Notes+about+too+much+lysozyme+during+plate+production

I originally had a problem seeing too strong of a lysozyme band on my Western blots. The problem was that I made a mistake calculating how much lysozyme to use when I scaled down from the flask to the plate. Originally I calculated the amount of lysozyme to scale down to based on the resuspension volume rather than based on the original culture volume. A more detailed explanation can be found on 6-16-11 of notebook. Western blot data can be found in the 6-6-11 folder as well as the 9-14-11 presentation.