Team:NTNU-Trondheim/Protocols
From 2013.igem.org
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12. To quantitate the vesicle yield in terms of mg vesicle protein/CFU, use a protein concentration determination assay to determine the total protein concentration in the vesicle preparation and divide the number by the CFU obtained from dilution plating of the culture at the time of harvest. In some cases, flagella and other non-vesicle proteins contaminate the preparation; however, further purification steps (e.g., using density gradient purification) prevent quantitative recovery. Therefore, vesicle yields often can be best compared using the quantity of vesicle-specific protein or lipid in the pelleted cell-free supernatant preparations. Here, an aliquot of the vesicle preparation is run on SDS-PAGE, stained for protein using Ruby or Coomassie, and either the total protein in each sample or the major outer membrane proteins (e.g., Omps F/C and A for E. coli ) in each sample are determined by densitometry. Subsequently, the densitometry value is divided by the CFU and this vesicle yield compared between strains or treatments. Finally, vesicle yield can also be determined based on lipid content using FM4-64, a lipophilic fluorescent dye. For FM4-64-based measurements, 20 μL vesicle preparation is diluted in 560 μ L of DPBSS, and 20 μL FM4-64 (1mg/mL) is added. Fluorescence (RFU) is measured with an excitation of 506 nm and emission of 750 nm using a spectro fluorometer. Subsequently, the RFU value is divided by the CFU and this vesicle yield value compared between strains or treatments. | 12. To quantitate the vesicle yield in terms of mg vesicle protein/CFU, use a protein concentration determination assay to determine the total protein concentration in the vesicle preparation and divide the number by the CFU obtained from dilution plating of the culture at the time of harvest. In some cases, flagella and other non-vesicle proteins contaminate the preparation; however, further purification steps (e.g., using density gradient purification) prevent quantitative recovery. Therefore, vesicle yields often can be best compared using the quantity of vesicle-specific protein or lipid in the pelleted cell-free supernatant preparations. Here, an aliquot of the vesicle preparation is run on SDS-PAGE, stained for protein using Ruby or Coomassie, and either the total protein in each sample or the major outer membrane proteins (e.g., Omps F/C and A for E. coli ) in each sample are determined by densitometry. Subsequently, the densitometry value is divided by the CFU and this vesicle yield compared between strains or treatments. Finally, vesicle yield can also be determined based on lipid content using FM4-64, a lipophilic fluorescent dye. For FM4-64-based measurements, 20 μL vesicle preparation is diluted in 560 μ L of DPBSS, and 20 μL FM4-64 (1mg/mL) is added. Fluorescence (RFU) is measured with an excitation of 506 nm and emission of 750 nm using a spectro fluorometer. Subsequently, the RFU value is divided by the CFU and this vesicle yield value compared between strains or treatments. | ||
- | == | + | == Recpies for buffers and growth media == |
+ | ====LB and LA medium==== | ||
+ | 1L dH<sub>2</sub>O | ||
+ | 10g Yeast extract | ||
+ | 5g NaCl | ||
+ | 5g Tryptone | ||
+ | |||
+ | To make LA media add 20g of agar powder. | ||
+ | Autoclave the media at 120°C for 20 minutes. | ||
+ | |||
+ | ====DPBSS (Dulbecco’s phosphate buffered saline supplemented with salt) buffer==== | ||
+ | |||
+ | 750 mL dH<sub>2</sub>O | ||
+ | 0.2g KCl | ||
+ | 0.2g KH<sub>2</sub>PO<sub>4</sub> | ||
+ | 11.7g NaCl | ||
+ | 1.15g Na<sub>2</sub>HPO<sub>4</sub> | ||
+ | 0.1 CaCl<sub>2</sub> | ||
+ | |||
+ | Add dH<sub>2</sub>O untill you have a total of 1L buffer | ||
+ | |||
+ | ====OptiPrep diluent buffer==== | ||
+ | 750 mL dH<sub>2</sub>O | ||
+ | 8.5g NaCl | ||
+ | 2.38 g Hepes | ||
+ | |||
+ | Bring the pH to 7.4 with NaOH. | ||
+ | Add dH<sub>2</sub>O to have in total 1L buffer. | ||
Revision as of 11:17, 23 July 2013