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- Posts: 56
- Joined: Fri Aug 19, 2011 4:49 am
I'm trying to get my head around the chemistry of the new BP dissolution method for levothyroxine, specifically the sample pre-treatment step which says:
"To a 5mL aliquot add 200 mcL of 0.1 M NaOH and 125 mcL of a 2% v/v solution of diethylamine"
I understand the purpose of the NaOH, since the dissolution medium is water, but why would you also need to add diethylamine? The mobile phase 30% ACN/70% dilute phos acid in water and suggested column is Spherisorb S5 CN, which as far as I can tell isn't an ion exchange column.
The use of triethylamine in mobile phases I understand. The addition of diethylamine to a sample has me beat, and I have tried googling.
The other thing about the BP method that seems odd is it says to inject 150 mcL which seems a very large volume to me.
By way of background, this is for a student research project so we're not "bound" to follow the BP method for analysis. I'd like to avoid adding diethylamine if it's unnecessary, simply because it's another potential source of contamination when reading at 223 nm. However, since the BP only just this year introduced the dissolution test I'm thinking there must be a reason for it?
Thanks
"To a 5mL aliquot add 200 mcL of 0.1 M NaOH and 125 mcL of a 2% v/v solution of diethylamine"
I understand the purpose of the NaOH, since the dissolution medium is water, but why would you also need to add diethylamine? The mobile phase 30% ACN/70% dilute phos acid in water and suggested column is Spherisorb S5 CN, which as far as I can tell isn't an ion exchange column.
The use of triethylamine in mobile phases I understand. The addition of diethylamine to a sample has me beat, and I have tried googling.
The other thing about the BP method that seems odd is it says to inject 150 mcL which seems a very large volume to me.
By way of background, this is for a student research project so we're not "bound" to follow the BP method for analysis. I'd like to avoid adding diethylamine if it's unnecessary, simply because it's another potential source of contamination when reading at 223 nm. However, since the BP only just this year introduced the dissolution test I'm thinking there must be a reason for it?
Thanks
