BiSeq trimClusters FDR.loc confusion
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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Hi I am running the BiSeq software and have 2 rejected clusters after running testClusters with FDR.cluster=0.1

When I attempt to run trimClusters on these two clusters I get no results unless I use a FDR.loc >= 1.5... I am having some trouble understanding what exactly this FDR.loc number means, in general and one as high as 1.5, and also why I have to use one so high to even see results? Could someone help me with some insight?

 

Thanks,

Marcus

biseq fdr data results • 3.5k views
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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Hi Katja,

Sorry one more question. Is there a way to write the DMRs object to a csv?

 

Thanks,

Marcus

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If your DMRs are GRanges do yourDMRs <- as.data.frame(DMR.GRanges) and then: write.table(yourDMRs, file = "yourDMRs.csv", rownames = FALSE, quote = FALSE, sep = "\t") Cheers, Katja ----- Original Message ----- > From: "mnaymik [bioc]" <noreply@bioconductor.org> > To: katjah@stanford.edu > Sent: Monday, April 27, 2015 10:09:18 AM > Subject: [bioc] A: BiSeq trimClusters FDR.loc confusion > Activity on a post you are following on support.bioconductor.org > User mnaymik wrote Answer: BiSeq trimClusters FDR.loc confusion : > Hi Katja, > Sorry one more question. Is there a way to write the DMRs object to a csv? > Thanks, > Marcus > You may reply via email or visit > A: BiSeq trimClusters FDR.loc confusion
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@katja-hebestreit-6495
Last seen 4.4 years ago
United States

Hi Marcus,

Are you sure that you used an FDR.loc > 1? What other values for FDR.loc did you try?

In general, it can happen that testing on CpG-wise level with the same FDR that you used for calling significant regions doesn't result in any significant CpG sites.

Cheers,

Katja

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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Yes, I tried incrementing the fdr.loc from .1 up to 1.5 by .1 until the results were not null. The way the code is written you are not restricted to any value <1. I tried 10 and got more locations than at 1.5. I imagine using something like 1000000 would just spit out every bp that was in the range of the cluster. This is why I am confused because statistically it seems that 1 should be the highest.

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@katja-hebestreit-6495
Last seen 4.4 years ago
United States

That is true, the FDR.loc should be restricted to be between 0 and 1. I will change this.

To figure out the problem here I would need reproducible data. Would it be possible for you to send me a subset of your data (e.g. only one chromosome) together with your code?

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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Yes, how should I send it? 

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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

I uploaded the .r script and chr 3 of the data, .bedgraph and .cov files, compressed into a tar.gz to my github @ https://github.com/naymikm/BiSeq_subset

Thank you very much!

Marcus

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Okay, thank you! I will look into it and will let you know! Cheers, Katja ----- Original Message ----- > From: "mnaymik [bioc]" <noreply@bioconductor.org> > To: katjah@stanford.edu > Sent: Thursday, April 16, 2015 10:06:51 AM > Subject: [bioc] A: BiSeq trimClusters FDR.loc confusion > Activity on a post you are following on support.bioconductor.org > User mnaymik wrote Answer: BiSeq trimClusters FDR.loc confusion : > I uploaded the .r script and chr 3 of the data, .bedgraph and .cov files, > compressed into a tar.gz to my github @ > https://github.com/naymikm/BiSeq_subset > Thank you very much! > Marcus > You may reply via email or visit > A: BiSeq trimClusters FDR.loc confusion
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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Hi Katja,

I figured out the issue. There was a problem with 2 of the samples that we decided to ultimately throw out due to sequencing quality issues, without these two samples the analysis runs fine. I do have one trivial question though just to be 100% sure... In the DMR results group 1 and group 2 correspond to the same order as the levels of factor(colData(rrbs)$group)?  In my case factor(colData(rrbs)$group) shows: 

Levels: L O

Hence, L is group 1 and O is group 2?

Thanks again,

Marcus

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Hi Marcus, Yes, exactly, the groups 1 and 2 correspond to the same order as the levels of the group factor. It's good that you don't run into this problem anymore. If you don't mind, I would still like to use your data to figure out why BiSeq showed this weird behavior. I just haven't had time yet. If you don't delete the files from Github before tomorrow I would still like to download them. Would that be okay for you? Cheers, Katja ----- Original Message ----- > From: "mnaymik [bioc]" <noreply@bioconductor.org> > To: katjah@stanford.edu > Sent: Wednesday, April 22, 2015 8:48:59 PM > Subject: [bioc] A: BiSeq trimClusters FDR.loc confusion > Activity on a post you are following on support.bioconductor.org > User mnaymik wrote Answer: BiSeq trimClusters FDR.loc confusion : > Hi Katja, > I figured out the issue. There was a problem with 2 of the samples that we > decided to ultimately throw out due to sequencing quality issues, without > these two samples the analysis runs fine. I do have one trivial question > though just to be 100% sure... In the DMR results group 1 and group 2 > correspond to the same order as the levels of factor(colData(rrbs)$group)? > In my case factor(colData(rrbs)$group) shows: > Levels: L O > Hence, L is group 1 and O is group 2? > Thanks again, > Marcus > You may reply via email or visit > A: BiSeq trimClusters FDR.loc confusion
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Hi Marcus,

Do you remember what the problem with the samples was, and how you figured it out? Because I am currently experiencing the same issue; I am not getting results unless I use FDR.loc = 1, and that seems too high.

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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Hi Katja,

Awesome thank you! Yes that is fine, I will leave them there for a while. To clarify, in the dataset we decided to throw out the samples T01 and  T07 which left 11 samples of L (control) and 9 samples of O (case).

Thanks,

Marcus

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Great! Thanks a lot! Katja ----- Original Message ----- > From: "mnaymik [bioc]" <noreply@bioconductor.org> > To: katjah@stanford.edu > Sent: Thursday, April 23, 2015 9:35:11 AM > Subject: [bioc] A: BiSeq trimClusters FDR.loc confusion > Activity on a post you are following on support.bioconductor.org > User mnaymik wrote Answer: BiSeq trimClusters FDR.loc confusion : > Hi Katja, > Awesome thank you! Yes that is fine, I will leave them there for a while. To > clarify, in the dataset we decided to throw out the samples T01 and T07 > which left 11 samples of L (control) and 9 samples of O (case). > Thanks, > Marcus > You may reply via email or visit > A: BiSeq trimClusters FDR.loc confusion
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mnaymik ▴ 10
@mnaymik-7522
Last seen 7.0 years ago
United States

Hi Katja,

Another question, I wanted to clarify what the median.p value is. Is this the median p-value for all sites within each DMR from the Wald test when testing for group effect?

Thanks,

Marcus

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Hi Marcus, Exactly, median.p is the median of all p-values arising from the CpG-wise Wald tests for group comparison. Cheers, Katja ----- Original Message ----- > From: "mnaymik [bioc]" <noreply@bioconductor.org> > To: katjah@stanford.edu > Sent: Monday, May 18, 2015 1:15:57 PM > Subject: [bioc] A: BiSeq trimClusters FDR.loc confusion > Activity on a post you are following on support.bioconductor.org > User mnaymik wrote Answer: BiSeq trimClusters FDR.loc confusion : > Hi Katja, > Another question, What exactly is the median.p value that is in the DMR > object refer to? I have been assuming that this is the p-value that was from > the Wald test when testing for group effect is this correct? > Thanks, > Marcus > You may reply via email or visit > A: BiSeq trimClusters FDR.loc confusion
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