User:Khyra A. Neal/Notebook/Chem 571/2014/10/14: Difference between revisions

October 14, 2014

Tasklist

1. SDS Page #2

• Mix 10 μL 0.6 g/L lysozyme with 10μL SDS-PAGE sample buffer in 1.5 mL centrifuge vial
• Mix 10 μL 0.12 g/L lysozyme with 10μL SDS-PAGE sample buffer in 1.5 mL centrifuge vial
• Mix 10 μL 30:1 Au/lysozyme colloid with 10μL SDS-PAGE sample buffer in 1.5 mL centrifuge vial
• Mix 10 μL 0.12 g/L unknown protein with 10 μL SDS-PAGE sample buffer in 1.5 mL centrifuge vial
• Place in heating block (set at 90 °C) for 5 minutes
• Store in refrigerator overnight

2. Bradford Analysis

• Analysis of Solutions that were extracted from wells that set for one week on October 8, 2014
  • Remove 20 μL of solution from each chamber (10 in all) and run Bradford analysis
  • Bradford reagent should be diluted 1:3 with 50mM Tris/50mM NaCl
  • Dilute to 1 mL by adding 780 μL stock 50 mM Tris/NaCl
  • Measure UV-Vis from 400 nm - 800 nm using polystyrene cuvettes.
  • Run blank of Tris/NaCl buffer
  • Run UV-Vis of undialyzed 0.6 g/L Lysozyme solution with Bradford reagent

3. Calibration Curve for undialyzed Lysozyme by Bradford Analysis

• 0.12 g/L, 0.3 g/L, 0.5 g/L, 0.6 g/L and 1 g/L Lysozyme
• 20 μL of Lysozyme
• Bradford reagent should be diluted 1:3 with 50mM Tris/50mM NaCl
• Dilute to 1 mL by adding 780 μL stock 50 mM Tris/NaCl
• Measure UV-Vis from 400 nm - 800 nm using polystyrene cuvettes.

4. Prepare 50 mL 66 mM Potassium Phosphate Buffer

• 0.361 g of monobasic potassium phosphate
• 0.105 g of dibasic potassium phosphate
• Add to 50 mL volumetric flask and dilute with HPLC water
• Final pH is 6.319

5. Fluorescence on protein containing solutions that were dialyzed on October 8, 2014

• Dilute Lysozyme sample 100x for each well.
• Transfer 100 μL to a small volume fluorescence cuvette
• Run fluorescence from 300 nm -550 nm and excitation at 280 nm

6. UV-Vis

• Run Uv-Vis on protein containing solutions that were dialyzed on October 8, 2014
• Run from 200 nm -400 nm