Team:ETH Zurich/Materials

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Preparation of stock solutions

Making LB media

Dissolve 12.5g of LuriaBroth in 500mL MilliQ H2O and autoclave

Making LB-Agar

Dissolve 12.5g LuriaBroth in 500mL MIlliQ H2O,add 7.5g Agar.
Before use: Heat it inb the microwave and let it cool down to 50 degree celsius before adding Antibiotics.

Antibiotics stock solutions

Ampicillin (amp): 100mg/mL (1000X)
Dissolve 1g Ampicillin in 10mL sterile H2O.Aliquot and store at -20 degree celsius.

Kanamycin (Kan): 50mg/mL (1000X)
Dissolve 0.5g Kanamycin in 10mL sterile H2O.Aliquot and store at -20 degree celsius.

Chloramphenicol(cam): 34mg/mL (1000X)
Dissolve 0.34g Chloramphenicol in 10mL sterile H2O. Aliquot and store at -20 degree celsius.

All stock solutions have to be diluted 1:1000 times when used for Cultures/Plates

Glycerol 20%

Mix 20mL of Glycerole 100% and 80mL of MilliQ H2O, autoclave

General cloning procedure

Minipreps

Sigma Aldricht Miniprep kit : Elute in 50uL for higher plasmid concentrations.

Restriction enzyme digest

50uL reaction Volume:
2ug of plasmid (max 45uL for low concentration minipreps)
5uL NEB buffer (which buffer for which enzzyme can be looked up on the NEB website)
add ddH2O up to 50uL
0.5/1uL of restriction enzyme (20000U/mL/10000U/mL)
Keep enzymes always on cooling block and don't take them out for too long.
Mix through pipetting

1h at 37 degree celsius
Heat inactivation : 20min at 65 degree celsius(not always necessary)

Dephosphorylation of backbones only (reduces plasmid slef ligation)
Add 1uL of Calf-intestine-phosphatase)
1h at 37 degree celsius
20 minutes heatinactivation at 65 degree celsius.

Add 10uL of loading buffer (6X)
Analysis on gel

Figure 1. iGEM suffix insertion
Figure 2. iGEM 3A Assembly


Ligation

100ng of backbone and corresponding amount of insert depending on size
Always do a negative control without insert
Add up to 10/15uL with ddH2O
1.1/1.65uL T4 ligation buffer
1uL Ligase
1h at room temperature
20 min at 65 degree celsius

Gel extraction

Sigma Aldricht Gel extraction kit

Transformation

Thaw competent cells on ice for 10 minutes
5uL of ligation product or 1uL of resuspended plasmid/miniprep in 50uL competent cells
30min on ice
1 min heat shock at 42 degree celsius
3 minutes on ice
add 900uL LB
1h shaking at 37 degree celsius
Centrifuge at 12000rcf
remove 750uL supernatant
resuspend the pellet in the remaining 200uL LB
Plate on pre warmed plates

Sequencing

1200ng of DNA
3uL sequencing primer (10uL)
send out for sequencing using Microsynth account
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PCR (for gene amplification or colony PCR)

PCR was used for gene amplification for cloning and for colony PCR for the clone sleection. For colony PCR TAg Polymerase was used whereas for the gene amplification due too higher needs in accuracy Phusion Polymerase was used. FOr gene Amplification PCR the reaction volume is 50uL and for colony PCR 20uL. 1-20ng of the template plasmids were used for the amplification. For the coplony PCR in some cases NEB QuickLoad 2X Taq master mix was used.

Gene Amplification PCR (50uL reaction volume) Colony PCR (20uL reaction volume
Volume uL Volume uL Volume uL
PCR Buffer 5X/10X 10 2 -
dNTP 10uM 1 0.5 -
Rev and fwd primer 10uM 1 0.75 0.75
Polymerase 2U/uL 0.5 0.5 -
Template DNA + H2O 36.5 15.5 10
QuickLoad 2X Taq - - 10


Experimental procedures

Two layer agar plate experiment

First layer of 1.5% LB-Agar
Second layer consists of 0.7% LB-agar
Receiver cells are dissolevd in 0.7% Agr and then added on top of the first layer
Grow receiver cultures to OD600 of 0.3, dilute into 2mL of 0.7% Agar