> Please remove me from the mailing list.
>
> Klara Balint
> Postdoctoral Fellow
> Dr. George Coukos` laboratory
> University of Pennsylvania
> 431 Curie Blvd, BRB 2/3, Rm 1331
> Philadelphia, PA 19130
> Phone: 215-573-4897
> Fax: 215-573-7627
> Email: [hidden email]
>
> ----- "Guy Cox" <[hidden email]> wrote:
>
>  
>> In terms of quantitation, surely the best result is to forget RGB
>> imaging altogether. From what I recall DAB gives a browny-black
>> colour, so a greyscale image should do fine. But I do echo Julio's
>> doubts about quantitation. If you are working in fluorescence, rather
>> than picking one RGB channel the best thing is to get a filter (or set
>> a spectral range) which matches your fluorochrome and excludes
>> anything else, then again record an image of just that channel.
>>
>> Guy
>>
>>
>>
>> Optical Imaging Techniques in Cell Biology
>> by Guy Cox CRC Press / Taylor & Francis
>> http://www.guycox.com/optical.htm
>> ______________________________________________
>> Associate Professor Guy Cox, MA, DPhil(Oxon)
>> Electron Microscope Unit, Madsen Building F09,
>> University of Sydney, NSW 2006
>> ______________________________________________
>> Phone +61 2 9351 3176 Fax +61 2 9351 7682
>> Mobile 0413 281 861
>>    
>
>