Difference between revisions of "Team:ICT-Mumbai/Experiments"

Components of media

SpC Medium

Add the following to 10ml of TBase

• 100 ul of 50% glucose
• 150 ul of 1.2% MgSO4.3H2O solution
• 200 ul of 10% yeast extract
• 250 ul of 1% CAS amino acids

SpII medium

Add the following to 10ml of TBase

• 100 ul of 50% glucose
• 700 ul of 1.2% MgSO4.3H2O solution
• 100 ul of 10% yeast extract
• 100 ul of 1% CAS amino acids
• 50 ul of 0. 1M CaCl2

TBase

• Dissolve the following in 1L of water and autoclave
• (NH4)2SO4 - 2g
• K2HPO4.3H2O - 18.3g
• KH2PO4 - 6g
• Trisodium citrate.2H2O - 1g

Procedure

1. Streak a large patch of Bacillus subtilis cells onto an LB agar plate (2.5% LB and 1% agar)
2. Incubate at 37 deg C overnight
3. Scrape cell’s off the patch into 10 ml of freshly made SpC medium (for contents of SpC medium see below) till OD of tube becomes approximately 0.5
4. Incubate at 37 deg C and 220 rpm for 5 hours
5. Inoculate 200ul of this culture into 10 ml of freshly prepared SpII medium (for contents of SpII medium see below)
6. Incubate at 37 deg C and 170 rpm for 90 min
7. Pellet cells in 1.5 ml microcentrifuge tubes. Decent and store supernatant
8. Resuspend pellets in 200ul of supernatant
9. Add 15ul of plasmid (pBS1C backbone)
10. Incubate at 37 deg C
11. Plate on LB agar plates (2.5% LB and 1% agar) containing chloramphenicol (25 ug/ml)
12. Incubate overnight at 37 deg C to grow colonies

GeneAll ExprepTM plasmid SV mini protocol used. Link provided below for the same:
GeneAll Prep

GeneAll ExpinTM protocol used. Link provided below for the same:
https://www.cambio.co.uk/library/images/html_images/GeneAll/2013_Expin_protocol_web.pdf

Procedure

1. Seeds of 4 crops were obtained as specimen.
   1. Rice
   2. Soybean
   3. Tomato
   4. Wheat
2. The seeds were sterilised by rinsing them with Ethanol a few times.
3. Common garden soil was collected, and sterilised in autoclave to avoid any outside contamination while collection of exudates.
4. Glass jars were filled upto quarter the volume with sterilised soil.
5. Sterilised seeds were sown in the jars, (4 jars per crop) and the crops were grown in clean room for 3 weeks.
6. When the height of crops was sufficient after 3 weeks, the crops were uprooted carefully and soil was mixed with GC (Gas Chromatography) grade water.
7. After incubating the mixture for 30 minutes, to allow all the exudates to be dissolved in water, the solution was filtered.
8. Filtered solution was evaporated in RotaVap. Vacuum was maintained to allow the evaporation at lower temperature as some of the exudates might be temperature sensitive.

1. Inoculate DH5 alpha cells - 10 ul from the glycerol stock into LB medium (2.5%).
2. Incubate overnight at 37 deg C.
3. Next day, subculture thi culture into fresh tubes containing 10ml LB medium (2.5%) each -100 ul of the overnight culture added to the LB media.
4. Incubate at 37 deg. C for approximately 2-3 hrs till you get an OD of around 0.6
5. Place these LB tubes and 0.1 M CaCl2 on ice (all further steps to be carried out on ice in a LAF)
6. Distribute each tube containing 10 ml culture into two / four microcentrifuge tubes.
7. Centrifuge the tubes and discard the supernatant. Ensure complete removal of the supernatant.
8. Resuspend pellets in 1 mL of 0.1M CaCl2.
9. Keep them in the ice for half an hour.
10. Now centrifuge the tubes again and discard the supernatant.
11. Resuspend pellets in 200 ul of 0.1 M CaCl2.
12. Once suspended add 40 ul of the glycerol.
13. Distribute this 240 ul of solution in each microcentrifuge tube into two microcentrifuge tubes with 120 ul in each.
14. Now store these cells in the -80 deg C.