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Problematic peaks for Gabapentin and Phe-Gly IS

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Problematic peaks for Gabapentin and Phe-Gly IS

avatar
ghie malig
Hi again everyone!

The reason why I'm looking for alternative IS here in the forum is because of the probrematic peaks of Gabapentin and Phenyl Glycine IS which I was able to separate at low pH. of around 3.1 I'm getting a tail like peak after the main peak for both analytes.

M.P. 0.02 M KH2PO4/ACN, 50:50, pH 3.1
Sample Prep: GBP is spiked in Plasma and precipitated with 20% Perchloric acid. 100 uL of Borate buffer, pH 10 is added to 10 uL of the supernatant followed by addition of derivatizing agent OPA-MPA solution.
50 uL is injected to LC with Fluorescence detector.
Column: C18, 150 x 4.6 (stable at pH range 2-7.5)

The reference journals i got even set the pH at around 2 but they did not get this tail like peak after the main peak of the analytes. If I increase the pH at 6.2, the tail-like peak disappeared but I'm not getting a good separation from the artifacts of the plasma though separations of the GBP and Phe-Gly is achieved. :(

I'm not sure if the tail-like peak is a degradant of both analytes at low pH because some journals used to work at even lower pH range. Pls. help! How will I eliminate the tail like peaks I am encountering in my chromatogram? Can I put anything that will make the peaks fused as one peak? The final product of derivatization is an isoindole ring. thanks! :lol:

-ghie-

avatar
Mark Tracy
I suspect that your mobile phase buffer may not have enough capacity to counter the pH 10 buffer in the sample. One way to check: Inject only half as much and see if the peak shape changes. Phosphate buffer is not a good choice at pH 3; formate is much better, and is compatible with your separation and detection system.
Mark Tracy
Senior Chemist
Dionex Corp.

avatar
Uwe Neue
You are also likely to get a better peak shape as you get closer to pH 2 with your phosphate buffer, since the phosphate will have a better buffering capacity.

avatar
ghie malig
Hi!

Thanks for all your help. I was able to solve the problematic peaks of Gabapentin and Phenyl Glycine Internal Standard. I lowered the pH to 2.1 and it seems that Phospate buffered well at this pH level. But I have another problem though. There is a small endogenous peak in the blank plasma that i cannot resolve with a change of ratio. Since I cannot play anymore with pH because if I raise the pH phenyl glycine will not be retained anymore. It is at pH 2 that the analytes are well resolved. The artifact in the blank moves with the IS Phenyl Glycine when the ratio of the mobile phase is changed. The analytes are OPA-MPA derivatized compounds. Would an addition of TFA or ion pair would resolve the problem? I'm not sure if this would work at low pH level. Any feedback? Thanks!

-ghie- :lol:
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