I am doing analysis of Cyclosporine A by UV spectrophotometer. I've standardized linearity for CyA at 210nm using acetonitrile as the solvent. But during time-bound solubility studies, the absorbance readings using the same protocol are not correct. Is it right to use UV for CyA? What could be the reason for random absorbance readings?
The recorded peak may be an artifact (if the recorded absorbance is very noisy, you may be sure about this issue). Record the acetonitrile spectrum: if it is highly absorbing at 200...220 nm, change it. Use a HPLC grade acetonitrile.
https://www.shimadzu.com/an/hplc/support/lib/lctalk/35/35lab.html
Can you provide the image of the recorded spectra for acetonitrile and cyclosporin A?
Thank you for your reply. I am using HPLC grade Acetonitrile for the studies. I used the same for full scan and linearity standardization. It's only during the detection of my samples, the readings are random and too high, i.e around Abs 2.5. Is it still possible to use UV?
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