Difference between revisions of "Team:Arizona State/Notebook"

From earlier this week the AUBr results showed that number 9 may be a match for the vector we needed but the sequencing was returned and it was an error. Redoing the AUBr today and running the PCR for the BTA3 to try for a result on at least one per receiver.

Since it is the weekend, instead of placing the new agar plate with the 24 samples of plated AUBr and BTA3 into the 37c incubator, leaving the sample out in room temperature as to not accelerate the growth too much over the weekend. See picture below:

Defrost template, 2x Master Mix and primers
Determine desired total working volume (~20uL per tube of 24 total/ each AUBr and BTA3 have 24 samples=520ul. The additional 40ul over the 480ul is to give 40ul (2 additional samples) over as precautionary buffer)
Label reaction tubes
Create below reaction mix
Place mixture in thermal cycler at settings shown below

* Used 24 PCR tubes and labeled 1-24 for each receiver

* Thawed two AMP plate and labeled 24 spots on tray / AUB/AMBER/6/23/17 and BTA3/BRIANNA/6/23/2017

* Used 260 μl of Go Taq Green - added to each 2 DNA tubes

* Added 249.6 μl of H20, to each of the 2 DNA tubes

* Added FP and RP 5.2 ul of each to DNA tubes,(1 μ molar as final concentration)

* Pipetted 20 μl of newly mixed green solution into each PCR tube

Colony Prep: See images at the beginning of todays entry for the new plated 24 samples of AUBr and BTA3

* Next scraped one colony at a time (up to the 24 used) from the existing grown AUB plate and gently placed the colonly onto the new AUB plate with the labeled 24 spots. Disposed of each tip used into the cooresponding PCR tube labeled to match the placement number on the new AUB plate. Same protocol for the BTA3.

* Used empty pipette to attach to each tip in the PCR tubes and pump up and down to mix and remove as much of the leftover bacteria from the tip as possible so it mixed into the PCR tube. Then disposed of the tips in dry waste.

* Took 2 full sets of 24 PCR tubes to the thermocycler and had Stephan help with the settings since each setting is different for each type of bacteria or sample being run for PCR.

* PCR set to take 2.5 hours/ in process now.

PCR finished up and running gels for both the AUBr and BTA3.

Running a gel to test the DNA vector concentration that we are looking for - AUBr has 24 samples with 20 μl in each PCR tube and BTA3 has 24 samples of 20 μl each PCR tube. Will run 2 gels, one for AUB and one for BTA3, each with with 5 μl of each sample in the gel. To fit everything we ran with 2 rows of the 14 wells.

* The first gel to run is the AUBr: The first well is the KB+ ladder, the 2nd well is blank. Across the top row, in numberical order, starting in the 3rd well, are samples number 1-12. In the second row the first well is the KB+ ladder, the second well is blank and starting in the 3rd well are numbers 13-24. Ran the gel at 110V for 45 minutes.

Image of the AUBr gel setup:

* The second gel to run is the BTA3: The first well is the KB+ ladder with the second well blank. Across the top row, in numerical order, starting in the 3rd well, are 5μl samples number 1-12. In the second row the first well is the KB+ ladder, the second well is blank and starting in the 3rd well are 5μl samples number 13-24. Ran the gel at 110V for 45 minutes.

Image of the BTA3 gel setup:

In the gel results for the AUBr there were ZERO/ 0 samples that were successful:

The gel results for the BTA3 below showed that there was ZERO / 0 successful BTA3 samples.

After closer examination there were some good samples but the placement of the DNA in the loading wells was mixed up. Sequencing confirmed the fragments were what we were looking for and the error was corrected resulting in a successful experiment.

Transformation of DH5alpha with PSB1C3 and PSB1A3 backbones

Wednesday, 7/19

In preparation Alyssa and I rehydrated 2 backbones from iGEM, the PSB1C3 and PSB1A3. The C3 was from plate 7 location O,23 and the A3 was from plate 4 location H,2. Will let the plates grow overnight in the incubator and make MP samples, in triplicates of each, tomorrow.

DNA extraction from kit and rehydration protocol:

To use the DNA in the Distribution Kit, follow these instructions:

Note: There is an estimated 2-3ng of DNA in each well, following this protocol, assume that you are transforming with 200-300pg/µL

With a pipette tip, punch a hole through the foil cover into the corresponding well of the part that you want. Make sure you have properly oriented the plate. Do not remove the foil cover, as it could lead to cross contamination between the wells.
Pipette 10µL of dH2O (distilled water) into the well. Pipette up and down a few times and let sit for 5 minutes to make sure the dried DNA is fully resuspended. The resuspension will be red, as the dried DNA has cresol red dye. We recommend that you do not use TE to resuspend the dried DNA.
Transform 1µL of the resuspended DNA into your desired competent cells, plate your transformation with the appropriate antibiotic* and grow overnight.
Pick a single colony and inoculate broth (again, with the correct antibiotic) and grow for 16 hours.
Use the resulting culture to miniprep the DNA AND make your own glycerol stock (for further instruction on making a glycerol see this page). We recommend using the miniprepped DNA to run QC tests, such as restriction digests and sequencing.

* To know which antibiotics to use, look at the plasmid that the part is in. The naming scheme for plasmids is specifically designed to indicate antibiotic resistance.

7/20/2017 - something went wrong with the process, the plates to not show sufficient growth. Tests and plating will be redone today.

Gathered the available colonies and put in LB with (AMP or CHLOR) to grow overnight and replate for more usable growth to be MP. samples in the shaking incu overnight, was able to grab 3 colonies from the A3 and two from the C3. Put everything in the shaking at 345pm.

Doing the MP on the A3 and C3 growth tubes. Concentrations:

psb1c3: 80ng/ul
psb1c3: 40ng/ul
psb1a3: 50ng/ul
psb1a3: 67ng/ul
psb1a3: 75ng/ul

Notebook: Brianna Lopez

Transformation of Negative Sender and LuxR

These colonies will be used for overnight liquid culture growth, which will be used in 96-well plating for overnight growth curves.
Transformation of a negative sender, and 2620 vector.
Concentration of 2620 & Neg Sender:

-2620 = 135 ng/uL

-Neg Sender = 461 ng/uL (will have to do 1:10 dilution)

Calculation Calculation to get concentration of 60 ng/uL each:
Negative Sender:

- 461 ng/ul (1uL into 9uL H20) = 46.1 ng/uL

- 46.1 ng/uL * x uL = 60 ng

- x = 1.3 uL

2620:

- 135 ng/uL * x uL = 60 ng

- x = .44 uL

Protocol:

Materials:

Ice bucket
2620
Negative Sender
DI H20

Dilution Procedure:

One 1.5mL tube was used to perform a dilution, and labeled dilution tube.
9uL of DI H20 was pipetted into the dilution tube.
1uL of negative sender was taken out of stock and pipetted into the dilution tube.
The volume was then pipetted up and down to mix and dilute the solution.

Transformation Procedure:

One tube was labeled 2620, the other negative sender
1.3uL of negative sender was pipetted from the dilution tube into the negative sender tube
0.44uL of 2620 was pipetted from 2620 stock tube into the 2620 tube.
Tubes were then placed on ice for 2-5 minutes
The tubes were then placed on the hot plate of 42C for exactly 45 seconds then immediately placed on ice for 5 minutes.
300uL of SOC was added to each tube
It was then placed in the 37C shaking incubator for 20-30 minutes
The tubes were then spun down at 3000 rpm for 1 minute
The liquid in the tubes were gently tapped out into liquid waste
100uL of SOC was added to the tubes and gently pipetted up and down to resuspend the cells
100uL of each tube were then plated onto LB/AMP plates
Then placed in 37̊C still incubator over night

Serial Dilutions

This is where the set range of dilution concentrations comes in handy.
The dilutions for these sets of ranges is a 1:10 dilution. So, a 1-part AHL and 9-part ethyl acetate solution.
No matter how large the volume of your dilutions, it will always be 1:10.
For this project, it is a 100uL volume, therefore 10uL will be AHL solution and 90uL ethyl acetate.
In some cases, the dilution mixture will be a 50uL volume with 5uL being AHL solution and 45uL will ethyl acetate. This is to conserve the longevity of the AHL when doing a single receiver at a time and plating with 2 AHLs.
For this particular example, however, a 100uL volume and its corresponding 1:10 dilution will be performed.

100uL of the 1*10^(-2)M stock solution is pipetted into a tube (for easy access and to prevent contamination of the stock solution)
10uL of the stock solution is pipetted into 90uL of Ethyl Acetate to bring the concentration down to 1*10^(-3)M
Mixing Each Tube:

Pipette up/down
Vortex
Spin down (using tabletop centrifuge)
Continue onto the next dilution

Steps 2- 3d will be repeated until the final lowest concentration is reached.
The dilutions will be set up as follows:

For half dilutions, i.e. 5*10^(-2), 5*10^(-3) it is the same concept except they are 1:1 dilutions instead of 1:10.
Two ways of doing this includes doing one 1:1 dilution with the stock solution, then doing a 1:10 dilution using the result from the 1:1 dilution. Or it can be done doing a 1:1 dilution for each individual concentration, i.e. 1*10^(-2), 1*10^(-3)

Note: When these solutions are plated, the concentration will be further diluted by 10^-2. For example, 1*10^-2M will be pipetted to its corresponding well on the well-plate, and the AHL final concentration on the well will be 1*10^-4M. This is where the 1*10^-4M to 1*10^-14M concentration range of AHL comes into effect.

Dissolving AHL in Ethyl Acetate

The first thing that must be done is to determine the molecular weight of the AHL, in this case the Lux AHL.
Usually the synthetic AHLs are purchased from Sigma-Aldrich and depending on the volume of what is bought from the company, the milligrams it comes in is important when calculating how much must be dissolved.
In the case of this project, the final stock concentration that was desired was 1*10^(-2)M. In this project, the highest AHL concentration desired was 1*10^(-4)M, but when plated the concentration is diluted down by 10^(-2). Therefore a starting concentrating of 1*10^(-2)M is beneficial.
Then Stoichiometry must be performed to determine the volume in which the AHL in milligrams will be dissolved in, then how much ethyl acetate must be added to get to the desired final stock concentration.

First is to determine the molecular weight and container size the AHL comes in.

213.2 g/mol
10 milligrams of AHL in the container

Then is to determine the desired stock concentration.

This depends upon your range of concentrations, and how high the range is.
Range is: 1*10^(-4)M- 1*10^(-14)M
Therefore stock solution concentration: 1*10^(-2)M

Then determine how large of a stock solution is needed

Since it is difficult to measure out exact milligrams of the AHL and back into a container without losing any grams, a large enough stock solution would be the most beneficial and use the entire AHL in the container.
Desired Volume of Stock Solution: 500uL

Determine Concentration of AHL contained in the stock volume

Here is where stoichiometry comes into play. The milligrams per stock volume must be converted into standard SI molarity.
10mg/500μL * 1g/1*103mg * 1*106L/1μL * 1mol/213.2g = 0.094M
The concentration found is the stock solution concentration needed for dilutions.
Once done with the dilution to 1*10^-2 M, immediately put inside a -80C freezer for long term storage.

With the concentration found above, it will be used in the C1V1=C2V2 equation.

C1 will be the concentration found above.
V1 is the amount of AHL from stock solution into ethyl acetate solution
C2 is the concentration of the stock solution
V2 is the volume of the solution that is going to be further diluted and used in plating
(0.094M)(V1)=(50uL)(1e-2M)
V1=5.32uL AHL

Subtract AHL volume from total volume

This volume of AHL will be used to find the volume of ethyl acetate to dilute the AHL into a 1*10^-2M solution.
So, 500 – 5.32uL = 44.68uL of ethyl acetate

Add these two amounts together in a 1.5mL centrifuge tube

Mixing the Tube:

Pipette up/down
Vortex
Spin down (using tabletop centrifuge)

Immediately place dilution in the -20C freezer for immediate use of plating or for further dilutions.

Notebook:Christina Smith

Friday 9/22/17 - Running Gradient PCR on the BjaR

Materials Used for this experiment

BjaR New Receiver G-Block
BioBrick prefix Forward Primer
BioBrick Suffix Reverse primer
Phusion Polymerase
dNTP 5 mM
HF Buffer (5x)
Distilled Water

There is no particular order to place these materials into an epindorph tube. However after these components are in the tube, needed to mix them thoroughly and spin them down. After, this mixture was divided into 8 PCR tubes with ~20 uL in each. A gradient PCR protocol was setup on the computer to run. The gradient annealing temperature would run from 70 ºC to 50 ºC.

Below is a chart to describe the particular quantities of the materials used:

Materials	Quantity used in Lab’s Protocols (µL)	Quantity in Correct Ratio (µL)
BjaR New Receiver	0.2	1.6
Forward primer	0.2	1.6
Reverse Primer	0.2	1.6
Distilled Water	14.4	115.2
Phusion Polymerase	0.2	1.6
dNTPs (5mM)	0.8	6.4
HF Buffer (5x)	4	32

This particular PCR ran for 1 hour and 16 minutes. After this, I needed to run a agarose gel to verify if the DNA amplified or not. Once the gel was made, I inputted a kb+1 DNA ladder into the first slot of the gel. I skipped the second slot and proceeded to input 2 µL 6X Loading Dye + 4 µL of PCR into the remaining 8 wells. The gel was ran at 110 V for 45 minutes. The following are the wells that correspond to the annealing temperature

A: 70 ºC
B: 66.8 ºC
C: 64 ºC
D: 61.2 ºC
E: 58.4 ºC
F: 55.6 ºC
G: 52.8 ºC
H: 50ºC

This is the process to make an agarose gel:

Weigh 0.6 grams of Agarose powder and place it into a 100 mL volumetric flask.
Next, add 60 mL of TAE to the powder and place into microwave.
Microwave for 1 minute. Take out the flask using heat protective gloves and swirl the flask to dissolve the particles
Place the flask back into the microwave and run it for another 8 seconds
Using heat protective gloves, take the flask out of microwave, swirl and add 6 µL of Syber Safe DNA Stain
Pour liquid into gel mold with small dividers and let it sit for 15 minutes or until opaque

Template:Arizona State Footer

@@ Line 329: / Line 329: @@
   </table>
-<p> This particular PCR ran for 1 hour and 16 minutes. After this, I needed to run a agarose gel to verify if the DNA amplified or not. Once the gel was made, I inputted a kb+1 DNA ladder into the first slot of the gel. I skipped the second slot and proceeded to input 2 µL 6X Loading Dye + 4 µL of PCR into the remaining 8 wells. The gel was ran at 110 V for 45 minutes<p/>
+<p> This particular PCR ran for 1 hour and 16 minutes. After this, I needed to run a agarose gel to verify if the DNA amplified or not. Once the gel was made, I inputted a kb+1 DNA ladder into the first slot of the gel. I skipped the second slot and proceeded to input 2 µL 6X Loading Dye + 4 µL of PCR into the remaining 8 wells. The gel was ran at 110 V for 45 minutes. The following are the wells that correspond to the annealing temperature<p/>
+<ul>
+<li>A: 70 ºC</li>
+<li>B: 66.8 ºC </li>
+<li>C: 64 ºC </li>
+<li>D: 61.2 ºC</li>
+<li>E: 58.4 ºC</li>
+<li>F: 55.6 ºC</li>
+<li>G: 52.8 ºC</li>
+<li>H: 50ºC </li>
+</ul>
 <p> This is the process to make an agarose gel: </p>