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Vitamins quantification
Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.
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Hi everybody! I am trying simultaneous quantification of vitamins A, E and D3. I tested them in spectrometry UV to know the best wavelenght for the LC analysis and I found different wavelengh for each one. Now, I have a doubt: have the wavelengh choosed for run LC an influence on the peak areas of the vitamins? How I chose the best wavelengh for them together? Thank you in advance
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Below is are fat soluble vitamins separated on Cadenza CD-C18 (UV @ 280nm):
http://www.imtaktusa.com/site_media/fil ... TI121E.pdf
http://www.imtaktusa.com/site_media/fil ... TI121E.pdf
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Since the question, "have the wavelengh choosed for run LC an influence on the peak areas of the vitamins?" has not been addressed:
Of course, if you choose a wavelength where your analyte does not absorb you don´t get a peak at all.
If your detector allows this you can change the wavelengths to the max lambda of each compound in the region where it elutes. According to Bryan a good compromise is to use 280 nm for all. In any case you have to calibrate.
Of course, if you choose a wavelength where your analyte does not absorb you don´t get a peak at all.
If your detector allows this you can change the wavelengths to the max lambda of each compound in the region where it elutes. According to Bryan a good compromise is to use 280 nm for all. In any case you have to calibrate.
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