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protamine problems

Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.

4 posts Page 1 of 1
hello,

could anyone help me with a problem im having,
i have a protamine analyte giving a 201nm lambda max abs,
the literature say for hplc:
UV 214nm,
h20/acn/tfa (qs/8%/0.15%)
pH 2.5
waters size exlusion column,

my problem is,
im getting negative peak for protamine. this is no great surprise but im having trouble composing a mobile phase with a lower abs than my analyte,
any suggestions would be gratefully taken.
derboyl

Hi Derboyl,

It’s TFA that absorbs too much light, especially in combination with ACN. But you knew it already – I presume. What I wonder about in this case is, what in earth’s name, is TFA’s role in Size Exclusion Chromatography? Just drop it and if you need the pH to be 2.5 (and I would expect, you do) then make 0.05 M phosphate buffer, mix it with 10 % or so ACN and you’re back in business.

Best Regards
Learn Innovate and Share

Dancho Dikov

hello danko,
thanks for that,

thruthfully, i didnt realise TFA absorbed more light with ACN, i was under the impression it was transparent at lower wavelenghts, less than 200nm
so i will try your suggestion and drop the TFA.
incidently, TFA was used by the autors of the method useing size exclusion columns that im trying to replicate and develop. i was curious about its use myself.

Just about everything absorbs below 200nm, TFA absorbs even far up.
Some years ago I tried TFA to decrease interactions of an antibody with the stat. phase in SEC. If you do a search of this forum you may find one result: I permanently decreased the separation power of the column (TSKgelSuper SW 3000). Incidentally, I still don´t know why, and that in spite of enormous efforts by local representatives of Tosoh to get info from Tosoh headquarters.
4 posts Page 1 of 1

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