[BioC] some basic questions

Richard Friedman friedman at cancercenter.columbia.edu
Sun Dec 4 00:47:24 CET 2011


Dear Anand,

 	I am not sure what you advisor means by "functionally group".

Best wishes,
Rich



On Fri, 2 Dec 2011, anand m t wrote:

> Dear Dr. Friedman,
>
> Thank you for the notes again. It was really helpful and my many questions
> got cleared after going through it.
> But what my adviser asking me to do is, i've normalized data (54 k probes),
> he's asking me to functionally group them all.
> After that, he wants me to perform significance test within each group to
> find out deferentially expressed genes.
> My question is how's that different from conventional way of finding DE
> genes and functionally grouping them ?? Is it valid??
>
> Dear Sean,
>
> I've data from HGU133 plus 2 array. I followed through the links but still
> i'm confused. I've attached a file for reference [this'a screen shot of a
> published data].
> In the attachment, the transcript audacin 3 gamma, is represented by 4
> different probe ID's and all are showing different intensity values.
> Now i want filter those probe ID's with significant deviation, from further
> analysis. How do i get this data of different probe's representing the same
> trascript ??
>
> Again sorry if my questions are lame, i'm new to microarray analysis and
> i'm getting confused and lost.
>
>
> On Wed, Nov 30, 2011 at 8:16 PM, Sean Davis <sdavis2 at mail.nih.gov> wrote:
>
>> On Wed, Nov 30, 2011 at 2:04 AM, anand mt [guest]
>> <guest at bioconductor.org> wrote:
>>>
>>> Hi all..
>>>
>>> i have following questions.
>>>
>>> 1) How many probesets represent a gene on microarray chip ?
>>>
>>
>> That depends on the array platform.  For a given platform, you can use
>> the annotation packages to answer this question.  To get started, take
>> a look at:
>>
>> http://bioconductor.org/help/workflows/annotation-data/
>>
>>> 2) How do i access raw intesity value of probes (before normalization) ?
>>
>> This will depend on the array platform and the software package you
>> are using to do your analysis.  Some specifics are probably needed.
>> To get started, be sure to take a look at:
>>
>> http://bioconductor.org/help/workflows/oligo-arrays/
>>
>>> 3) Do i need to read cdf file to do that ??
>>
>> Generally not.  Depending on the software package that applies, the
>> data from the CDF file are usually repackaged for use in bioconductor.
>>  Again, some specifics of your data and experiment are important.
>>
>>> 4) After pre-processing the data and normalization, we generally go for
>> significance tests and gene grouping. My question is, if i group the genes
>> before performing  significance test (say now i have 3 groups based on
>> apoptosis,cell cycle, DNA replication) and then perform significance test
>> within each group, will the results be same as that of conventional way ??
>> Is it a valid method to do so??
>>>
>>
>> You might take a look at this question and response on biostar:
>>
>>
>> http://biostar.stackexchange.com/questions/14796/gene-expression-analysis-microarrays-geneset
>>
>> Hope that helps.
>>
>> Sean
>>
>>
>>> Sorry if my questions are silly.
>>>
>>>  -- output of sessionInfo():
>>>
>>> --NONE--
>>>
>>> --
>>> Sent via the guest posting facility at bioconductor.org.
>>>
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>>
>
>
>
>

-- 
------------------------------------------------------------
Richard A. Friedman, PhD
Associate Research Scientist
Herbert Irving Comprehensive Cancer Center
Biomedical Informatics Shared Resource
Lecturer
Department of Biomedical Informatics
Box 95, Room 130BB or P&S 1-420C
Columbia University Medical Center
630 W. 168th St.
New York, NY 10032
(212)305-6901 (5-6901) (voice)
friedman at cancercenter.columbia.edu
http://cancercenter.columbia.edu/~friedman/

"The last 250 pages of the last Harry Potter
book took place in one day because alot
happened in that day. All of Ulysses takes
place in one day and nothing happened in that day."
-Rose Friedman, age 11



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