Hi, I am looking to run a tandem mass spec experiment for proteomics.
Obviously I will need to validate the results of this using another method such as Western Blotting/Elisa.
The question is, do I need to validate all the hits i want to look at, or can I validate a selection of these across the range of say fold change and use these to show the methods are similar? (assuming that they show the same directional change between my cases and controls)
In addition, it depends on the statement made/ conclusion withdrawn. Pinpointing a pathway or a candidate gene would indeed require validation. You might afford to skip validation in profiling experiments given that your experimental design is flawless and you use stringent statistical analyses.
Matthew, I basically agree with Sebastian and Vipul: the depth of the validation depends on what you want to say or how much "strength" your results should/must have. Do you want to quantitate? Is precision important? LLOQ? What about linearity? Ion suppression? Effectivity of digestion? If you answer "yes", then you're talking about a classical validation (FDA, EMA) meaning, indeed, every result. Even if you're just screening, the results must have a certain validity. I don't see the necessity of validating the tests with a second method if the current method, itself, is validated. It's ok to do comparisons in the scope of a validation, but as I see it, that's not absolutely necessary. Good luck!
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