kholdsnare Posted December 4, 2011 Posted December 4, 2011 Detailed answers would be appreciated: 1) What is the difference, in terms of data obtained, between Coomassie Blue staining and Western blotting. 2) What kind of important information can be obtained from purifying a protein from the native species itself? 3) Why is it not a good idea to use too much of template DNA for a PCR reaction? Any help would be appreciated, thank you
kholdsnare Posted December 4, 2011 Author Posted December 4, 2011 no its for a research presentation that i need to give
shaung Posted December 5, 2011 Posted December 5, 2011 not goin to answer for you, but: 1. what do you use to help visualise the proteins on a western and isnt used on a coomassie? I.e. what does your secondary antibody bind to in a western? why can you see so many bands in a whole cell lysate coomassie? 2. talk about native protein structure, binding partners, etc. 3. say you have a ball pit full of yellow balls (being your DNA template) and 1 green ball (being your primers) in a room with no gravity, how easy would it be for the green ball to move between the yellow balls to find their specific binding sites. hope this helps!
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