Guest biomante Posted March 31, 2005 Posted March 31, 2005 Hi I was wondering if someone knows any good electronic resource (or book) about enzyme kinetics, specially trouble-shooting. I know it is simple, but I am stuck just trying to measure the concentration of a substrate I am working with using a coupled enzyme assay. It is supposed to be very straightforward, but I am getting pretty weird results. Any help would be really appreciated.
ecoli Posted April 1, 2005 Posted April 1, 2005 here you go...http://users.rcn.com/jkimball.ma.ultranet/BiologyPages/E/EnzymeKinetics.html http://www.chem.qmul.ac.uk/iubmb/kinetics/ let us know how it works out!
Guest biomante Posted April 1, 2005 Posted April 1, 2005 Thanks, I will check the link. The weird results are that I am getting (according to my calculations), extremely low substrate concentrations (silly low). Probably I am messing up the units.
Guest biomante Posted April 5, 2005 Posted April 5, 2005 OK This thing is still not working, and I am kind of running out of time (and patience). The thing is this, I am using a coupled enzyme assay to measure the concentration of a substrate; the reaction of the first enzyme can't be followed but the second one uses NADH, so the depletion of it can be followed with a spectrophotometer. So I just measure the absorbance (340nm) before adding enzyme (the first in the reaction) and sometime after adding it (I do it after 5 minutes), when I don't see any change in absorbance, right? To get the concentration I use this formula: (ΔA/6220)x(1000/V) = mM ΔA = change in absorbance 6220 is the extinction coefficient of NADH V= volume of substrate solution used in the 1 ml cuvette So, I should get the mM concentration of the substrate right? Well, I am still getting a very low concentration, so low I don't even think I would see any measurable enzyme activity, so it must be wrong. If there is anyone out there that can help me with this, I would appreciate it. Thanks
Skye Posted April 6, 2005 Posted April 6, 2005 This does the calculation for you. The pathlength of a normal cuvette is 1 cm. http://www.changbioscience.com/calculator/BeerLambert.html You will often get low concentrations. Remember that you are using tiny amounts of enzyme, and a mole is a huge number.
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