Scaling fcs files with flowCore
1
0
Entering edit mode
Jiang, Mike ★ 1.3k
@jiang-mike-4886
Last seen 3.1 years ago
(Private Address)

 

On 04/05/2016 12:15 AM, TODOROV HELENA p1001837 wrote:
>
> This is how I scale the matrix :
>
>
> > b<- read.FCS(fcs​_file,transformation="scale")
>
> > mat<-exprs(b)
>
> > scaled_matrix<-apply(mat,2,scale)
>
>  
> ​> scaled_b<-new("flowFrame", exprs=scaled_matrix, parameters=parameters(b), description=description(b)) 
> ​> write.FCS(scaled_b, outFile)
>
> But I have issues reading the generated fcs file. I suppose it may come from the fact that description parameters such as $PnE, $PnR, MaxRange... no longer correspond to the values of parameters?
>
> Also, could you tell me why the "transformation = "scale" " option from the read.FCS() function does not transform the data so that each markers mean = 0 and sd = 1?
>
> Thank you in advance
> Helena
>>
>>
>
> De : Mike <wjiang2@fhcrc.org>
> Envoyé : lundi 4 avril 2016 20:01
> À : TODOROV HELENA p1001837
> Cc : Emilie Westeel
> Objet : Re: Scaling fcs files with flowCore
>  
> What kind of scaling method do you use to transform the data?
>
> On 03/29/2016 03:08 AM, TODOROV HELENA p1001837 wrote:
>>
>> Dear Dr Jiang,
>>
>>
>> I've encountered some issues to scale my fcs data. I use the function :
>>
>>
>> ​> b<- read.FCS(fcs​_file,transformation="scale")
>>
>>
>> ​But the transformed data are not scaled per marker. Indeed, if I check the summary of the object I generated, the mean for each marker is different from 0 and the sd is different from 1 (I attached a screenshot of this summary to this mail). Is there any way to scale the data per marker with flowCore/ or another Bioconductor package?
>>
>>
>> Also, I transformed my data manually (by extracting the matrix and scaling it per column), but the files I regenerate with the following functions :
>>
>>
>> > scaled_b<-new("flowFrame", exprs=scaled_matrix, parameters=parameters(b), description=description(b)) 
>>
>>
>> > write.FCS(scaled_b, outFile)
>>
>> present some problems when I try to read them with cytometry data analysis tools such as Phenograph, Visne, Scaffold. I tried to change some parameters manually, like the Rmin Rmax ranges that changed when I scaled the exprs matrix, which worked for some files but not for all, and which is also very time consuming. So I was wondering if there was any way to efficiently regenerate a description and parameters which correspond to the new matrix I generate, to create an FCS file that would be readable again?
>>
>> Thank you in advance,
>>
>> Helena Todorov
>>

flowCore flowcytometry • 2.2k views
ADD COMMENT
0
Entering edit mode
Jiang, Mike ★ 1.3k
@jiang-mike-4886
Last seen 3.1 years ago
(Private Address)

The behavior of transformation="scale" in 'read.FCS' is not as what you thought. Type '?read.FCS' to read more carefully about 'transformation' argument. It is actually about  'logarithmic amplification'  when the data is stored as 'logarithmic scale'.  See '$PnE' section of 'FCS3.1 standard'(http://isac-net.org/PDFS/90/9090600d-19be-460d-83fc-f8a8b004e0f9.pdf) for more details.

Based on what you've described, your custom transformation should be done through 'transform' method after 'fcs' is loaded. e.g.

data("GvHD")
fr <- GvHD[[1]]
chnl_to_transform <- c("FL1-H", "FL2-H")
translist <- transformList(chnl_to_transform, scale)
fr_trans <- transform(fr, translist)

Type '?transformList' for more help on this.

ADD COMMENT
0
Entering edit mode

Thank you Mike, this function is working perfectly !

ADD REPLY

Login before adding your answer.

Traffic: 692 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6