NOTEBOOK.

I should probably put some Table of Contents up here, so one could easily skip from day to day... at any rate, here's the current info dump.

Heads-up: I know there aren't circles on the list. This is apparently harder to do than I had envisioned?

6/13/16

(HC) Made LB-Amp plates

450ml of DI water
5.0g tryptone
2.5g yeast
5.0g NaCl
7.5g Agar

This was then adjusted to a pH of 7.0 using NaOH. It was then autoclaved. 2.5mL of 10mg/mL of Amp for a final concentration of 50 μg/mL was achieved.

6/14/16

(HC) made CSM -His plates

6/15/16

(XX) Goal: Run a gel to check whether pSB416 GPD has PstI site removed (diagnostic gel)

1. pSB416 GPD cut wit AvaI
2. pSB416 GPD cut with PstI
3. p146GPD cut with AvaI
4. p416GPD cut with PstI

Major steps:

Digest:

6 sterile water, 1 CutSmart buffer, 2 DNA, 1 enzyme (AvaI or PstI-HF)

Gel Order: L, 1, 3, 2, 4

Expected results on this diagnostic gel:

1. No cut because no AvaI site in pSB416 GPD
2. Should only see one cut because only one PstI site
3. Should see one cut
4. Should see two bands

Experimental results:

Gel results are not good; need to rerun this diagnostic gel

Other Activities:

Created mRPS12+/KanMZ- (parent) and mRPS12-/KanMX+ (mutant) master plate on YPD
Replica plating YPG (Should this be YPD???) , YPG, -His, -Ura, -Ura+Glycerol, YPD+Paro, YPG+Paro

6/16/16

(HC) Ran a boiling and spin prep on P413 GPD

Boiling Prep Procedure:

1) Pellet cells from 1.5mL of an overnight L-Amp culture of transformed E. coli cells in a microcentrifuge for 20-30 seconds and remove supernatant.
2) Use a toothpick and vortexer to resuspend the cells in 100 μl(0.1mL) of STET buffer(8% sucrose; 5%Triton X-100;50 mM EDTA; Tris-Cl, pH 8.0) containing 1mg/mL lysozyme(prepare 1 mg/mLenzyme in STET just prior to use; 1mL= 10 preps).
3)Place the suspension in a boiling water bath for 90 seconds.
4) Spin in a microcentrifuge for 15 min at the highest speed.
5)Remove the pellet (a gelatinous mass of cell debris) with a toothpick and discard.
6) Precipitate nucleic acid at -20℃ for 30 minutes using an equal volume of isopropanol.
7) Spin the tube in a microcentrifuge for 10 minutes at RTo to pellet the nucleic acids.
8) Was pellet twice with 70% ethanol and dry thoroughly.
9) Resuspend the pellet in 50 μL of sterile DI water or TE buffer.

Spin Prep: We used the QIAprep Spin Miniprep Kit to run a spin prep and followed the instructions inside.

(XX)Goal: Rerun the diagnostic gel stated yesterday (6/15/16)

Experimental results:

Good gel results, confirming that the PstI site has been removed in pSB416 GPD. pSB416 ready to be sequenced.

Other activities:

Incubated pSBIC3 mRPS12 TU and pSBIC3 mRPS12 mls (from last year iGEM team??) in LB-chloramphenicol broth @37C overnight at 250 rpm

6/17/16

(HC) Ran two digests for P413 GPD

Analytical Digest:
5 μL of DNA(Boiling Prep)
1μL of PstI HF
1μL of CutSmart buffer
3μL of sterile DI water
Preparative Digest:
7μL of DNA(Spin Prep)
1μL of NheI
1μL of NsiI
1μL of CutSmart buffer

Gel Results:

PREP GEL
Lane 1: Ladder
Lane 3: Preparative Digest
INSERT NOTEBOOK PICTURE #001 HERE
ANALYTICAL GEL

Lane 1: Ladder
Lane 2: Uncut (2μL of DNA and 8μL of water)
Lane 3: Analytical Digest

INSERT NOTEBOOK PICTURE #002 HERE

(XX) Master plate results:

Nothing grew on control plates (-His, -Ura, -Ura+Glycerol)
Both parent and mutant grew on YPD and YPD+Paro, indicating that Paro has no effect on yeast growth
Mutant cannot grow on YPG or YPG+Paro because of the mRPS12 gene knockout

Other Activities:

Cut p413GPD with NheI and NsiI to get rid of the illegal PstI site
Massive gel to run boiling preps

Conclusion:

P413GPD cut looks like an uncut plasmid
Massive gel has many blurry bands, which indicates that boiling preps are very impure

6/20/16

(XX) Unltimate Goal:

Put pSBIC3 mRPS12 TU into our own standardized yeast vectors
Validate mls function by creating mls-yeGFP construct

Goal for today:

Digest and Harvest mRPS12 TU from pSBIC3(tube 1)
5μL of DNA
1μL of EcoRI-HF
1μL of pstI-HF
1μL of CutSmart buffer
2μL of sterile water
Digest and Harvest mRPS12 mls from pSBIC3 (tube 2)
5μL of DNA
1μL of EarI
1μL of SpeI
1μL of CutSmart buffer
2μL of sterile water
Gel Order: L, 1C, 1XX, 1XL, 2C, 2XX, 2XL
**C-uncut plasmid, XX-Xintong, XL-Xander
Gel results:
Uncut does not show up on the gel
Not a very good results but we harvested the bands anyway
Other activiites:
Excise bands from the gel and perform gel extraction (QIA kit):
Tube 1 = 0.26 g
Tube 2 = 0.14 g
Tube 3 = 0.17 g
*tube 3 contains p413 GPD with NsII/NheI cut
Prepare Yeast Competent Cells
10 mL YPD, inoculated at 250RPM @ 30C
Both BY4741 and BY4741 mRPS12 is prepared

6/21/16

(XX) Goal for Today:

DNA Assembly

Major Steps:

We used nanodrop to determine the amount of DNA in tube 1 (TU) and tube 2 (mls)
Tube 1: 4.5 ng/
Tube 2: 4.0 ng/
* Nano drop results indicate that we need to precipitate DNA for further experiment


After precipitation, nanodrop reports 12.6 ng/ DNA


NEBuilder HiFi DNA Assembly Cloning Kit:
2μL Ear/SpeI digest pSBIC3 mls
8μL fragment 16-4 (yeGFP)
10μL HiFi Master
*All three above, set the reaction on ice; 1:2 vecotr: insert
Thermocycler

Other Activities:

Yeast competent cell from yesterday did not grow
Prepare new yeast competent cells: 5 mL YPD in round bottom tubes

6/22/16

(XX)Goal:

Prepare Yeast Competent cells
Diagnostic gel on mRPS12 TU minipreps

Major Steps:

Yeast competent cells:
Spectromphotometer OD 260:
1000 YPD Blank
1000 KnockOut(KO) has 1.777 Abs.
1000 Parent has 2.222 Abs.
Regrow these cells into 15 mL broth for about 2 hrs:
Take 0.5 mL current culture into 14.5 mL YPD
Spectrophotometer Results:
KO: 0.390 Abs.
Parent: 0.692 Abs.
Follow yeast competent cell protocol
Diagnostic Gel:
1: pSBIC3 mRPS12 TU miniprep 1 cut with EcoRI and PstI
2: pSBIC3 mRPS12 TU miniprep 2 cut with EcoRI and PstI
3: pSBIC3 mRPS12 TU miniprep 1 cut with PstI
4: pSBIC3 mRPS12 TU miniprep 2 cut with PstI
Gel Order: L, 1, 2, 3, 4
Gel Results:
For #2, fragment should be around 500bp
Gel results indicate that we should redo minipreps or bad enzymes



6/24/16