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- Posts: 77
- Joined: Thu Sep 22, 2011 5:02 pm
I would appreciate any comments, suggestions, resources, or references.
Thanks Kindly for the support!
-Best
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Discussions about GC-MS, LC-MS, LC-FTIR, and other "coupled" analytical techniques.
You can get reasonable separations with a 300 angstrom pore reversed phase column in that size range.. many (too many!) years ago (in the 80's I think) I was able to separate iodinated from non-iodinated insulin, mono from di iodinated, and the A and B chain mono iodinated forms from each other... and that was obviously before UPLC and without MS.Hi Thomas, we are just trying to quantify the amount in our formulation. I was not aware that intact analysis is possible because the protein is 6Kd.
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