Difference between revisions of "User:Mary Mendoza/Notebook/CHEM572 Exp. Biological Chemistry II/2013/04/09"

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==Objective==
 
* Using solutions made last week, a run of 40 μM adenosine with 25 μM varying inhibitors were conducted using the UV 2500 Shimadzu spectrophotometer.
 
* Three runs of each inhibitor were taken; the average of the runs were taken. The standard deviation were calculated and added as error bars.
 
* Produce histogram
 
  
==Protocol==
 
  
* The reagents were added in the following sequence:
 
** 1.78 mL of phosphate buffer
 
** 600 μL of 200 μM adenosine (final concentration 50 μM)
 
* This was allowed to mix through venting and placed on  the chamber for absorbance reading.
 
** 300 μL of phosphate buffer (or inhibitor dissolved in phosphate buffer)
 
** 300 μL of dimethyl sulfoxide (DMSO) (or inhibitor dissolved in DMSO)
 
* The cuvette contents were mixed by venting and placed on the chamber for absorbance reading.
 
** 20 μL of adenosine deaminase (ADA) was added to catalyze the reaction
 
* The kinetics of the reaction was taken using the UVProbe software.
 
  
==Description==
 
*Cuvette Mixture with Inhibitor
 
[[Image:InhibitorCuvetteTable.png]]
 
  
*Cuvette Mixture no Inhibitor
 
[[Image:CuvetteMixtureNoInhibitor.png]]
 
  
*Inhibitors Ran today:
 
#Aspirin
 
#Kaempferol
 
  
==Data==
 
* [[Image:409HistogramTable.png]]
 
  
* [[Image:409AverageVelocityHisto.png]]
 
  
* [[Image:409PercentChangeHisto.png]]
 
  
==Notes==
 
*Solution Preparation/Calculations: Catherine Koenigsknecht
 
*Cuvette preparation: Mary Mendoza
 
*Data Evaluation: Dhea Patel
 
*Overall Lab Assistance: Mike Nagle
 
  
 
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Latest revision as of 21:37, 26 September 2017

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