supplied >>>>> arguments (too many NAs) >>>>> Calls: RangedData -> is -> IRanges -> solveUserSEW0 -> .Call >>>>> >>>>> I'll think about how to show you the data (it's hosted and processed >>>>> with Galaxy, so it might be possible to share it.) >>>>> >>>>> Regards, >>>>> >>>>> Steffi >>>>> >>>>> On 03.11.2011 13:16, Oscar Flores wrote: >>>>>> Hi Stefanie, >>>>>> >>>>>> I'm the developer of nucleR, so let's see if I can help you ;) >>>>>> >>>>>> After the processing, processReads converts the input data to a >>>>>> RangedData >>>>>> object for a easier manipulation later, so this error is occurs at >>>>>> the last >>>>>> step of the call, but data can be messed in previous steps. It's >>>>>> hard to tell what is happening without having a look to the input >>>>>> data, >>>>>> which I guess is huge... >>>>>> >>>>>> I would like to have a look to the raw data, but I know it is >>>>>> difficult >>>>>> to send it if it's not in a public repository. Maybe you can >>>>>> contact me >>>>>> directly about that (oflores@mmb.pcb.ub.es)... >>>>>> >>>>>> Meanwhile, if you want to try a workaround, you can directly >>>>>> convert the >>>>>> imported reads to RangedData format (which is the other format >>>>>> supported >>>>>> by processReads): >>>>>> >>>>>> (being "ar" your imported AlignedReads object) >>>>>> >>>>>> res = RangedData(IRanges(start=position(ar),width=width(ar)), >>>>>> strand=strand(ar),space=ar@chromosome) >>>>>> >>>>>> reads_pair = processReads(res, type="paired", >>>>>> fragmentLen=fragment_len) >>>>>> >>>>>> This should work, but will be nice to have a look to your data >>>>>> to fix a possible problem in the AlignedReads method. >>>>>> >>>>>> Regards, >>>>>> >>>>>> Oscar >>>>>> >>>>>> _______________________________________________ >>>>>> Bioconductor mailing list >>>>>> Bioconductor@r-project.org >>>>>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>>>>> Search the archives: >>>>>> http://news.gmane.org/gmane.science.biology.informatics.conductor >>>>> >>>> >>> >>> >> > > [[alternative HTML version deleted]]