Hello,

To those who have experience in using flow cytometry for counting bacteria (anexic cultures), I would like to know what is the detection limit.

I just had a kind of argument with a colleague about the sensitivity of FACS compared to CFU/ml counting by plating. 

My opinion is that by plating we cannot obtain a "absolute" or "real" number of bacteria, and that we need to use other method such as FACS, most over when we face low concentration. This method is nevertheless suitable for comparing 2 conditions, as in both cases we are suffering the same biases, but not to obtain an "absolute" counting of bacteria contained in a solution.

In order to do so, I suggested FACS as an alternative, but I was said that FACS is not sensitive enough. My colleague claimed that culture plating is much more sensitive. 

I disagree.

Please, could you let me know what do you think about it? I would appreciate some elucidation about this matter.

Thanks in advance

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