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- Posts: 15
- Joined: Wed Jan 12, 2011 10:13 am
Dear all,
I am developing a UPLC method for the simultaneous analysis of 6mercaptopurine (drug) and its metabolites (thioguanine, 6methylmercaptopurine). I am using an Acquity (Waters) system
I have employed a great variety of conditions. The best being the following:
Acquity BEH C18 [1.7 um, 2.1 x 100 mm]
Tcolumn= 25C
A = 96:1:3 0.02M KH2PO4(pH 2.25): MeOH : AcN
B = AcN, 0.1% formic acid
flow rate of 0.5ml/min
gradient conditions of 0.0-10 min, 100%A to 80%A
10-10.5 min, back to 100%A
10.5-12 min, 100%A
I get very nice peaks for all analytes. However, the two metabolites being rather polar elute at 1.322 and 1.165 min, respectively (the drug elutes at 4.551 min). How can I improve elution times (later within run) and peak separation??
I really need your feedback on this..
Kind Regards,
T
I am developing a UPLC method for the simultaneous analysis of 6mercaptopurine (drug) and its metabolites (thioguanine, 6methylmercaptopurine). I am using an Acquity (Waters) system
I have employed a great variety of conditions. The best being the following:
Acquity BEH C18 [1.7 um, 2.1 x 100 mm]
Tcolumn= 25C
A = 96:1:3 0.02M KH2PO4(pH 2.25): MeOH : AcN
B = AcN, 0.1% formic acid
flow rate of 0.5ml/min
gradient conditions of 0.0-10 min, 100%A to 80%A
10-10.5 min, back to 100%A
10.5-12 min, 100%A
I get very nice peaks for all analytes. However, the two metabolites being rather polar elute at 1.322 and 1.165 min, respectively (the drug elutes at 4.551 min). How can I improve elution times (later within run) and peak separation??
I really need your feedback on this..
Kind Regards,
T
