I am working on carbonic anhydrase immobilization into MOFs.
I am facing problems with low enzyme loading..
The other issue is that when using p-NPA activity test to detect the activity of the enzyme at 400nm.. the MOF itself has peak at 400 nm so I am confused with the results..
What your suggestions?
Thanks in advance
Can you prepare samples of MOF with no enzyme attached to use as blanks? You could then subtract the blank absorbance from the absorbance of the MOF+enzyme.
Adam B Shapiro I did this as a baseline but there was still overlapping in the peaks of the MOF and the product
Does this mean that the enzyme was not effectively immobilized, or that the enzyme was indeed immobilized but had low activity? Answering this question will help determine the appropriate solution. To determine if the enzyme was immobilized successfully, you need to measure the activity of the unbound enzyme solution. If it shows significant activity, this indicates a problem with the immobilization procedure. If it shows no activity, this means that the enzyme was immobilized but its active site was blocked.
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