Team:NTNU Trondheim/Protocols

From 2011.igem.org

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(Protocols)
(Isolating plasmids:)
 
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==Resuspending DNA from registry-parts:==
==Resuspending DNA from registry-parts:==
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*Poke a hole in foil of corresponding well
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*Poke a hole in foil of corresponding well.
*Resuspend DNA in 10 µL dH2O (pipette up and down a few times)
*Resuspend DNA in 10 µL dH2O (pipette up and down a few times)
*Wait 5 minutes.
*Wait 5 minutes.
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*Transfer the resuspended DNA to pCR tube and store in -20C.
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*Transfer the resuspended DNA to a PCR tube and store in at -20°C.
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==Transforming competent cells:==
==Transforming competent cells:==
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*Mix with 2 µL plasmid DNA
*Mix with 2 µL plasmid DNA
*Incubate on ice 30 minutes
*Incubate on ice 30 minutes
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*Heat-shock cells 45 seconds in 42C water-bath.
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*Heat-shock cells 45 seconds in 42°C water-bath.
*Incubate 5 minutes on ice
*Incubate 5 minutes on ice
*Add 200 µL SOC
*Add 200 µL SOC
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*Incubate the Eppendorf tubes in Erlenmeyer flask 37C shaking incubator for 2 hours
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*Incubate the Eppendorf tubes in Erlenmeyer flask 37°C shaking incubator for 2 hours
*Plate 50 µl and 200 µl of the transformation onto the dishes, and spread.
*Plate 50 µl and 200 µl of the transformation onto the dishes, and spread.
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*Incubate ON in 37C
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*Incubate ON in 37°C
==Isolating plasmids:==
==Isolating plasmids:==
*Inoculate one colony in 3 mL LB with appropriate antibiotic. (IE 1,5µL amp stock in 3 mL LB)
*Inoculate one colony in 3 mL LB with appropriate antibiotic. (IE 1,5µL amp stock in 3 mL LB)
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*Grow in shaking incubator 30C ON
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*Grow in shaking incubator 30°C ON
*Isolate plasmid using [http://www.ebiotrade.com/buyf/productsf/Promega/tb225.pdf SV Miniprep procedure]
*Isolate plasmid using [http://www.ebiotrade.com/buyf/productsf/Promega/tb225.pdf SV Miniprep procedure]
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*Store in -20C
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*Store in -20°C
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==Gel Extraction:==
==Gel Extraction:==
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==Restriction Digest:==
==Restriction Digest:==
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*Add 500ng of DNA to be digested, and adjust with dH20 for a total volume of 42.5ul.
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*Add 500ng of DNA to be digested, and adjust with dH20 for a total volume of 42.5 µl.
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*Add 5ul of NEBuffer 2 to the tube.
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*Add 5µl of NEBuffer 2 to the tube.
*Add 0.5µl of BSA to the tube.
*Add 0.5µl of BSA to the tube.
*Add 1µl of your first enzyme.
*Add 1µl of your first enzyme.
*Add 1µl of your second enzyme.
*Add 1µl of your second enzyme.
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*There should be a total volume of 50ul. Mix well and spin down.
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*There should be a total volume of 50 µl. Mix well and spin down.
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*Incubate the restriction digest at 37C for 30min, and then 80C for 20min to heat kill the enzymes.
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*Incubate the restriction digest at 37°C for 30 min, and then 80°C for 20 min to heat kill the enzymes.
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==Ligation:==
==Ligation:==
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*Add 1ul of T4 DNA Ligase
*Add 1ul of T4 DNA Ligase
*Mix well, and spin down.
*Mix well, and spin down.
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*Incubate for 30min at 16C and 20min at 80C to heat kill.
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*Incubate for 30min at 16°C and 20min at 80°C to heat kill.
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*Use 2ul of ligation to transform into competent cells.
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*Use 2µl of ligation to transform into competent cells.
==Alternatively:==
==Alternatively:==
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* Repeat 2-4 34 times
* Repeat 2-4 34 times
* Final elongation: 72C 7 min
* Final elongation: 72C 7 min
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* Cooling: 4 C HOLD
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* Cooling: 4°C HOLD
==Testing of construct==
==Testing of construct==
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*Inoculate in 5 mL ON
*Inoculate in 5 mL ON
*Dillute 4 x 1:100 in LB, grow to OD 0,5
*Dillute 4 x 1:100 in LB, grow to OD 0,5
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*Pellet, resuspend 2x in 0,9% NaCl, 37C, 2x in LB
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*Pellet, resuspend 2x in 0,9% NaCl, 37°C, 2x in LB
*Grow 3 hrs?
*Grow 3 hrs?
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*Inoculate in 5 mL ON
*Inoculate in 5 mL ON
*Dillute 4 x 1:100 in LB, grow to OD 0,5
*Dillute 4 x 1:100 in LB, grow to OD 0,5
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*Pellet, resuspend 2x in no amino acid media, 37C, 2x in LB
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*Pellet, resuspend 2x in no amino acid media, 37°C, 2x in LB
*Grow 3 hrs?
*Grow 3 hrs?
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*Inoculate in 5 mL ON
*Inoculate in 5 mL ON
*Dillute 6 x 1:100 in LB, grow to OD 0,5
*Dillute 6 x 1:100 in LB, grow to OD 0,5
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*Pellet, resuspend in LB, Incubate 2 x 25C, 2 x 37C, 2x 40C ?
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*Pellet, resuspend in LB, Incubate 2 x 25°C, 2 x 37°C, 2x 40°C ?
*Grow 3 hrs?
*Grow 3 hrs?
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== TSS competent cells preparation: ==
 
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* Make TSS
 
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* Inoculate 5 ml LB (w/o antibiotic) from company stock stored in –80C and let grow o/n. 
 
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* Inoculate 30 ml LB (w/o antibiotic) with 300 μL from the o/n culture. (Alternative:  Inoculate 3 ml for 5 hrs and dump into 30ml culture.)
 
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* Monitor OD until it reaches 0.4-0.5. 
 
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* When OD reaches 0.4 remove from shaker and put on ice.
 
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* Pellet the cells in 50ml falcon (or autoclaved tube) tube at 6000g, 4C for 10 minutes.
 
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* Decant liquid and place cells back on ice.
 
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* Resuspend cells in 3.0ml TSS, pipet up and down and vortex. (resuspend in 10% original volume of TSS.  ie. 30ml culture, 3 ml TSS)
 
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* Pipet 250 μL cells into each prelabeled and precooled microfuge tube
 
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* Store at –80C
 
== Making blunt ends on DNA with sticky ends: ==
== Making blunt ends on DNA with sticky ends: ==
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* Digested DNA was cooled on ice, 2 µl 2 mM dNTP and 1 µl T4-DNA polymerase was added.
* Digested DNA was cooled on ice, 2 µl 2 mM dNTP and 1 µl T4-DNA polymerase was added.
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* The mix was incubated at 16 C for 12 min.
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* The mix was incubated at 16°C for 12 min.
* Inactivate enzyme and isolate fragment by using PCR purification kit.
* Inactivate enzyme and isolate fragment by using PCR purification kit.
= Recipes used in the lab =
= Recipes used in the lab =
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== LB Broth ==
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== LB medium ==
*Bacto-tryptone: 10 g/L
*Bacto-tryptone: 10 g/L
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* Filter through 0.22 μM syringe filter
* Filter through 0.22 μM syringe filter
* Autoclave centrifuge tubes, flasks and bottle/beaker for TSS
* Autoclave centrifuge tubes, flasks and bottle/beaker for TSS
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* Store at -20 C
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* Store at -20°C
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{{:Team:NTNU_Trondheim/NTNU_footer|}}
{{:Team:NTNU_Trondheim/NTNU_footer|}}

Latest revision as of 13:33, 21 September 2011



Protocols

Resuspending DNA from registry-parts:

  • Poke a hole in foil of corresponding well.
  • Resuspend DNA in 10 µL dH2O (pipette up and down a few times)
  • Wait 5 minutes.
  • Transfer the resuspended DNA to a PCR tube and store in at -20°C.

Transforming competent cells:

  • Thaw competent cells on ice
  • Mix with 2 µL plasmid DNA
  • Incubate on ice 30 minutes
  • Heat-shock cells 45 seconds in 42°C water-bath.
  • Incubate 5 minutes on ice
  • Add 200 µL SOC
  • Incubate the Eppendorf tubes in Erlenmeyer flask 37°C shaking incubator for 2 hours
  • Plate 50 µl and 200 µl of the transformation onto the dishes, and spread.
  • Incubate ON in 37°C


Isolating plasmids:

  • Inoculate one colony in 3 mL LB with appropriate antibiotic. (IE 1,5µL amp stock in 3 mL LB)
  • Grow in shaking incubator 30°C ON
  • Isolate plasmid using [http://www.ebiotrade.com/buyf/productsf/Promega/tb225.pdf SV Miniprep procedure]
  • Store in -20°C

Gel Extraction:

  • Using QIAquick Gel Extraction Kit [http://molecool.wustl.edu/krolllab/Kroll_Lab_Protocols/Molecular%20Biology%20protocols/Cloning%20protocols%20folder/Gel%20extraction-Qiagen.pdf protocol]
  • eluating with dH20


Restriction Digest:

  • Add 500ng of DNA to be digested, and adjust with dH20 for a total volume of 42.5 µl.
  • Add 5µl of NEBuffer 2 to the tube.
  • Add 0.5µl of BSA to the tube.
  • Add 1µl of your first enzyme.
  • Add 1µl of your second enzyme.
  • There should be a total volume of 50 µl. Mix well and spin down.
  • Incubate the restriction digest at 37°C for 30 min, and then 80°C for 20 min to heat kill the enzymes.

Ligation:

  • After digestion, separation, purification.
  • Add 11ul of dH20
  • Add 2ul from each sample you will be ligating (destination plasmid, and part)
  • Add 2ul of T4 DNA Ligase Reaction Buffer
  • Add 1ul of T4 DNA Ligase
  • Mix well, and spin down.
  • Incubate for 30min at 16°C and 20min at 80°C to heat kill.
  • Use 2µl of ligation to transform into competent cells.

Alternatively:

  • After gel extraction:
  • Add 1 µL T4 DNA Ligase Reaction Buffer
  • ca 6:1 molar ratio of insert to vector (~10ng vector)
  • Add (8.5 - vector and insert volume)μl
  • 0.5 μL T4 Ligase

PCR

PCR mix:

  • Work on ice
  • 0.5 µL DNA
  • 5 µL 10x PCR buffer 2 (w/MgCl2)
  • 0.5 µL 10 mM dNTPs
  • 1 µL fwd primer
  • 1 µL rev primer
  • 0.5 µL polymerase
  • 41.5 µL H20

PCR program:

  • Temperature of lid: 103°C
  • Heat cycles:
  • Initial denaturation: 94°C for 2 min
  • Denaturing: 94°C for 30 s
  • Annealing: 58°C for 30 s
  • Elongation: 72°C for 60 s
  • Repeat 2-4 34 times
  • Final elongation: 72C 7 min
  • Cooling: 4°C HOLD

Testing of construct

Test 1 Nullmedium:

  • Inoculate in 5 mL ON
  • Dillute 4 x 1:100 in LB, grow to OD 0,5
  • Pellet, resuspend 2x in 0,9% NaCl, 37°C, 2x in LB
  • Grow 3 hrs?


Test 2 Amino acid deprived:

  • Inoculate in 5 mL ON
  • Dillute 4 x 1:100 in LB, grow to OD 0,5
  • Pellet, resuspend 2x in no amino acid media, 37°C, 2x in LB
  • Grow 3 hrs?


Test 3 Temperature:

  • Inoculate in 5 mL ON
  • Dillute 6 x 1:100 in LB, grow to OD 0,5
  • Pellet, resuspend in LB, Incubate 2 x 25°C, 2 x 37°C, 2x 40°C ?
  • Grow 3 hrs?

Making blunt ends on DNA with sticky ends:

T4 DNA polymerase was used (Fills in 3' overhang and removes 5' overhang.

  • Digested DNA was cooled on ice, 2 µl 2 mM dNTP and 1 µl T4-DNA polymerase was added.
  • The mix was incubated at 16°C for 12 min.
  • Inactivate enzyme and isolate fragment by using PCR purification kit.

Recipes used in the lab

LB medium

  • Bacto-tryptone: 10 g/L
  • Yeast extract: 5 g/L
  • NaCl 5 g/L

Adjust pH to 7,4 with NaOH, autoclave.

LA

  • Dissolve LB
  • Add agar, 15 g/L

Adjust pH to 7,4 with NaOH, autoclave.

SOC:

  • Bacto-tryptone: 20 g/L
  • Yeast extract: 5 g/L
  • NaCl 0,5 g/L
  • 10 mL 250 mM KCl (25mM) → 0,186 g / 10mL H20
  • 5 mL 2M MgCl2 (10mM) → 0,952 g / 5mL

Autoclave, cool, then add:

  • 20 mL 1M sterile-filtered glucose (20mM)

Ampicillin-plates:

Use stock 200 mg/mL. → 100µg/mL in liquid agar. I.E. 250 µL stock in 500 mL agar. Add when cool enough to pour.

Spectinomycin-plates:

Use stock 100 mg/mL. → 100µg/mL in liquid agar. I.E. 500 µL stock in 500 mL agar. Add when cool enough to pour.

Ampicillin-IPTG plates:

Ampicillin 100 µg / mL (500 µL amp stock (200 mg/mL) in 500 mL agar) IPTG 0,1 mM ( 63,5 µL IPTG stock (0,8 M))

M9 minimal medium

Make M9 salts

  • To make M9 Salts aliquot 800ml H2O and add
    • 33.93g Na2HPO4 16,7 g
    • 15g KH2PO4 7,5g
    • 2.5g NaCl 1,25g
    • 5.0g NH4Cl 2,5g
    • Stir until dissolved
    • Adjust to 1000ml with distilled H2O
    • Sterilize by autoclaving
  • Measure ~700ml of distilled H2O (sterile)
  • Add 200ml of M9 salts
  • Add 2ml of 1M MgSO4 (sterile)
  • Add 20 ml of 20% glucose (or other carbon source)
  • Add 100ul of 1M CaCl2 (sterile)
  • Adjust to 1000ml with distilled H2O

Transfection Storage Solution (TSS)

50 ml TSS:

  • 10 % Polyethylene glycol 5 g
  • 5 % Dimethyl Sulfoxide (DMSO) 2,5 ml
  • 20 mM MgCl2 1 ml
  • Bring to 50 ml with autoclaved LB
  • Stir until dissolved
  • Filter through 0.22 μM syringe filter
  • Autoclave centrifuge tubes, flasks and bottle/beaker for TSS
  • Store at -20°C