How does one functionalize a protein?
How do you know what beads to use? What is the significance to the different tags?
How do you know what beads to use? or columns? or anything else?
Does it matter what pool we use?
What is a good starting amount of pmol?
Do we need to start a new notebook, or can we use the old one?
Is the buffer they mention on the data sheet the one we should use?
*Reminder for Brad: Please send terrible binding assay results to Michael and I! :)
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