>
> Search the CONFOCAL archive at http://listserv.acsu.buffalo.edu/cgi-
> bin/wa?S1=confocal
> =
> Hi Maria,
>
> It's difficult to give a precise answer without knowing how much you
> already know or don't know. But basically:
>
>
> 1. Prepare all samples in the same manner; ideally at the same time
>
> 2. Get good images (maximize the dynamic range with your microscope
> system): on a confocal, try to get the background close to, but not
> equal to zero, and get your highest signals close to the max
> intensity limit, but not saturated.
>
> 3. Collect all images under the same conditions ; ideally, collect
> them back to back on the same day, so as to minimize any instrument
> (and operator) variability. Adjust settings for the brightest sample,
> and use the same for all other samples. If images obtained this way
> are not good and you need to change imaging parameters between
> samples, you should either include reference standards (e.g. beads),
> or do the appropriate calculations to normalize results (but this may
> be complicated, and not necessarily accurate)
>
>
> 4. Use your favorite software to measure the pixel intensities
> (total, average, intensity profile, etc, depending on what you need
> to know) in your regions of interest; ImageJ is great as a start:
>
> http://rsbweb.nih.gov/ij/
>
> If you want to measure labeling intensities in the entire
> microorganisms, then you should image the whole cells in 3-D,using
> proper sampling in x, y, and z, and use some 3-D imaging software to
> get the numbers. You can also do that with ImageJ by analyzing all
> relevant sections (or projections of all relevant sections)
>
>
> If you can make it this far, then you should use the additional
> suggestions (such as Jim Pawley's 39 steps...)
>
> If you can make it that far but still have difficulties, let us know
> what the specific problem is...
>