Team:Carnegie Mellon/Met-Protocols
From 2012.igem.org
Protocols
Overview
Kit Protocols
1. | Z-Competent E. Coli Transformation Kit for making competent cells for easy transformation. Modified to incubate cells on ice for 1 hour during transformation |
2. | Phusion High Fidelity PCR Kit for amplifying our inserts and cassettes. |
3. | Wash 1mL induced cells once with PBS and resuspend in 1mL M9 media. |
4. | Add 1µL of 50nM Mg2+ to the tubes (from MgCl2 from PCR kit) |
5. | Aliquot (100ul/200ul) of cells into desired wells of a 96-well plate. |
6. | Add various doses of DFHBI to the wells, followed by adding the desired doses of MG |
7. | Plate read with plate reader (Tecan Safire II). First find cell density using OD600. Then use Excitation/Emission of 469/501 for Spinach and 635/660 for Malachite-green. |
Dosage Curve
1. | First culture a fresh batch of cells using 1:100 of overnight culture of promoter construct. Culture for around 2 hours or until the solution is lightly turbid. |
2. | Induce cells by adding 1ul of 1mM IPTG. |
3. | Wash 1mL induced cells once with PBS and resuspend in 1mL M9 media. |
4. | Add 1µL of 50nM Mg2+ to the tubes (from MgCl2 from PCR kit) |
5. | Aliquot (100ul/200ul) of cells into desired wells of a 96-well plate. |
6. | Add various doses of DFHBI to the wells, followed by adding the desired doses of MG |
7. | Plate read with plate reader (Tecan Safire II). First find cell density using OD600. Then use Excitation/Emission of 469/501 for Spinach and 635/660 for Malachite-green. |
Cloning Protocol
1. | Start digestion of vector and insert DNA using desired restriction enzyme manufacturer protocol. |
2. | After 2 hours, add Phosphatase [CIP] to insert to prevent self-ligation |
3. | Purify and clean DNA using kit. [Zymo Research] |
4. | Measure vector/insert concentration. [Nanodrop] |
5. | Divide the concentration by the length of the sequence and calculate ligation ratios of 1 vector to 3 insert. Mix the ratios according to the calculations, including T4 buffer and ligase. |
6. | Leave ligation products at room temperature for 1 hour. |
7. | Transform ligation products into competent cells using appropriate protocol. Incubate on ice for 1 hour if using Zymo competent cells |
8. | Plate cells and incubate at 37 degrees overnight. Check for colonies the next day |