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- Posts: 53
- Joined: Thu Dec 13, 2012 6:29 pm
Our system: Waters Acquity UPLC coupled to Xevo TQ-S MS/MS detector
Mobile Phase: MeOH/Water gradient with 0.1% formic acid and 10mM Ammonium Formate buffer
Column: Waters Atlantis HSS T3 and Waters XBridge BEH C18 for backup/additional confirmation
Inject: 4uL of a 0.25g/mL extracted sample in MeOH/Formic/Acetonitrile (modified QuEChERS), samples consist of various fruits and vegetables, but we are starting a new study for salmon
Pesticide Screen: 140 pesticides, 2 transitions each
Calibration: 4 points (1x, 2x, 5x, 10x LOD), origin ignored, 1/x weight, concentration range varies depending on pesticide sensitivity (lowest is 1ppb (Bupirimate, Carbendazim, Fluridone, Triazphos... to name a few) and highest is 100ppb (Pendimethalin, Pyrimethanil))
For those with a similar setup/application, what are the typical maintenance protocols you follow? I have been cleaning the cone assembly almost weekly, but I still have poor sensitivity so I clean the Ion Block - which is visibly dirty - and sensitivity improves slightly, but not back to where it was right after PM by service engineer. Am i overloading the system because my calibration standards too high? Injection volume too large? Sample concentration too high? Any thoughts/comments/suggestions welcomed on this!!
I am working on validating the LOD for all compounds in this screen, as some are definitely not true LODs - SNR of >1000 for 1xLOQ standard!?!?!
Any tips for me as I work on this?
Thank you for your time!
fyi - we also analyze these samples using GC-QQQ but maintenance protocols are established as it has been in use longer, LC-MS/MS is newer and no protocols established as of yet....hopefully soon this will change!
Mobile Phase: MeOH/Water gradient with 0.1% formic acid and 10mM Ammonium Formate buffer
Column: Waters Atlantis HSS T3 and Waters XBridge BEH C18 for backup/additional confirmation
Inject: 4uL of a 0.25g/mL extracted sample in MeOH/Formic/Acetonitrile (modified QuEChERS), samples consist of various fruits and vegetables, but we are starting a new study for salmon
Pesticide Screen: 140 pesticides, 2 transitions each
Calibration: 4 points (1x, 2x, 5x, 10x LOD), origin ignored, 1/x weight, concentration range varies depending on pesticide sensitivity (lowest is 1ppb (Bupirimate, Carbendazim, Fluridone, Triazphos... to name a few) and highest is 100ppb (Pendimethalin, Pyrimethanil))
For those with a similar setup/application, what are the typical maintenance protocols you follow? I have been cleaning the cone assembly almost weekly, but I still have poor sensitivity so I clean the Ion Block - which is visibly dirty - and sensitivity improves slightly, but not back to where it was right after PM by service engineer. Am i overloading the system because my calibration standards too high? Injection volume too large? Sample concentration too high? Any thoughts/comments/suggestions welcomed on this!!
I am working on validating the LOD for all compounds in this screen, as some are definitely not true LODs - SNR of >1000 for 1xLOQ standard!?!?!
Any tips for me as I work on this?Thank you for your time!
fyi - we also analyze these samples using GC-QQQ but maintenance protocols are established as it has been in use longer, LC-MS/MS is newer and no protocols established as of yet....hopefully soon this will change!
BHolmes
Any problem worthy of attack, proves its worth by hitting back...never give up!
Any problem worthy of attack, proves its worth by hitting back...never give up!
