User:Melissa Novy/Notebook/CHEM-571/2012/09/25
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< User:Melissa Novy | Notebook | CHEM-571 | 2012 | 09(Difference between revisions)
(→Horseradish Peroxidase Stock Solution in H2O) |
Current revision (11:18, 9 October 2012) (view source) (→Horseradish Peroxidase Chemiluminescence Assay) |
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==Objectives== | ==Objectives== | ||
* Remake 2.5 mM luminol stock solution and 2.3 μL HRP solution to continue HRP chemiluminescence assay. | * Remake 2.5 mM luminol stock solution and 2.3 μL HRP solution to continue HRP chemiluminescence assay. | ||
| - | * Make starter culture media and expression culture media to use with <i>E. coli</i> cells expressing adenosine deaminase enzyme. | + | * Make four sets of 1 L each of starter culture media and four sets of 1 L each of expression culture media to use with <i>E. coli</i> cells expressing adenosine deaminase enzyme. |
** No alterations were made to the [[AU_Biomaterials_Design_Lab:Protocols/Starter_Culture_Media|starter culture media protocol]] or the [[AU_Biomaterials_Design_Lab:Protocols/Expression_Culture_Media|expression culture media protocol]]. | ** No alterations were made to the [[AU_Biomaterials_Design_Lab:Protocols/Starter_Culture_Media|starter culture media protocol]] or the [[AU_Biomaterials_Design_Lab:Protocols/Expression_Culture_Media|expression culture media protocol]]. | ||
| - | ** The media were then autoclaved according to the [[AU_Biomaterials_Design_Lab:Protocols/Autoclave|procedure]]. | + | ** The media were then autoclaved according to the [[AU_Biomaterials_Design_Lab:Protocols/Autoclave|procedure]]. Please refer to [[User:Dhea_Patel/Notebook/Experimental_Biological_Chemistry_Notebook/2012/09/25|Dhea Patel's entry]] for modifications to the autoclaving procedure. |
** Please refer to [[User:Keyun_Wang/Notebook/Experimental_Biological_Chemistry_I/2012/09/25|Keyun Wang's entry]] for actual masses and volumes used to make the media. | ** Please refer to [[User:Keyun_Wang/Notebook/Experimental_Biological_Chemistry_I/2012/09/25|Keyun Wang's entry]] for actual masses and volumes used to make the media. | ||
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==Luminol Stock Solution in H<sub>2</sub>O and Carbonate Buffer== | ==Luminol Stock Solution in H<sub>2</sub>O and Carbonate Buffer== | ||
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[[Image:HRP_Assay_2012-09-25.png]] | [[Image:HRP_Assay_2012-09-25.png]] | ||
* Graph of intensity versus time of <i>p</i>-iodophenol-enhanced solutions of luminol, H<sub>2</sub>O<sub>2</sub>, and horseradish peroxidase. | * Graph of intensity versus time of <i>p</i>-iodophenol-enhanced solutions of luminol, H<sub>2</sub>O<sub>2</sub>, and horseradish peroxidase. | ||
| - | * Please refer to the above table for initial concentrations of the components. Final concentrations will be calculated in the future. | + | * Please refer to the above table for initial concentrations of the components. Final concentrations of the components in the ~2 mL final volume of the reaction solution will be calculated in the future. |
* Based on the shape of the curves, it appears that the reaction is proceeding too quickly upon the addition of HRP, such that the slope is too steep. It is recommended that the concentration of HRP be decreased, while the concentration of luminol to H<sub>2</sub>O<sub>2</sub> optimized. | * Based on the shape of the curves, it appears that the reaction is proceeding too quickly upon the addition of HRP, such that the slope is too steep. It is recommended that the concentration of HRP be decreased, while the concentration of luminol to H<sub>2</sub>O<sub>2</sub> optimized. | ||
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Objectives
Luminol Stock Solution in H2O and Carbonate Buffer
Horseradish Peroxidase Stock Solution in H2O
Horseradish Peroxidase Chemiluminescence Assay
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