Hey everyone!
i´m pretty new in using ImageJ, and sometimes i have doubts than don´t meet an answer so easily... i´m trying to quantify the colocalization of two proteins in cultured cells. I mark each protein with a fluorofore (red and green) and i take confocal micrographies. Since i´m going to repeat the experiment several times (obviously), i´m very careful in keeping always the same adquisition parameters in the microscope (voltage of PMT). Afterwards, i correct the background with "background substraction", the same rolling ball in the cases. That gave reasonable results in some experiments, but in the last one i got a very dim intensity in the channel for red colour. It is so that, when quantifying (i run the plugin "colocalization thresholds" for that), the threshold set is below zero, or above the maximum intensity value in any pixel of the image!! Is it neccesary to keep constant those parameters inter- experimentally? Or, can i define them for each experiment? I don´t know if i explained my situation properly so one can understand it. Sorry, i´m not familiar with these words and concepts. Thanks! i hope someone can help me! i don´t want to waste time doing non-correct analysis!! Best regards, Itsaso. ******************************** Itsaso Garcia-Arcos Department of Physiology, University of the Basque Country Medical School UPV/EHU, Spain. ******************************** |
I'm glad that your brought this up. I am also new to ImageJ, and I'm trying
to use it to measure colocalization, with not much luck. I work with spinal cord sections double- and triple-labeled with several antibodies. I take confocal images with a Leica microscope. This is what I got so far... - I can't get ImageJ (v1.37f, with the WCIF load of plugins) to open my Leica stacks. It does open the individual TIFF files. - I have used the Intensity Correlation Analysis (ICA) and Colocalization Threshold (CT) plugins on matched pairs of optical sections (individual TIFF fiels). - I ran several controls. Positive controls are two antibodies (different species) labeling the same epitope (neurokinin 1 receptors or the peptide CGRP). This should give maximal colocalization. Negative controls are two antibodies that are not expected or observed to colocalize. - Of all the parameters produced by the plugins, only the Pearson's Correlation Coefficient (Rr) seems realistic. Mander's Overlap Coefficient (R) and Mander's Correlation Coefficients (M1 and M2) are always high, for both positive and negative controls. - The histograms produced by the plugins correspond well with the expected levels of colocalization, but they seem to have little relationship with R, M1 and M2. - I am also using another program, Imaris Colocalization, to analyze the same data. I got a free trial license until the end of May. Imaris loaded the whole Leica stacks without problem, and analized them together. It produced much more realistic parameter values than ImageJ. - Imaris also has an automatic thresholding feature for colocalization. However, this feature failed for some data stacks. For the other data, it tend to give colocalization vaues that are too high (even for negative controls). I decided not to use it, and set the threshold by eye. I don't mean to advertise for Imaris. I much rather not spend the money and use ImageJ. Imaris is quite expensive! But this is where I am right now... To adress your question, I think that background subtraction is redundant with thereshold. Why eliminate some dark pixels if you are going to exclude them from the analysis later on, by setting a threshold? Also, the important Rr parameter is independent of thereshold, and my instinct is to obtain it for the raw date. By doing background subtraction you are biasing the data already. If you are doing things right on the confocal, your background should be very low, anyway. According with my experience with Imaris, threshold should be set "by eye", and a bit high. I use a pixel value of 60-80. Automatic threshold can be problematic. If you use it, you should run some controls, both positive and negative. I hope this helps you... If somebody reads this and can help with my problems with ImageJ, I'll be grateful. Buena suerte! Juan Carlos Marvizon |
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