Bioequivalence and Bioavailability Forum

hi,

Please check pre dose sample with IS. if analyte area in this sample showing significant area as compare to standard 1 than pre dose sample can be repeated other wise not required to repeat samples.

by
kaushal

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Edit: Full quote removed. Please see this post! [Ohlbe]

Dear Alhas,

❝ If a predose (without IS) shows a very high concentaration

You can't calculate a concentration in a sample without IS, by comparison to a standard curve with IS ! Of course if you have a slight carry-over, or something your chromatographic software identifies as an IS peak, the software will calculate a concentration. But it is meaningless and it should be disregarded. All you can do with this sample is check that you have no interference at the retention time of your IS, and compare the analyte peak area to that of the first calibration sample.

Regards
Ohlbe

Hi,

I agree with kaushal that you have to check the same pre-dose with IS. If the peak area is similar than it can tells you if it's coming from the sample itself. This can mainly happen in pre-doses of period 2 if the wash out period is not enough.

❝ If a predose (without IS) shows a very high concentaration, as per the

❝ bioanalysit it is due to back calculation of analyte area, the analyte area

❝ is less than 20% compared to the Standard A.

Dear Alhas,

What ever your analysts said seems to be absolutely correct. How come one can estimate the concentration of the drug in a blank (predose sample) with out Internal standard.
Check the area at the RT of analyte and IS and it should meet your SOP criteria, If it meets then you can accept the data and no need to perform reanalysis.