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- Posts: 32
- Joined: Mon Oct 04, 2004 1:39 pm
I would like to know why ceffine only to be used to calibrate HPLC.
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Discussions about HPLC, CE, TLC, SFC, and other "liquid phase" separation techniques.

That's how it's done w/ older Shimadzus. You prepare a potassium permangenate solution series, shut off the detector's "autozero on wavelength change" function and step through different wavelengths at each solution concentration. From these numbers, molar absorbtivities are calculated...At the risk of sounding stupid, if you don't have a scanning detector you could make a "sufficiently concentrated" solution and manually fill the detector cell with it. You can then manually change the detector wavelength and record the absorbance. While the detector might have an autozero function whenever the wavelength is changed, there might be a way to switch this function off while you are performing the check. Somewhat tedious and time consuming, but perhaps quicker than perfoming multiple runs. Not sure if there is some problem with this approach.

It's not my procedure, but I would guess that the multiple concentrations serves to demonstrate linearity (across different wavelengths). If each concentration were prepared from a different weighing of the solid, you would also have 4 different molar absorbtivity values (per wavelength tested) to average. In theory, this minimizes the chance of systematic error skewing the values.DR, why use different concentrations?

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