User:GeorgeXu: Difference between revisions
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I clonewelled the [http://parts.mit.edu/registry/index.php/Part:BBa_R0011 R0011], [http://parts.mit.edu/registry/index.php/Part:BBa_R0051 R0051], and [http://parts.mit.edu/registry/index.php/Part:BBa_R0052 R0052]. | I clonewelled the [http://parts.mit.edu/registry/index.php/Part:BBa_R0011 R0011], [http://parts.mit.edu/registry/index.php/Part:BBa_R0051 R0051], and [http://parts.mit.edu/registry/index.php/Part:BBa_R0052 R0052]. | ||
[[ | [[User:GeorgeXu#My_First_Clonewell|Protocol]] | ||
====Dephosphorylation Again==== | ====Dephosphorylation Again==== |
Revision as of 10:06, 16 July 2007
Me
Important Stuff that was done (in reverse chronological order)
7/15/07
Transformation Again
I transformed the
into Top10 and plated on LB carb plates.
Ligation Again
I ligated the following parts:
Vacufuge Again
There were about .3 mL of water left in the the R0011, R0051, and R0052, so I vacufuged for about 2 hours and then resuspended in 20 µL nuclease-free water.
Clonewell Again
I clonewelled the R0011, R0051, and R0052.
Dephosphorylation Again
After discovering that the colony PCR's of the BL21 transformations were horrible, Perry decided we should try it again, but dephosphorylate before we clonewell. So I dephosphorylated the R0011, R0051, and R0052 with the following mix:
- 38 µL DNA
- 3 µL Antarctic Phosphatase
- 4.6 µL Antarctic Phosphatase Buffer
7/13/07
Transformation
I transformed the following ligated parts into BL21:
Ligation
I ligated the combinations of parts:
with the Roche Ligation Kit (the small white box with the tubes numbered 1-3)
Protocol:
- 3 µL vector (R0051 and R0011) + 7 µL insert (P0140 and P0340)
- Vortex
- 10 µL Vial 1 (ligation buffer)
- Vortex
- 1 µL Vial 3 (ligase)
- Vortex, Spin down
- Let stand for 5 min at room temperature
Dephosphorylation
I treated the R0011 and R0051 with Antarctic Phosphatase. My mix was:
- R0011
- 23.2 µL gel extracted R0011
- 2.7 µL Antarctic Phosphatase Buffer
- 1 µL Antarctic Phosphatase
- R0051
- 22.3 µL gel extract R0051
- 2.6 µL APB
- 1 µL AP
I then incubated for 1 hr @ 37dC and heat inactivated for 10 min @ 65dC.
Vacufuge
I vacufuged the samples digested on 7/12/07 for a total of about 3 hours. I then resuspended the samples in about 20 µL of nuclease-free water. I nanodropped them, but the numbers were ridiculously high (~200 ng/µL) and the curves looked awful. Note to self: never Nanodrop gel extraction again.
7/12/07
My First Clonewell
- Get iBase+Clonewell gel. Remove gel (leave the comb!) and place into iBase.
- Pre-run (Mode 0) for two minutes while the comb is still in the gel
- Take out comb, load each well in top row with 20 µL samples, the middle well with ~10 µL ladder, and the bottom row wells with 20 µL nuclease-free water
- Run the gel with (Mode 5: Run Clonewell), watch the bands and stop the gel when your desired band hits the dashed line above the bottom row of wells
- With the gel stopped, fill the bottom row wells with nuclease-free water.
- Run the gel again. When you see the band starting to enter the well, take out the sample in the well and put into clean labeled centrifuge tube. Then refill the well with 20 µL nuclease-free water and continue running the gel.
- Repeat this procedure until you get enough sample. If the band runs past the well, you can use Mode 6: Reverse Clonewell to make the band move back into the well
So basically, I did this for the stuff that was digested (see immediately below) and I ended up with a lot of water, so I am going to vacufuge the results tomorrow.
Digests of P0140, P0340, R0011, and R0051
- XbaI and PstI digests
- SpeI and PstI digest
- Mixture
- 42.5 µL DNA
- 1 µL enzyme 1
- 1 µL enzyme 2
- 0.5 µL BSA
- 5 µL Buffer 2
Perry's E-gel
I ran an E-gel for Perry's colony PCR.
- Take out E-gel (leave comb in) and put in one of the bases. NOTE: One of the red bases has a faulty contact which requires covering by aluminum foil to work correctly.
- Pre-run the gel for 2 minutes. (Press and hold either 15min or 30min on the red bases or Mode 0 on the gray bases)
- When the pre-run is finished, press any button to stop the beeping.
- Load 10 µL of nuclease-free water and 10 µL of ladder into the first well. Then 10 µL nuclease-free water + 10 µL sample into every other well. If there are empty wells, put in 20 µL of nuclease-free water into the empty wells. NOTE: Nick mentioned this and it is a pretty good idea. Put the ladder in the middle well or if there are empty wells, put ladder in the end empty wells. This way, it is easier to compare, especially if the bands bend.
- Run the E-gel for 30-min (Press 30min on the red bases, or run Mode 1 - changing the time if necessary)
- When the run is done, press any button to stop the beeping. Use the UV machine in the small room to visualize the gel.
It confirmed that P0140 and P0340 were correct. However, I don't think his GFPmeks turned out very well.
7/11/07
Sequencing
I sent out the following for Genewiz sequencing:
Part | Nanodrop (ng/µL) |
F2620 > E0240 | 130 |
I13273 | 150 |
J23039 > T9002 | 140 |
S03608 > I13507 | 220 |
S03623 > E0240 | 190 |
S03623 > I13507 | 75 |
The plan was to dilute the above samples to about 40-60 ng/µL and I did the dilutions, but I stupidly ended up using the stock instead of the dilution so our samples had a LOT more DNA than we had planned. Eh, it still ended up working out.
Order Summary:
Tube Label | Part | Primer |
AV01 | S03623 > I13507 | VF2 |
AV02 | S03608 > I13507 | VF2 |
AV03 | S03623 > E0240 | VF2 |
AV04 | F2620 > E0240 | VF2 |
AV05 | I13273 | VF2 |
AV06 | J23039 > T9002 | VF2 |
AV07 | S03623 > I13507 | VR |
AV08 | S03608 > I13507 | VR |
AV09 | S03623 > E0240 | VR |
AV10 | F2620 > E0240 | VR |
AV11 | I13273 | VR |
AV12 | J23039 > T9002 | VR |
7/10/07
7/9/07
Growing Liquid Cultures of Tomorrow's Plate Reader Samples
Stephanie and I grew liquid cultures of the following parts:
Also, Stephanie left the T9002 (+) sample incubating with 1000 nM OHHL to serve as a comparison to J37015.
Colony PCR of Ligated Parts
Stephanie, Perry, and I colony PCR'ed the parts that they ligated the week before.
See Stephanie's notebook for results.
6/29/07 FACS DAY (I13263)!
- 8:30 AM - Stephanie and I took the OD of the overnight cultures.
- Results - 1.785, 1.793, 1.780
- 9:15 AM - Stephanie and I performed first dilution (growing the 4 hr induction cells). Unfortunately, we didn't dilute correctly...
- 1:40 dilution: 50 µL liquid culture + 148 µL LB broth + 2 µL ampicillin
- 1:80 dilution: 25 µL liquid culture + 173 µL LB broth + 2 µL ampicillin
- 1:100 dilution: 20 µL liquid culture + 178 µL LB broth + 2 µL ampicillin
- 10:30 AM - Oopsie, we realized we didn't dilute 1:40, etc.; instead, we had actually diluted 1:4, etc. We measured the OD's of these incorrectly diluted samples and rediluted the samples. Note that in order to measure the OD, we diluted samples 1:100, measured the OD, and multiplied the measured OD by 100 to give us our measurement for the actual sample.
- 1:4 sample OD = 3, redilute 1:100 giving us a sample of about OD=0.03
- 1:8 sample OD = 1.8, redilute 1:30 giving us a sample of about OD=0.05
- 1:10 sample OD = 1.3, redilute 1:100 giving us a sample of about OD=0.01
- Also, we diluted 1:40, 1:80, and 1:100 2 mL samples from the overnight stock to grow as our 2 hr induction cells
- 11:00 AM - I diluted the stock solution 1:10,000 and 1:1,000,000 in 100 µL 200-proof ethanol to give a 97 µM and 97 nM solution.
- 11:30 AM - Stephanie and I diluted 1:40, 1:80, and 1:100 2 mL samples from the overnight stock to grow as our 1 hr induction cells
- 12 noon - Stephanie and I took the OD of the 4 hr induction cells
- 4 hr induction cells, 1:40: 0.2
- 4 hr induction cells, 1:80: 0.2
- 4 hr induction cells, 1:80: 0.1
Since each of these were about 2 mL samples, we didn't have enough sample to have 2 mL cuvette samples. Instead, we used 1mL of cells with 10.5 uL HSL. 2 samples were taken from the 1:40 first dilution (8:30am) - used for the 10 and 100nM HSL runs - and 1 from the 1:80, used with 1nM HSL.
- 1:30 pm - Took OD of the 1hr and 2hr samples + Induce the 2 hr samples
See Stephanie's entry for the rest
Transformation and Liquid Culture of Assorted BioBricks
Perry and I transformed and prepared liquid cultures of the following parts:
6/28/07
Resuspending the HSL stock
I took the 25 mg of N-Butyryl-DL-homoserine lactone and resuspended in 1.5 mL of 200-proof ethanol. I then put the tube in the Quorum sensing box in the freezer at Stephanie's bench.
This was done in preparation for inducing the FACS samples on 6/29/07.
Digestion of F1610: Part Two
Stephanie ran another F1610 digest with
- 2.5 µL Buffer 2
- 0.5 µL BSA
- 0.5 µL XbaI
- 0.5 µL PstI
- 21 µL F1610
Basically it is the same as the previous digestion except we now have 21 µL vs. 15 or 6 µL of DNA. This was done because the Clonewell of the F1610 that Perry and I ran had an almost invisibly faint band corresponding to the F1610. Where did all the DNA go?
Grow Liquid Cultures of I13263
Stephanie and I grew I13263 in preparation for the FACS on 6/29/07.
Sequences
Perry checked the sequences that we got back from Genewiz
Results
- F1610 (something is very wrong...)
- The actual part is 798 bp, we got back a sequence ~300 bp
- The sequence contains the terminator and some random junk after it
- I13263 (w00t)
- The first and last ~650 bp are perfect.
- I13273
- !!!!add something here
!!!!upload the sequences?
Clonewell of F1610
[User:GeorgeXu#My_First_Clonewell Protocol]
Results
F1610 is about 800 bp. There is an almost invisibly faint band at 800 bp. What happened to all the DNA? We need to run it again
Transformation of Additional Parts
Perry and I transformed the following parts
Digestion of F1610 (XbaI, PstI)
Mix 1:
- 2.5 µL Buffer 2
- 0.5 µL BSA
- 0.5 µL XbaI
- 0.5 µL PstI
- 15 µL F1610 (168 ng/µL)
- 6 µL Nuclease-free water
Mix 2:
- 2.5 µL Buffer 2
- 0.5 µL BSA
- 0.5 µL XbaI
- 0.5 µL PstI
- 15 µL Nuclease-free water
- 6 µL F1610 (168 ng/µL)
Perry and I ran two digests of F1610 with different amounts of DNA. The plan is to gel extract and ligate with the promoters that Perry has transformed.
6/27/07
Sequencing the Midiprepped QS parts
Just checking if the Midiprepped sequences are correct. Details of the order:
Tube Label | DNA Name | DNA Length | Primer |
AV01 | F1610 | 3987 | VF2 |
AV02 | F1610 | 3987 | VR |
AV03 | I13263 | 4123 | VF2 |
AV04 | I13263 | 4123 | VR |
AV05 | I13272 | 4162 | VF2 |
AV06 | I13272 | 4162 | VR |
Transformation of I13263
Stephanie and I transformed 1 µL of the I3263 that we midiprepped into 30 µL of BL21. We then plated them onto agar+ampicillin plates. We eventually want to carry out a test experiment by inducing the I3263 with different concentrations of HSL to test and possibly start characterizing the part.
Hispeed! Midiprepping of the QS parts
Perry and I Midiprepped the QS parts in order to get DNA that we could sequence and transform.
6/26/07
Growth of QS parts in Liquid Cultures
We grew the QS parts in a liquid LB+ampicillin broth.
Nanodrop
Results
10mer: 389.8 ng/µL
15mer: 278.6 ng/µL
20mer: 168.7 ng/µL
Nucleotide Removal of the 10mer, 15mer, and 20mer library
Again, this was done in preparation for the ligation reaction that we will do with the massive amounts of DNA.
PCR Extension of the 10mer, 15mer, and 20mer library
Basically, this was done in preparation for the ligation reaction that we will do with the massive amounts of DNA.
6/25/07
Transforming and Plating the QS parts
Perry transformed the parts F1610, I13263, and I13272 into Top10 cells and plated them on LB+ampicillin plates. We want to sequence the parts, test them, and eventually use them in our BL21 cells.
6/22/07
Counting colonies: Overnight vs. Short Ligation
We counted the number of colonies in the Overnight vs. Short Ligation plates.
Results
Nanodrop of Ligated Colonies
Results
OmpA1+random library+extension: 50.8 ng/µL
OmpA2+random library+extension: 50.7 ng/µL
The curves looked smooth. %
6/21/07
Protein Gel of OmpA+His/OmpA+Strep Cells
We ran this protein gel to see if the OmpA1+His, OmpA1+Strep, OmpA2+His, and OmpA2+Strep was actually expressed. Also, we wanted to see if there was any difference between the immediate induction, delayed induction, and no induction.
Bacterial Innoculation and Induction
Inocculation and Induction Protocol
Measuring Optical Density Protocol
We took the OmpA1+His, OmpA1+Strep, OmpA2+His, and OmpA2+strep that were grown in liquid culture overnight starting on 6/20/07 and split them into three sets. The first set was not induced, the second set was immediately induced with 10 µL IPTG¸ and the final set was induced once it hit log phase, which we determined by measuring the optical density.
6/20/07
Gel Extraction
We extracted the DNA from the gel we ran on 6/19/07
6/19/07
Running the OmpA1/OmpA2 gel
We poured a gel and ran the DNA from the dephosphorylated samples.
Dephosphorylating the OmpA1/OmpA2
Six times this amount of mix was made as a Master Mix in order to dephosphorylate the OmpA1 and OmpA2. There were five groups total:
- Group 1: OmpA1, Nhe1, Pst1
- Group 2: OmpA1, Nhe1, Pst1
- Group 3: OmpA2, Nhe1, Pst1
- Group 4: OmpA2, Nhe1, Pst1
- Group 5: Perry...