N-Glycosidase F Protocol & Troubleshooting
Protocol
Using N-glycosidase F (Product No. NGLYF-RO) with less soluble proteins in PBS and other non-denaturing buffers
Consider using the following protocol:
Dilute 100 μg protein in 250 μL solution of 8 M urea + 0.5 M ß-mercaptoethanol, pH 7.5 adjusted with 1 M Tris.
Incubate at +37 °C overnight.
Dialyze against 20 mM iodine acetamide + 50 mM K-phosphate.
Dialyze against 50 mM K-phosphate, pH 7.5 (4 x 2 h).
Add 12 U enzyme, digest overnight at +37 °C.
Troubleshooting
Modified Incubation Conditions
The enzyme is unstable in higher concentrations of both urea and guanidinium-HCl, but it is possible to use as substrate a glycoprotein which was denatured with urea.
A procedure to remove the urea is given in ′Protocols′.
DTT does not interfere, independently of the concentration.
Um weiterzulesen, melden Sie sich bitte an oder erstellen ein Konto.
Sie haben kein Konto?