Difference between revisions of "Team:NU Kazakhstan/Notebook"
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<li>Freeze in -80°C</li></ol> | <li>Freeze in -80°C</li></ol> | ||
− | + | <h3>6.06.15</h3> | |
− | + | <p><ol><li>PCR clean-up of:<br> | |
− | + | -[FixK2+rbs] = 30.15 ng/µl<br> | |
− | + | -[tetR] = 57.47 ng/</li> | |
− | + | <li>Gel extraction after digestion:<br> | |
− | 6.06.15 | + | -[FixK2 + rbs] = 5.862 ng/µl<br> |
− | + | -[tetR] = 4.621 ng/µl</li> | |
− | PCR clean-up of | + | <li> |
− | [tetR] = 57.47 ng/ | + | Ligation with Fermentas enzymes<br> |
− | + | -[tetR] = 20/4.621ng/µl = 4.3 µl<br> | |
− | [FixK2 + rbs] | + | -[FixK2+ rbs] = 40ng/5.862 ng/µl = 7 µl</li> |
− | [tetR] = 4.621 ng/µl | + | <li>Ligation of:<br> |
− | + | -Pveg + FixJ<br> | |
− | Fermentas | + | -FixK+ rbs+tetR<br> |
− | [tetR] = 20/4.621ng/µl = 4.3 µl | + | -TetR+double terminator</li></ol></p> |
− | [FixK2+ rbs] = 40ng/5.862 ng/µl = 7 µl | + | |
− | + | ||
− | + | ||
− | + | ||
− | + | ||
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Revision as of 16:27, 12 September 2015
Notebook
1.06.15
- Preparation of the LB agar
We used 37 g of nutrient agar for 400 mL of distilled water - Extraction of genome from S.mutans
- First, culture S.mutans in 5 mL liquid BHI + bacitracin
- Centrifuge for 15 min at 4000 rpm
- Then dissolve the pellet in 500 microliters of Lysis Buffer
How to prepare Lysis Buffer (1 mL):
Lysis Buffer contains EDTA, Tween 80%, tris HCl,125 microliters of 8 M EDTA,5 µl of Tween 80, Tris HCl 1M 50 µl, Proteinase K (200 µg/mL). 0.0002 grams of powder Proteinase K were put into 1 mL of Lysis Buffer. The balance could not read 0.0002 g of proteinase K, so 0.02 g of proteinase K were taken.
- Incubation for 2 hours at 55°C. Heat at 90°C for 5 minutes.
- Then add equal volume of cold isopropyl alcohol.
- Incubate in freezer for 20 minutes.
- Centrifuge at the maximum speed for 30 min. Remove the supernatant.
- Add enough amount of ethanol to the pellet in order to wash
- Then add 50 µl of TE buffer
- Add 0.5 µl of the RNAase
- Incubate at 37°C for 1 hour
- Inactivate at 60°C for 10 min
- Run it in an agarose gel
- Construction of the light system
pFixK2(K592006) + rbs + tetR(C0040) + double terminator + Ptet(R0040) + rbs + RFP(J06505) + double terminator- [rbs] = 139.15 ng/µl
- [Ptet + GFP] = 199.2 ng/µl
- [pFixK2] = 131.6 ng/µl
- [double terminator] = 70.21 ng/µl
- [tetR] = 78.76 ng/µl
- Restriction digests:
Protocol for Restriction digest:
Take following amounts of reagents:
-1000 ng of DNA
-0.5 µl of each Restriction Enzyme(we used NEB enzymes)
-5 µl of CutSmart Buffer
-dH2O to get final volume of 50 µl
Incubate this mixture at 37 C for 1-2 hours and heat inactivate for 20 min at the temperature needed for particular enzyme.
Example mixture:
-pFixK2 (250 bp) was cut with EcoRI and SpeI.- pFixK2 – 7.6 µl
- EcoRI = 0.5 µl
- SpeI = 0.5 µl
- dH2O = 36.4 µl
- cut smart = 5 µl
- Overall: 50 µl
-RBS (15 bp) was cut with .
-TetR (685 bp) was cut with EcoRI and SpeI.
-Double terminator (95 bp) was cut with XbaI.
- Gel extraction of the pFixK2, RBS, tetR and double terminator
- Invitrogen by Life Technologies PureLink Quick Gel Extraction Kit was used to purify DNA.
- The small area of the gel containing the DNA fragment of interest was cut under UV.
- Mass of FixK2 = 220 mg, RBS = 80 mg, tetR = 150 mg, dTer = 140 mg
- The protocol of the PureLink Quick Gel Extraction was used to dissolve the gel and extract the DNA
- [FixK2] = 5.727 ng/µl
- [Rbs] = 4.499 ng/µl
- [tetR] = 5.216 ng/µl
- [double terminator] = 2.694 ng/µl
- Ligation of the Parts:
Protocol for Ligation:
-Take 50 ng of vector or just of bigger DNA part
-Take amount of smaller DNA part to have 1:3 molar ratio
-1 µl of T4 ligase enzyme
-2 µl of T4 buffer
-Add dH2O to have final volume of 20 µl
Incubate this mixture for 16 hours at 16 C and heat inactivate for 10 min at 65 C.
Example Ligation mixture:
-Ligation of pFixK2 + rbs- pFixK2 = 8.5 µl
- RBS = 8.5 µl
- T4 ligase = 1 µl
- T4 buffer = 2 µl
- Overall: 20 µl
-Ligation of TetR + double terminator
When ligated DNA was transformed, the plate with pFixK2 + RBS had colonies grown. The mini-prep of pFixK2 + rbs was done - The concentrations of the transformed parts:
- FixK2+ rbs= 75.79 ng/µl
- FixK2+ rbs= = 72.80 ng/µl
- TetR + dter= 56. 93 ng/µl
- TetR + dter= 95.86ng/µl
- Pveg= 84.84 ng/µl
- FixJ= 161.1 ng/µl
- PCR (Thermo Scientific Phusion High Fidelity PCR Master-mix):
Protocol for PCR reaction:
Take following reagents:
-10 ng of DNA
-10 µl of PCR MasterMix
-2 µl of each 5 µM Primer
-Add dH2O to get final volume of 20 µl
Example PCR mixture:
-PCR of FixK2- DNA = 0.03 µl *10 reactions = 0.3 µl
- Water = 5.97 µl= 59.7 µl
- Master Mix = 10 µl= 100 µl
- VF2 = 2µl = 20 µl
- VR= 2 µl = 20 µl
-
-PCR of RBS
-PCR of FixK2 + rbs
-PCR of tetR+dter
-PCR of tetR
-PCR of Double terminator
Result:
-The ligation of the FixK2+ rbs did not work
-The ligation of the tetR+ dter worked - Restriction Digests of:
-tetR
-Double terminator - PCR of the ligated parts after transformation and mini-prep:
-PCR of [FixK2+rbs+tetR] = 108.54 ng/µl
-PCR of [tetR+ double terminator] = 166 ng/µl - Running of PCR products on a gel in the following order:
- Ladder
- FixK2+ RBS
- FixK2+ rbs+tetR
- TetR
- tetR+ dter
- Inoculate a single colony into 5 mL LB in 50 mL falcon tube (taped on a loosed tap)
- Grow on 37°C with shaking for 130 rpm overnight
- Use 1 mL to inoculate 100 mL to inoculate 100 mL of LB in 250 mL bottle the next morning
- Shake 37°C for 1.5-3 hours
- When OD is between 0.3-0.4 put cell on ICE
- Hold cells on ice for the 10 minutes
- Collect cells by centrifugation for 3 min at maximum speed (4700 rpm)
- Decant supernatant and gently resuspend on 10 mL ice-cold 0.1 M CaCl2 (prepared in ddH2O). Treat them gently.
- Incubate on ice for 20 minutes.
- Centrifuge again at maximum speed (4700 rpm)
- Discard supernatant and gently resuspend in 5 mL cold 0.1 M CaCl2 (15% glycerol)
- Dispence into chilled microtubes, put on the dry ice. Perform this procedure very quickly!
- Freeze in -80°C
- PCR clean-up of:
-[FixK2+rbs] = 30.15 ng/µl
-[tetR] = 57.47 ng/ - Gel extraction after digestion:
-[FixK2 + rbs] = 5.862 ng/µl
-[tetR] = 4.621 ng/µl -
Ligation with Fermentas enzymes
-[tetR] = 20/4.621ng/µl = 4.3 µl
-[FixK2+ rbs] = 40ng/5.862 ng/µl = 7 µl - Ligation of:
-Pveg + FixJ
-FixK+ rbs+tetR
-TetR+double terminator
3.06.15
4.06.15
5.06.15
Protocol for making the competent dh5alpha
6.06.15