array CGH
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Lisa Luo ▴ 40
@lisa-luo-1830
Last seen 10.2 years ago
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@sean-davis-490
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On Thursday 12 October 2006 23:34, Lisa Luo wrote: > Dear List, > > I have a set of BAC array CGH data to analysis. I am new to this kind of > analysis. Could anyone please recommend me a good package? > > I read some papers on aCGH. For the size of BAC clones, is averaging a few > probes a good idea? I tried DNAcopy and I am not happy with the results > either. Another question: Can we use the ratio to call it amplification > or deletion? In my normal samples, I should expect ratio to be about 1. > But ratios in some probes/chromosomes tend to be high and ratios in another > probes/regions tend to be lower. So how to use the ratio? Lisa, Segmentation methods (GLAD, DNAcopy, aCGH, etc.) are the way to go here, as others have suggested. Averaging is not a good idea given the availability of segmentation methods, which accomplish the same goal of reducing noise as does averaging, but do so with minimal loss of resolution. The ratio is the number of interest, yes. Your normal samples should have a ratio of approximately 1, yes. However, because of technical variation, some probes and regions may drift a bit away from 1. If you have these normal/normal hybs, you can use these to help you to determine where your data (in terms of ratio) becomes believable. Another useful measure is to look at the ratios that you see on the X-chromosome when comparing two samples with different genders in comparison to the ratio that you see for the autosomes. Finally, were there DNA quality issues that could explain some variation in your results? Were the samples amplified or directly labeled? Sean
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On Friday 13 October 2006 10:04, Lisa Luo wrote: > Thank you, Sean and all others who replied to me. > > First for segmentation method, I am not satisfied with DNAcopy. A > extreme in this case is that when I have a break point near the middle, it > could not detect it if I used the SD trim method. Or it gave too many > breaking points. You may have to change parameters multiple times to get the results that you like. Also, you might consider using a merging function like that implemented in snapCGH rather than using trimming, but others may not agree here. > Also, it can not detect full chromosome change that you > have to rely on the ratio. The goal of the segmentation methods is not to call gains and losses, but to determine regions of constant copy number. There is another step in the process to determine whether a copy number estimate actually represents a gain or loss. > Is BAC array CGH single strand PCR arrays? If so, should repeat affact > the result? In my tumor samples with opposite sex for control, I found > that the ratio for X varied from sample to sample. In one sample, it is > even 1. The explaination I got is that chrX has more repeat regions. Are > you suggesting that DNA quality may play a role in this? Of course quality plays a role in the array result--both quality of the arrays and quality of the DNA. If you have arrays on which you have a male and a female hybed and the mean of the X-chromosome is the same of the mean of the autosomes, there are a few explanations: 1) Sample mixup--the samples are actually the same sex 2) One of the samples has either gained/lost an X chromosome (cell line artifact, if the samples are from cell lines) 3) The processing/hybing of the array failed for some reason 4) Probes are somehow mismapped, either by you or by the person supplying the annotation. 5) There actually IS a difference between the X-chromosome and the autosomes, but the difference is small or difficult to notice given the noise; for practical purposes, the X-chromosome/autosome ratio represents signal and noise can be quantified in numerous ways (SD, MAD, etc). Arrays with low signal-noise-ratio for whatever reason will look like there is very little difference between the autosomes/X-chromosome. > I am planning to look at each BAC at one time, comparing tumor vs normal. > Is this a good idea? This sounds fine, but I would use the data calculated from the segmentation results as the input to your test; this will reduce the noise associated with individual probes. Also, note that the data are not likely to be normally distributed at a given probe across samples, since each sample is potentially drawn from a different population (mean copy number). Sean
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@alberto-goldoni-711
Last seen 10.2 years ago
There are tho main packages: GLAD (plus MANOR for the qualit? test) and aCGH Best regards Dr Alberto Goldoni Medical Genetics Unit S. Orsola-Malpighi Hospital Via Massarenti n.9, Pad 11 40100 Bologna, Italy Mobile Phone: +39-338-4145970 Fax: +39-051-636-4004 alberto.goldoni at eurogene.org www.eurogene.org www.lagem.it -----Messaggio originale----- Da: bioconductor-bounces at stat.math.ethz.ch [mailto:bioconductor-bounces at stat.math.ethz.ch] Per conto di Lisa Luo Inviato: venerd? 13 ottobre 2006 5.34 A: bioconductor Oggetto: [BioC] array CGH Dear List, I have a set of BAC array CGH data to analysis. I am new to this kind of analysis. Could anyone please recommend me a good package? I read some papers on aCGH. For the size of BAC clones, is averaging a few probes a good idea? I tried DNAcopy and I am not happy with the results either. Another question: Can we use the ratio to call it amplification or deletion? In my normal samples, I should expect ratio to be about 1. But ratios in some probes/chromosomes tend to be high and ratios in another probes/regions tend to be lower. So how to use the ratio? Thank you so much for your help! Lisa --------------------------------- [[alternative HTML version deleted]] _______________________________________________ Bioconductor mailing list Bioconductor at stat.math.ethz.ch https://stat.ethz.ch/mailman/listinfo/bioconductor Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor
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Mark Dunning ▴ 320
@mark-dunning-1634
Last seen 10.2 years ago
Hi Lisa, The snapCGH package might be a good place to start because it allows you to try out methods from the most common CGH packages (GLAD, aCGH, DNAcopy etc..) and displays the results in a common format, allowing for easy comparison. Regards, Mark On Oct 13 2006, Lisa Luo wrote: >Dear List, > > I have a set of BAC array CGH data to analysis. I am new to this kind of > analysis. Could anyone please recommend me a good package? > > I read some papers on aCGH. For the size of BAC clones, is averaging a > few probes a good idea? I tried DNAcopy and I am not happy with the > results either. Another question: Can we use the ratio to call it > amplification or deletion? In my normal samples, I should expect ratio to > be about 1. But ratios in some probes/chromosomes tend to be high and > ratios in another probes/regions tend to be lower. So how to use the > ratio? > >Thank you so much for your help! > >Lisa > > >--------------------------------- > > [[alternative HTML version deleted]] > > _______________________________________________ Bioconductor mailing list > Bioconductor at stat.math.ethz.ch > https://stat.ethz.ch/mailman/listinfo/bioconductor Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > -- Mark Dunning PhD Student Computational Biology Group Hutchison / MRC Research Centre Department of Oncology University of Cambridge Hills Rd, Cambridge CB2 2XZ Email : md392 at cam.ac.uk Phone : +44 (0) 1223 763380
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@hilmar-berger-1799
Last seen 10.2 years ago
Hi Lisa, if after applying segmentation methods to your data the normal samples still indicate gains or losses you might want to have a look at http://projects.tcag.ca/variation/ for a list of known large scale copy number polymorphims. Hilmar Lisa Luo schrieb: > Dear List, > > I have a set of BAC array CGH data to analysis. I am new to this kind of analysis. Could anyone please recommend me a good package? > > I read some papers on aCGH. For the size of BAC clones, is averaging a few probes a good idea? I tried DNAcopy and I am not happy with the results either. Another question: Can we use the ratio to call it amplification or deletion? In my normal samples, I should expect ratio to be about 1. But ratios in some probes/chromosomes tend to be high and ratios in another probes/regions tend to be lower. So how to use the ratio? > > Thank you so much for your help! > > Lisa > > > --------------------------------- > > [[alternative HTML version deleted]] > > _______________________________________________ > Bioconductor mailing list > Bioconductor at stat.math.ethz.ch > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor > -- Hilmar Berger Studienkoordinator Institut f?r medizinische Informatik, Statistik und Epidemiologie Universit?t Leipzig H?rtelstr. 16-18 D-04107 Leipzig Tel. +49 341 97 16 101 Fax. +49 341 97 16 109 email: hilmar.berger at imise.uni-leipzig.de
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