Vincent Parker Notebook

From 2007.igem.org

(Difference between revisions)
 
(2 intermediate revisions not shown)
Line 143: Line 143:
*Could not transform since we were lacking of Righty competent cells.
*Could not transform since we were lacking of Righty competent cells.
*Miniprepped otsB-RBS-otsA-TT(BRAT).
*Miniprepped otsB-RBS-otsA-TT(BRAT).
-
*Used wrong enzyme to digest T7-RBS and BRAT. Fact thatT7-RBS was too small to gel extract did not occur to me. Re-set up a digestion using Bsa1 and BamHI. Sizes of bands would be even so i also digested T7-RBS with Alwn1.
+
*Used wrong enzyme to digest T7-RBS and BRAT. Fact thatT7-RBS was too small to gel extract did not occur to me. Re-set up a digestion using Bsa1 and BamHI. Sizes of bands would be even so i also digested T7-RBS with AlwnI.
*Digested BRAT with Bsa1 and BglII.
*Digested BRAT with Bsa1 and BglII.
*Sent off sequences for BRAT.
*Sent off sequences for BRAT.
Line 156: Line 156:
*Colony PCRed otsBA and transferred to liquid media.
*Colony PCRed otsBA and transferred to liquid media.
*Just transferred TBRAT into liquid media. (The addition of T7-RBS is too small to make a significant difference in band sizes.)
*Just transferred TBRAT into liquid media. (The addition of T7-RBS is too small to make a significant difference in band sizes.)
 +
 +
[[User:Vparker|Vparker]] 13:53, 27 July 2007 (EDT)
 +
*Digested otsBA-TT with using BsaI, BglII.
 +
*Ligated digestion of otsBA-TT with T7-RBS.
 +
*After heat kill digested again with BglII/BamHI.
 +
*Transformed BA-Operon to righty cells.
 +
*Miniprepped TBRAT and sent off 28 sample sequences of TBRAT and BA-Operon.
 +
*Transformed TBRAT into BLR plasmid.
 +
 +
[[User:Vparker|Vparker]] 13:53, 28 July 2007 (EDT)
 +
*Placed colonies from TBRAT and BA-Operon into liquid media.
 +
 +
[[User:Vparker|Vparker]] 13:53, 30 July 2007 (EDT)
 +
*Miniprepped BA-Operon and then transformed into the BLR strain as well.
 +
*Made variable samples containing BLR, BLR+TBRAT, BLR+TBRAT+inducer.
 +
*Streaked BLR onto a plate.
 +
*Also transformed more T7-RBS running low on supplies.
 +
 +
[[User:Vparker|Vparker]] 13:53, 31 July 2007 (EDT)
 +
*Took out tubes and checked plates.
 +
*Transferred BA-Operon and T7-RBS into liquid media.
 +
*Learned about mid-log and then placed media into incubator to reach mid-log.
 +
*Used Specto to check O.D. of the media.
 +
*Used liquid nitrogen and froze pelleted samples once mid-log was reached and then went upstairs and put into lypholizer overnight.
 +
 +
[[User:Vparker|Vparker]] 13:53, 1 August 2007 (EDT)
 +
*Put BA-Operon into incubator to reach mid-log like with TBRAT.
 +
*Resuspended cells that were freeze dried and made a dilution which was then transformed.
 +
*Suspended some mid-log tubes in drierite.
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
-
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
+
*Checked plates for growth of TBRAT.
-
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
+
*Put in 5 different flasks of BLR mixtures.
-
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
+
 
-
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
+
Time put into incubator 10:45      OD @ 11:45    OD @ 12:20    OD @ 12:50    OD @ 1:05      OD @ 1:25
-
[[User:Vparker|Vparker]] 13:53, 2 August 2007 (EDT)
+
1.BLR                              1).096        1).17        1).32         
 +
2.BLR+Plasmid                      2).4          2).08        2).126        2).17       
 +
3.BLR+BA Plasmid                    3).7          3).11        3).2          3).27        3).255
 +
4.BLR+PLasmid+Inducer              4).056        4).04        4).04                        4).032
 +
5.BLR+BA Plasmid+Inducer            5).056        5).04        5).04                        5).039
 +
 
 +
Seeing as growth stopped after a certain amount of time it was decided to redo the assay.
 +
Did however place a mol in the lyopholizer overnight to test resistance to freeze-drying.
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 3 August 2007 (EDT)
 +
*Resuspend tubes taken out of lyopholizer in dilutions of X, 10X, 100X, and 1000X.
 +
*Resuspended in 2 mols of LB broth. Vortexed out to mix.
 +
*once resuspended transformed onto plates and left in incubator to grow overnight.
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 6 August 2007 (EDT)
 +
*From plates left in incubator only colonies grew on X and 10X plates of the BLR+BA Plasmid and BLR+Plasmid(TBRAT plasmid)
 +
*Decided to retry experiment with a new variable: sucrose.
 +
*Took .4 grams and dissolved into 10 mil of water. Then added to shaker flasks of BLR, BLR+BA Plasmid, and BLR+BA Plasmid+Inducer. Used only BA plasmid because produced best results.
 +
 
 +
Placed in Incubator @ 1:45        OD @ 2:45    OD @ 3:45    OD @ 4:15
 +
1.BLR                            1).156      1).137        1).150
 +
2.BLR+BA Plasmid                  2).068      2).07        2).69 
 +
3.BLR+BA Plasmid+Inducer          3).065      3).065        3).62 
 +
4.(S)BLR                          4).142      4).152        4).168 
 +
5.(S)BLR+BA Plasmid              5).061      5).063        5).062 
 +
6.(S)BLR+BA Plasmid+inducer      6).064      6).063        6).059
 +
 
 +
*In order to continue experimentation I needed to streak new BLR and put the BA Operon into liquid media to use for tomorrow.
 +
 
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 7 August 2007 (EDT)  
 +
*Assay seemed to be missing something. I decided to reproduce the experiment but with new media.
 +
* grew new media and ran procedures for lypholization.
 +
 
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 8 August 2007 (EDT)
 +
*Resuspended 1 mil of each flask and resuspended for transformation.
 +
*6 plated in AMP(BLR+plasmids) 2 plated in agar(BLR only)
 +
 
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 9 August 2007 (EDT)
 +
*No living colonies seen on any plate.
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 10 August 2007 (EDT)
 +
*Since i need to switch mid log media i will have to use Ptet strain as my new vector.
 +
*Need to ligate otsBA-TT to Ptet vector.
 +
*Did ligation then second digestion with Bam/Bgl.
 +
 
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 12 August 2007 (EDT)
 +
*Came in this weekend to miniprep real fast and i took 5 colonies of Nhu's plates and put them into liquid media and then into the incibator.
 +
 
 +
 
 +
[[User:Vparker|Vparker]] 01:49, 13-17 August 2007 (EDT)
 +
After having successflly cloned my operons into Ptet strain. I realized that I have run out of time on my project over the summer. My conclusion is that indeed trehalose does help with dessication in biological organisms and that from my experiment my operon produced better from not having an inducer and plated at higher concentration rates. If my part of the project were continued I could have continued experimenting with the Ptet strain and eventually found a promoter and RBS site that would produce better results that would have more percentage the bacto-blood recover after having been freeze dried.
 +
 
 +
      It was a great experience for me over the summer and it was great working with all of the iGEM crew.

Latest revision as of 06:28, 26 October 2007

My Construction Files
My Sequencing Files

Vparker 17:11, 20 June 2007 (EDT) The sequences of the oligos I designed are as follows:

   VP1AF-cgtaaAGATCTATGAGTCGTTTAGTCGTAGTATC
   VP2AIF-CGATGACATTATCTGGATtCACGATTATCACCTG
   VP3AIR-CAGGTGATAATCGTGaATCCAGATAATGTCATCG
   VP4AR-cgtatCTCGAGttaGGATCCTTACGCAAGCTTTGGAAAGGTAGC
   VP5BF-cgtaaAGATCTATGACAGAACCGTTAACCGA
   VP6BIF-GCAACGTATTACTCAGATtTGGCCACAAATGGCG
   VP7BIR-CGCCATTTGTGGCCAaATCTGAGTAATACGTTGC
   VP8BR-cgtatCTCGAGttaGGATCCTTAGATACTACGACTAAACG

The oligos were named according to my initials, numerical sequence, and letters determining direction of oligo. Ex. VP1AF- Vincent Parker 1 otsA Forward.


Vparker 15:04, 21 June 2007 (EDT) After a long wait the oligos that I have ordered have arrived. I ordered 8 which PCR the two genes and get rid of the internal restriction sites. The template used to make the oligos was called MG 1655. In the ApE file which was split into two genes they were called ostA and otsB. They came in powder form and we have to dilute them down to 10 micro mols. That makes my master supply of my oligos when i use them i have to dilute them down to 100 micro mols. Using my oligos I can determine my PCR products... otsA will be broken up into two parts; PartA is 413 bps and PartB is 1077 bps. OtsB; PartA 485bps, PartB 381bps. I will PCR them overnight and digest tomorrow. Part A of otsA will be called V1-3 because i am using oligos 1 and 3 to PCr that specific part. Part B of otsA will be called V2-4. Part A of otsB will be called V5-7 and part B of otsB will be called V6-8.

VParker 16:37, 22 June 2007 (EDT) Big day planned. I have to take out my tubes V1-3, V2-4, V5-7, and V6-8 from the PCR machine.These are the 4 parts to my two genes. V1-3 is Part A of my otsA gene, it ends at the internal restriction BamHI site. V2-4 is part B to my otsA gene and it starts with the BamHI restriction site. I have already designed my oligos which code for a silent mutation within the BamHI site and codes for Leucine. V5-7 is part A of my otsB gene and ends at an internal BglII restriction site. V6-8 is part B of my otsB gene and starts at the BaglII restriction site and I have designed the oligos for that gene to have a silent mutation in the BglII site that codes for Isoleucine. As i came in to PCR my two genes, otsA and otsB, with the 8 oligos i designed. Two oligos per part. The oligos are named by number so when I mention V1-3 i am referring to part A of otsA but it will be PCRed with the first and 3rd oligos. Unfortunately when i came into the lab it was flooded and all I managed to do was take out Hannah's tube and my four out of the PCR machine and put them into the freezer for Monday. I did manage however to go home and sleep some more :-)


Vparker 16:02, 25 June 2007 (EDT)

Today i came into the lab and found that 3 out of the 4 PCR tubes were in the freezer but that i have lost the tube marked V6-8. I had the PCR products from the tubes V1-3, V2-4, and V5-7. After having fumed a bit over my lost PCR I went to work on setting up a new PCR tube for V6-8 and to also clean tubes V1-3, V2-4 and V5-7. Austin was kind enough to share the PCR machine with me and i put in the tube V6-8 in and also the sewing reaction i was working on named V1-4. V1-4 is a combination between V1-3 and V2-4. Since V1-3 and V2-4 are two parts of one gene and I had to PCR out the internal restriction site.
This is the gel of the PCR tubes of V1-3, V2-4 and V5-7 since 6-8 was missing. I took the gel out a little bit early but it shows that PCR did work by the fact that the bands are so solid and bright I put the gel back in for another 5 minutes.

Decided to try my hand in Agar plates today so I volunteered the High School team to learn how to prepare and pour them since Arthur was not here. They turned out looking good with no bubbles. So i was behind today in terms of my PCR and i have to digest and ligate tomorrow instead of today. Losing the V6-8 tube set me back an hour and a half so i will save the rest for tomorrow.
PCR V1,3; V2,4; V5,7


Vparker 15:04, 26 June 2007 (EDT) Started off today with digestion of tubes V1-4 and V5-8 which are my genes that i PCRed. V1-4 was my otsA gene and V5-8 was my otsB gene. Atfer storing them in cultivation for an hour and a half Sam showed us how to prepare Agar solution and broth. we just put them in the autoclave machine and are waiting for both digestion and the autoclave to finish. There were problems with the autoclave because maybe the person who used it before us did not reset it after. Our Agar jars had to sit out while the machine exhausted itself and reset to take in our bottles. Nhu and I poured over 5 sleeves to help out the lab. The digestion of my tubes went well there were no problems and afterward I had to gel extract the DNA. I did not take a picture because too much exposure to UV rays is dangerous to my DNA and I wanted to keep as much of it as I could for the ligation process after I cut out the bright DNA bands from the gels. I had to melt the gels and put them through gel extraction recovery kit which binds the DNA to a filter and washes out all the enzymes and other solutions not wanted when I ligate the DNA to the vector. The number on the vector tube was 9145 and I named my ligation tubes otsA9145 and otsB1945. After ligation I had to heat shock the competant E.coli cells so that their membrane would become passive to the plasmid which contained my genes. I then used the little glass balls and smeared my competant cells with now hopefully my plasmid inside them. Tomorrow after I come in i will see if my bacteria grow. If not i am a complete failure :-(


Vparker 14:57, 27 June 2007 (EDT)

Came into work and had a nice spread of bacteria growing on my agar plates. On the agenda for today: colony PCR, which I am doing as I type this, followed by gel to make sure the colony I chose for PCR has the insert I want, and then I have to drop a colony into liquid media so that I can mini-prep for tomorrow. So far I am off to a rough start as I am only PCRing two colonies and I should have done at least 2 from each gene so that I can maximize my chances for success. I have basically done a gamble by only doing one colony for each gene and that chances of failure are high. With some great luck hopefully both were successful colonies and I won't have to re-PCR them. After lunch we will see after the gels if my colonies were chosen wisely. Just returning from lunch and PCR was already completed. Took 15 minutes to gel and the picture was perfect. The two genes I wanted to show within the bacteria are both present and my cloning process was a success. For today I have to transfer the bacteria to a liquid media and let incubate in a shaker over night. Tomorrow we will mini=prep the liquid media and then send off for sequencing. Also today we have a staff meeting at 3:00pm when I have to tell the group where I am and just an overall presentation of what I have done so far. Here is a picture of my gel form today.
Colony PCR 1


Vparker 16:37, 28 June 2007 (EDT)

After taking my 4 tubes out of the shaker, two tubes from each plate of colonies. All 4 of them where the proper color meaning that the plasmid was taken into the E.coli and the RFP was taken out. After mini-preping and accidentally drifting a little from the manual the DNA is in digestion right now to make sure the the plasmid that is in the Bacteria does in fact have our insert. I am digesting the plasmid with BglI and AlwnI which one cuts the insert and one cuts the plasmid. So if I have a band that does not correspond with what the digestion should be then that means the plasmid does not have my insert. If the bands are good then I can send them off for sequencing and tomorrow I will have to verify the sequences. With digestion done, gel has been completed and heres the pic:
The DNA analysis of the digestion of otsA and otsB


Vparker 15:20, 29 June 2007 (EDT) Sequences came in today with complete success in terms of my inserts being inside the plassmids and the cloning process was perfect. Today I have to design my operons using 6 basic Biobrick parks. My operon will look like this:


T7(promoter)-AGGAGG(Rbs site)-otsB-AGGAGG(Rbs site)-OtsA-terminator site.


The T7 promoter will make it transcribe a lot since we want the bacteria to produce a lot of the Trehalose sugar which will allow it to recover form freeze drying. We want otsB to be expressed more thats why its in front and then HOPEFULLY our Rbs sites will work. If not I will have to go to the library to experiment with others. I also clone saved my otsA and otsB. I have transformed everything I need for the operon into plates and they should be ready on Monday. I was also given an extension on my project. Besides the operon i designed Chris also wants me to form the operon of how it naturally exists in the E.coli cell. In the E.coli there is no Rbs site inbetween the otsB and otsA and they actually overlap a little which means I will have to sew together a 3 piece gene. The operon looks like this.


T7(promoter)-AGGAGG(Rbs site)-otsBotsA-terminator site.



Vparker 12:45, 2 July 2007 (EDT)

Today I took out my plates and saw that bacteria formed on all of them. I set those aside to transfer into liquid media later. But I then took out my PCR product of the sewing process where I needed to PCR out the internal sites again. The PCR product would be bigger because it is both otsB and otsA together and I have no idea how much of them is actually overlapping. But I took out the 3 pieces I tried to sew and took a picture and gel extracted. I had to take a quick picture so as to not damage my DNA because I had to cut it out of the gel too
PCR of the gene that contains the combination of otsB and otsA together. The way E.coli naturally has it in its chromosomes.
After the gel extraction and cleaning I attempted in sewing all three pieces of the PCR product together so that I could have whole otsB otsA gene. After that PCR I took a picture of the gel to see the outcome. The picture was kinda double vision but you could still see where the bands correlated with the marker.
The gel of my finished 3-way sew shows that all three PCR's worked and that i have no use for the two bands on the side since the middle band worked.
The picture showed success and I have so far sewed 3 pieces together. I decided to digest overnight for 16 hours so hopefully the finished piece is the length I want it when I gel it next morning. I then transferred my plates to liquid media so that they can be in use to others.


Vparker 13:34, 3 July 2007 (EDT) I took out the liquid media and mini-prepped my 5 samples. I then gelled them all to see if my transforming worked properly. After gelling I went to gel extract each one and they all had bright bands. The only problem was that otsA only had one band and it was supposed to have two. So I cut each one out and gel purified anyways but i set up an overnight digestion of otsA so that in the mornign I could re-gel it and re-gel extract it. As for otsBA I digested, then extracted and then ligated into 9145 plasmid and transformed into competent cells. I should have colonies for tomorrow to put into liquid media and then later to prep.


Vparker 13:34, 4 July 2007 (EDT) Came in rather early just to get work done fast. I helped out Nhu by mini-prepping some of her liquid medias for her while i was gel purifying otsA and waiting to put otsBA into liquid media. OtsA did in fact have 2 bands this time around so I extracted from the gel, purified it and then brought out the T7, RBS,otsB, and TT purified end results from PCR clean up. I then transformed T7, otsA, and otsB into lefty competent cells and transformed RBS and TT into righty competent cells. Took out a colonized plate of otsBA and went straight into liquid media.


Vparker 13:34, 5 July 2007 (EDT)

Failure. Failure. Failure. I mini-prepped otsBA but then I was reminded that I never colony PCRed so I decided to send them off for sequencing anyways with 3 samples to help increase odds. That was one of the first things that went wrong. Second was when I gel extracted my T7 I cut a band that was close to 2k bp when the T7 promoter is only about 50 bp in itself. So my plate that grew with lefty T7-RBS is garbage and I also did not do another digestion with BglII after the ligation. Which means that there is a high probability of impure plasmid being transformed with what I want. So I set up another digestion of lefty T7-RBS, lefty otsB-RBS, and righty otsA-TT. But this time, after ligation I re-digested with BglII and then transformed into their corresponding competent cells. I prepared my 12 samples of otsBA for sequencing and sent them off. I just forgot to put on the order form that samples 7-12 were premixed with primers already so I have to hope for the best. Since I had plates with lefty T7-RBS, lefty otsB-RBS and righty otsA-TT I had to do a colony PCR of 24 samples one from each plate just to see if any of them had what we wanted. After we gelled. It confirmed that our T7 was garbage and that otsA-TT was ok and maybe otsB-RBS. there was speculation about the otsB becuase the band was closer to otsA's than to where otsB should've been.
The gel of my T7-RBS on top shows the bands are way too big to contain the part I need. Bottom left 8 are otsA which are good bands and the bottom right 8 are otsB and are questionable about success.


Vparker 13:34, 6 July 2007 (EDT) A taste of failure again. Could not gel the digest of the T7 to analyze to see if bands matched. All I managed to see BOTH times were just nice black bands and no DNA whatsoever. Then I colony PCRed the composite parts of LT(lefty T7), LB(lefty otsB), and RA(righty otsA) and the bands did not match up with the bands I wanted. I needed to start the cloning process over again. I transformed some more T7 because I used most of it trying to see bands. Need to put into liquid media and mini-prep to have new stock of T7. I did another digestion of T7 and used a different buffer and used more insert and did actually get a gel which showed that the T7 was a good plasmid. Also made my construction file of otsBA. Left an overnight digestion of my new composite parts which I will ligate and transform on Monday.


Vparker 15:10, 9 July 2007 (EDT) Needed more otsA and otsB in the lefty for my composite parts so i miniprepped more from my stock. I ligated the overnight digestion of the composite parts and put them into lefty and righty E.coli competent cells. Needed to gel extract before ligation. Also need to send off otsBA my original PCR for sequencing because I got back the sequences for my forward and reverse primers and I unfortunately had a point mutation that was not silent. And I need to send it off for sequencing to see if it is from my original PCR product. Also need to put T7 into liquid media to mini prep tomorrow for Tulga.


Vparker 17:50, 10 July 2007 (EDT) Mini-prepped more T7 105 wild type for Tulga and gave him a new stock and started to mini-prep otsBA but then sequences came back with the same point mutation and so T just threw away the otsBA tubes. I then re-PCRed V5-7 from my original template Mg1655 to try to cleanse the point mutation out. After PCRing V5-7 again I gelled it along with the conolyPCR product of otsB-RBS and otsA-TT. I also had T7-RBS but I needed to make a special gel with twice the amount of agarose in it to have the thickness needed so that the small band wouln't travel too fast. I then waited until before I left to transfer X's I made of the conolyPCR's bacterial colonies into liquid media so that tomorrow I would have usable mini-prepped stocks of my composite parts for tomorrow.

The gel of my otsB-RBS, otsA-TT and of my PCR or 5-7.
I then PCRed together my 5-7 and an old finished 6-4. This would sew together the two pieces and give me the entire otsBA genes together.


Vparker 18:22, 11 July 2007 (EDT) Gel extraction right when I got to work. Extracted the PCR cleanup of 5-4 which was the finished product of 5-7 and 6-4. I then sent it off for PCR sequencing to see if I managed to defeat that pesky point mutation. Needed to digest lefty otsB-RBS and righty otsA-TT in order to be able to ligate them together. But then I found out we were out of plasmid so I digested some plasmid in BglII and XhoI so that I could refill the stock for the lab. I digested my lefty otsB-RBS with EcoRI and BamHI. I digested my righty with EcoRI and BglII. My left will turn into my insert and my righty will turn into my vector. After digestion gel extraction was necessary to purify out the bands I needed. The lefty I took the smaller band and the righty I took the only band because the other band is too small to see. Problem came with the bands form my digestion of the Bca1144 plasmid which should have had two bands but instead had 3 bands with two of them very close together. So I took the band that was closer to 2k which was the one that was originally supposed to be taken. Digested otsBA too with BglII and XhoI so that it would be able to be ligated with Bca1144. Cut out that band with no problems. Ligated together LB(lefty otsB-RBS) and RA(righty otsA-TT). After that ligation sat for a half an hour I heat killed the ligase and then digested again with BglII and BamHI to take advantage of the methylated sites from the lefty and righty competent cells. I then transformed the digestion straight into righty competent cells to grow for the next morning.


Vparker 18:22, 12 July 2007 (EDT) Richard gave me my sequences and compared them. I had success with the T7-RBS. 2 out of 4 samples had what I needed but I did not number my samples of I need to send them off again just to verify which ones are which. My otsB-RBS came back perfect. My otsA-TT sequences actually came back coding for otsB-RBS so I either gave them all otsB-RBA and no otsA-TT or I actually have no otsA-TT and just otsB-RBS and I need to make some otsA-TT. I then took my plates from the RA and LB and colony PCRed that. The picture I took of it after was dismal. I was expecting 2k bands which in reality I somehow got a 1k band in each well. Meaning I have all parent vectors or.... its only otsB-RBS which would be closest with that band. Went to pizza lunch provided by Kate and after I transformed the otsBA in 1144 into lefty competent cells to only check if the plasmid is O.K. The sequences from otsBA the PCR came back with the same point mutation!!! This has been very troublesome since my other otsB that I originally PCRed did not have this mutation. I have traced the roots to template provided to me by Chris. I had an original tube which gave me my separate otsA and otsB. I ran out of the tube before I could use it for otsBA and Chris supplied me with a new tube from which I have yet to have a mutation free otsB come out of. I then decided to PCR from my original otsB and I actually had some left mover V5-7 in my box which I just then continued to sew to 6-4 which by my calculations should not have the point mutation I loath so much.


Vparker 14:52, 13 July 2007 (EDT)

  • Tranformation of Vector Bca1144 turned up all pink.
  • Sequences from otsBA in mutation still found.
  • Left PCR of otsB. Gel extracted, Cleaned up, and digested.
  • Pcr 5-7/6-4

Vparker 14:52, 16 July 2007 (EDT)

  • Ligation of L otsA and R TT.
  • Digested with BamHI/BglII and tranformed.
  • Gelled 5-7/6-4 PCR and digested with BglII/XhoI and then ligated to clone vector.
  • otsBA Transformed.

Vparker 14:52, 17 July 2007 (EDT)

  • Did not show up. Bonds did ligation of otsA-TT again because plates did not grow.
  • Colony PCRed otsBA and all samples worked well.

Vparker 14:52, 18 July 2007 (EDT)

  • Miniprepped otsBA.
  • Sent off 2 samples for sequencing. Went to A's Game.
  • Digested L otsBA, L otsA and R TT.

Vparker 14:52, 19 July 2007 (EDT)

  • Ligated and digested otsA-TT. Will tranform.
  • Sequences for otsBA came in and mutation still there.
  • Ordered oligos to quickchange out the mutation.
  • Caught up on construction files for composite parts.

Vparker 14:08, 20 July 2007 (EDT)

  • Colony PCRed otsA-TT with one being a big ligation and one bing a small ligation. They were thus dubbed L and S.
  • Transferred to liquid media immediately after colony PCR.
  • Prepared the oligos for the quickchange of otsBA to PCR out the mutation.
  • Then did quickchange of otsBA, then digested and tranformed.
  • Clone saved otsB-RBS.

Vparker 14:08, 21 July 2007 (EDT)

  • Miniprepped samples for Nhu and my otsA-TT's.
  • Colony PCRed the quickchange of otsBA and simultaneously transferred to liquid media.
  • Digested otsB-RBS and otsA-TT with Eco/Bam and Eco/Bgl.
  • Gel extraction and purification then ligated together.
  • Another digested of Bgl/Bam and then transformed into 4 dishes. S1, S2, L3, & L2.

Vparker 14:08, 23 July 2007 (EDT)

  • Miniprepped otsBA quickchange.
  • Sent of 16 sequencing samples of otsA-TT and otsBA.
  • Colony PCR of otsB-RBS-otsA-TT proved positive.
  • Digestion of otsBA, gel extracted and ligated to TT.
  • Out of Righty comp. cells so put in freezer until more are available.

Vparker 14:08, 24 July 2007 (EDT)

  • Checked sequences from Richard and otsA-TT and otsBA are both good samples.
  • Miniprepped otsBA quickchange.
  • Took risk and digested otsBA and then ligated the TT terminator.
  • Did not heat kill. Set back one hour to heat kill and re-digest with BamHI and BglII.
  • Could not transform since we were lacking of Righty competent cells.
  • Miniprepped otsB-RBS-otsA-TT(BRAT).
  • Used wrong enzyme to digest T7-RBS and BRAT. Fact thatT7-RBS was too small to gel extract did not occur to me. Re-set up a digestion using Bsa1 and BamHI. Sizes of bands would be even so i also digested T7-RBS with AlwnI.
  • Digested BRAT with Bsa1 and BglII.
  • Sent off sequences for BRAT.

Vparker 14:50, 25 July 2007 (EDT)

  • BRAT sequences came in all looking good but decided to use 2S2 as clone Saver.
  • Gel extracted overnight digestiong of T7-RBS and BRAT.
  • Ligated together to make TBRAT. Transformed 4 TBRATS into regular comp cells and two otsBA-TT's into righty comp. cells.

Vparker 14:50, 26 July 2007 (EDT)

  • Colonies on all plates.
  • Colony PCRed otsBA and transferred to liquid media.
  • Just transferred TBRAT into liquid media. (The addition of T7-RBS is too small to make a significant difference in band sizes.)

Vparker 13:53, 27 July 2007 (EDT)

  • Digested otsBA-TT with using BsaI, BglII.
  • Ligated digestion of otsBA-TT with T7-RBS.
  • After heat kill digested again with BglII/BamHI.
  • Transformed BA-Operon to righty cells.
  • Miniprepped TBRAT and sent off 28 sample sequences of TBRAT and BA-Operon.
  • Transformed TBRAT into BLR plasmid.

Vparker 13:53, 28 July 2007 (EDT)

  • Placed colonies from TBRAT and BA-Operon into liquid media.

Vparker 13:53, 30 July 2007 (EDT)

  • Miniprepped BA-Operon and then transformed into the BLR strain as well.
  • Made variable samples containing BLR, BLR+TBRAT, BLR+TBRAT+inducer.
  • Streaked BLR onto a plate.
  • Also transformed more T7-RBS running low on supplies.

Vparker 13:53, 31 July 2007 (EDT)

  • Took out tubes and checked plates.
  • Transferred BA-Operon and T7-RBS into liquid media.
  • Learned about mid-log and then placed media into incubator to reach mid-log.
  • Used Specto to check O.D. of the media.
  • Used liquid nitrogen and froze pelleted samples once mid-log was reached and then went upstairs and put into lypholizer overnight.

Vparker 13:53, 1 August 2007 (EDT)

  • Put BA-Operon into incubator to reach mid-log like with TBRAT.
  • Resuspended cells that were freeze dried and made a dilution which was then transformed.
  • Suspended some mid-log tubes in drierite.

Vparker 13:53, 2 August 2007 (EDT)

  • Checked plates for growth of TBRAT.
  • Put in 5 different flasks of BLR mixtures.

Time put into incubator 10:45 OD @ 11:45 OD @ 12:20 OD @ 12:50 OD @ 1:05 OD @ 1:25 1.BLR 1).096 1).17 1).32 2.BLR+Plasmid 2).4 2).08 2).126 2).17 3.BLR+BA Plasmid 3).7 3).11 3).2 3).27 3).255 4.BLR+PLasmid+Inducer 4).056 4).04 4).04 4).032 5.BLR+BA Plasmid+Inducer 5).056 5).04 5).04 5).039

Seeing as growth stopped after a certain amount of time it was decided to redo the assay. Did however place a mol in the lyopholizer overnight to test resistance to freeze-drying.

Vparker 01:49, 3 August 2007 (EDT)

  • Resuspend tubes taken out of lyopholizer in dilutions of X, 10X, 100X, and 1000X.
  • Resuspended in 2 mols of LB broth. Vortexed out to mix.
  • once resuspended transformed onto plates and left in incubator to grow overnight.

Vparker 01:49, 6 August 2007 (EDT)

  • From plates left in incubator only colonies grew on X and 10X plates of the BLR+BA Plasmid and BLR+Plasmid(TBRAT plasmid)
  • Decided to retry experiment with a new variable: sucrose.
  • Took .4 grams and dissolved into 10 mil of water. Then added to shaker flasks of BLR, BLR+BA Plasmid, and BLR+BA Plasmid+Inducer. Used only BA plasmid because produced best results.

Placed in Incubator @ 1:45 OD @ 2:45 OD @ 3:45 OD @ 4:15 1.BLR 1).156 1).137 1).150 2.BLR+BA Plasmid 2).068 2).07 2).69 3.BLR+BA Plasmid+Inducer 3).065 3).065 3).62 4.(S)BLR 4).142 4).152 4).168 5.(S)BLR+BA Plasmid 5).061 5).063 5).062 6.(S)BLR+BA Plasmid+inducer 6).064 6).063 6).059

  • In order to continue experimentation I needed to streak new BLR and put the BA Operon into liquid media to use for tomorrow.


Vparker 01:49, 7 August 2007 (EDT)

  • Assay seemed to be missing something. I decided to reproduce the experiment but with new media.
  • grew new media and ran procedures for lypholization.


Vparker 01:49, 8 August 2007 (EDT)

  • Resuspended 1 mil of each flask and resuspended for transformation.
  • 6 plated in AMP(BLR+plasmids) 2 plated in agar(BLR only)


Vparker 01:49, 9 August 2007 (EDT)

  • No living colonies seen on any plate.

Vparker 01:49, 10 August 2007 (EDT)

  • Since i need to switch mid log media i will have to use Ptet strain as my new vector.
  • Need to ligate otsBA-TT to Ptet vector.
  • Did ligation then second digestion with Bam/Bgl.


Vparker 01:49, 12 August 2007 (EDT)

  • Came in this weekend to miniprep real fast and i took 5 colonies of Nhu's plates and put them into liquid media and then into the incibator.


Vparker 01:49, 13-17 August 2007 (EDT) After having successflly cloned my operons into Ptet strain. I realized that I have run out of time on my project over the summer. My conclusion is that indeed trehalose does help with dessication in biological organisms and that from my experiment my operon produced better from not having an inducer and plated at higher concentration rates. If my part of the project were continued I could have continued experimenting with the Ptet strain and eventually found a promoter and RBS site that would produce better results that would have more percentage the bacto-blood recover after having been freeze dried.

     It was a great experience for me over the summer and it was great working with all of the iGEM crew.