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- Posts: 24
- Joined: Thu Apr 24, 2014 3:25 pm
Hello I was looking for advice on how to deal with this problem.
First I would like to describe WHY I think i'm having these problems and ask for general advice on how to gain the skills I need to not have these problems anymore...because thats part of why I think I don't know what to do. I'm a synthetic chemist by training, and lcms was previously just used to analyze reactions or product mixtures without caring about the QUALITY of the data. But now I am doing quant. work and it does matter very much If I am getting the best peakshape possible. knowing how to troubleshoot to get this quality data is my problem, so any resources you could suggest for gaining these skills is helpful.
I have oxymorphone and noroxycodone (and their deuterated counterparts) that elute at almost the same time. The peaks are not fully resolved and have some overlap.
Anyhow, the chromatography can't really be changed much because there are a million other compounds in this method and changing the chrom might throw alot of other stuff off and cause many problems at this point.
The problem in data analysis: The peaks are not being identified properly by the software. IE its not choosing what the peak for the correct compound and not integrating each peak seperatley as if it was a totally isolated peak on a chromatogram (like It would if I had nothing near it). I also had use specific product ions for each one, since if you choose to use other product ions for these compounds they will be very similar masses you are looking for. Should I try adding more product ions to the compounds to be used in their identification? Because as of right now...its identifying "both of them" as one compound for one of them....while for the other one it seems to identify just the one relevant peak.
I am using a shimadzu lcms with labsolutions software.
Can anyone provide recs on how to go about solving this problem so I can get on to the quantitation aspect?
also another question.
I have another drug in this method that I have tried optimizing and just cannot get good peak resolution. what do you suggest I do to fix this without changing the chromatography? This compound ionizes well and is very similar to other compounds that are working well. But when the method is run with LC and the whole 9 yards peak is too broad.
thanks
First I would like to describe WHY I think i'm having these problems and ask for general advice on how to gain the skills I need to not have these problems anymore...because thats part of why I think I don't know what to do. I'm a synthetic chemist by training, and lcms was previously just used to analyze reactions or product mixtures without caring about the QUALITY of the data. But now I am doing quant. work and it does matter very much If I am getting the best peakshape possible. knowing how to troubleshoot to get this quality data is my problem, so any resources you could suggest for gaining these skills is helpful.
I have oxymorphone and noroxycodone (and their deuterated counterparts) that elute at almost the same time. The peaks are not fully resolved and have some overlap.
Anyhow, the chromatography can't really be changed much because there are a million other compounds in this method and changing the chrom might throw alot of other stuff off and cause many problems at this point.
The problem in data analysis: The peaks are not being identified properly by the software. IE its not choosing what the peak for the correct compound and not integrating each peak seperatley as if it was a totally isolated peak on a chromatogram (like It would if I had nothing near it). I also had use specific product ions for each one, since if you choose to use other product ions for these compounds they will be very similar masses you are looking for. Should I try adding more product ions to the compounds to be used in their identification? Because as of right now...its identifying "both of them" as one compound for one of them....while for the other one it seems to identify just the one relevant peak.
I am using a shimadzu lcms with labsolutions software.
Can anyone provide recs on how to go about solving this problem so I can get on to the quantitation aspect?
also another question.
I have another drug in this method that I have tried optimizing and just cannot get good peak resolution. what do you suggest I do to fix this without changing the chromatography? This compound ionizes well and is very similar to other compounds that are working well. But when the method is run with LC and the whole 9 yards peak is too broad.
thanks
