Team:BYU Provo/Notebook/CholeraDetection/Springexp/Period1/Dailylog

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| colspan="3" | <font color="#333399" size="5" font face="Calibri"> '''Cholera Detection May - June Notebook: July 1 - July 7 Daily Log'''</font>
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: '''Cholera Detection May-June Notebook: May 1 - May 14 Daily Log'''</font>
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: [[Team:BYU_Provo/Cholera_-_Detection|Overview]]
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: <u> '''Cholera Detection''' </u> </font>
: [[Team:BYU Provo/Notebook/Cholera_-_Detection/Winterexp|March-April]]
: [[Team:BYU Provo/Notebook/Cholera_-_Detection/Winterexp|March-April]]
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<font size="4"> '''9/4/2013''' </font>
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<font size="4"> '''5/1/2013''' </font>
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BYU iGEM can count on every member, now that summer is over and all are again enrolled in classes. We took time at the beginning of class to list our main projects (aside from research itself) from here on out: they include cloning our parts into the iGEM backbone plasmid, filming a synthetic biology techniques video to collaborate with another team, finishing the website, and publishing our synthetic biology Children's Book and collecting data to demonstrate that children who read it and the included parental guide improve their understanding of science generally and synthetic biology in particular.
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KK Over the break we did little Lab work. Kelton was in Rexburg, and Clarice and I didn’t have the necessary primers to continue working. Today the primers came! We submitted primers for all the genes that have been cloned into pIG78 with pIG78 for sequencing. (I believe we included the primers for all the genes). We also have primers for working with CRO in the pBAD plasmid.
 +
Today our assignment was to make goals and set plans for what we hope to accomplish by the end of the term. Our plans are to be submitted by Friday. Our plans are spelled out in a table we’re printing, but they include understanding (via sequencing) what is ocurring in the plasmid by May 13th, correcting our system by May 29th, and demonstrating that we can induce Lambda into lysis through expression CRO. We will place CRO on the pBAD plasmid with the pBAD promoter (or on pLAT with a pBAD promoter), and the pBAD promoter is induced by arabinose.
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Kelton and I are responsible to see the book published, and the data collected.  We set ourselves the following deadlines:
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KP Today we were trained in Cholera handling safety and we made our plans and goals for a summer full of success.  
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Sep. 8th: Have in our possession the edited, shaded version of the book.  Redge (the illustrator) confirmed that he would finish by Sunday the 8th.
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Sep. 11th: Submit the book for publishing.
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Sep. 20th: Distribute paper copies/pdf copies to elementary school teachers and parents.  Children will be given a pre test before reading the book, and later a post test.  The test results will allow us to quantifiably show that our book improves understanding of synthetic biology among young children.
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Sep. 25th: Compile and analyze the data.
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Several weeks ago, I read a paper indicating that lysogenic lambda is induced to lysis by host cell recognition of AHL's, the molecules used in bacterial quorum sensing systems. I thought that our bacterial strain with the Lambda lysogen, TT9907, might recognize cholera's autoinducer, and perhaps that might trigger Lambda. I streaked a line of TT9907 next to cholera and then away from cholera. No bacteria grew next to cholera, but the strain did grow away from cholera! Now, we need to show that it is indeed lambda that is killing the cell and not some toxin from cholera.
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CHFirst day of new semester. Our First assignment is due Friday which is a detailed plan for the semester. Need to think about the web page and register for the team. Explained the whole process of plasmid modification to Kendal and Kelton. Figured out plan to modify pLat (pIG12 or pIG13) so that cro will be inserted right after pBAD (using restriction sites PstI and ecoRI).
 +
List of primers we are using for sequencing:
 +
IG11- pLat MCS forward
 +
BI219- hap rev.
 +
BI220- GFP for.
 +
BI222-GFP rev.
 +
BI225- RFP for.
 +
BI227- Qrr4 rev.
 +
BI228- Lux O for.
 +
BI229- Lux U rev.
 +
BI230- CqsS for.
 +
BI247- CqsS rev. middle
 +
BI248- LuxO for. middle
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We designed an experiment with 6 bacterial strains: 2 without the lambda lysogen, 1 with the lambda lysogen, and three that may have the lambda lysogen. The latter three strains are each from single colonies that grew following an electroporation procedure to get TT9907 to take up the plasmid pIG87. Amazingly, top agar lawn assays with a drop of hydrogen peroxide added to stress lambda into lysis show that after electroporation, there are no plaques.  Either Lambda gets out during electroporation or TT9907 loses its susceptibility to lambda. Anyway, we took these six strains and streaked a line of them next to a patch of cholera and away from the patch. Depending on how the bacteria grow we'll be able to say if cholera (perhaps some toxin) kills TT9907 or lambda kills TT9907.
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<font size="4"> '''5/3/13''' </font>
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KP Today Kendall and I did PCR for the first time. Jordan and Clarice showed us how to do it. We did PCR on our E. Coli that has our lysogenic lambda encased within. We also froze down our lambda e. coli samples for future use.
 +
 
 +
KK Kelton and I worked with Jordan today to PCR amplify the CRO gene from π9907-infected E.Coli. We boiled the E.Coli to use as template and then followed the PCR protocol as outlined. Jordan actually was performed most of the protocol so that we could learn. Our control was E.Coli that had not been infected with lambda.
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<br>
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<font size="4"> '''5/6/13''' </font>
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We ran a gel of our PCR product that we had created over the weekend. This was the first time I had ever done so, so it was fun and interesting! To make the gel, we mix 100 mL of TAE buffer with 1 gram of agar and heat in the microwave. The agar powder needs to completely dissolve. That mixture, with ethidium bromide, is added to the gel dock, and let set for about 20 minutes, or if you set the gel in the fridge it is a little less time.
 +
The CRO gene is about 300 base pairs. However, when we ran our PCR product against the ladder and against our negative control, our PCR product matched the control and did NOT match the length that indicates 300 base pairs. So, we know that our PCR reaction failed. It may be because we used a colony that did not include that lambda prophage.
 +
 
 +
Today we did the PCR reaction to amplify CRO again, but this time we amplified CRO from colonies that had been infected with our three distinct strains of Lambda. We will check our product tomorrow.
KK, KP
KK, KP
 +
 +
PCR amplified Cro from one of our lamda phage ecoli. It didn’t give us a product so we need to redo it. Froze down lamda phage Ecoli strains in -80. (220ul DMSO added to 1.3ml saturated overnight culture)
 +
IGM46 = 23281
 +
IGM47 =9901
 +
IGM48 =9907
 +
Figured out that the vector we need for our Cro insert is pIG12 or pIG13. Obtained this strain from the -80. Did PCR clean up on the PCRs we set up last time turns out no good. Redid the PCR this time having a reaction for each of the three strains (IGM46, IGM47, and IGM48) and a control.
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 +
CH
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<font size="4"> '''9/6/13''' </font>
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<font size="4"> '''5/8/13''' </font>
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Our results from the side-by-side plate comparison of cholera with several strains of bacteria are encouraging!  We grew a patch of V. cholerae for one week on LB plates. Then, we streaked a line of a bacteria adjacent to the patch and another away from the patch.  We did this for six different strains on six different plates.  None of the bacterial strains plated adjacent to cholera grew.  All strains grew away from cholera.  However, TT9907, the strain with lambda lysogen, showed plaques! There were distinct plaques on the line of bacteria leading away from Cholera. Through what we believe is a quorum sensing pathway, the lambda lysogen recognizes that E.Coli has detected cholera.  It mobilizes excision from the genome, replicates, and lyses it's host.
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We prepared top agar lawns of our 6 strains, with cholera plated in the middle, to show more clearly the result we saw today.
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We did a few different procedures today. We started out by doing a PCR purification for BI7701, BI7707, and BI23.... It was successful, but our concentration was very low (11.9). We also set up another PCR for BI7701, BI7707, and BI23... It will be done tomorrow. Today we also did a digest of our plasmid and our cro insert.
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Clarice transformed the iGEM backbone into E.Coli and grew it up in an overnight. From those cells we isolated the plasmid, pIG91, in two Eppendorfs, at concentrations of 52 ng/uL and 82 ng/uL. Monday we will digest the plasmid and the SdiA gene to splice it in and submit to the registry.
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Having confirmed that our CRO insert was indeed PCR amplified (see picture above; very faint lines about 500 base pairs; wells 1-3 represent three strains of lambda, while 4 is a negative control), we performed a PCR cleanup on ALL 3 of our samples, in an attempt to isolate concentration of CRO insert possible. On the spectrophotometer our A260 reading gave us a concentration of 11.9 ng/microL.  
 +
Following that we ran a digest of our CRO insert and pLAT plasmid with pBAD promoter using restriction enzymes PST1-HF and ECOR1-HF. Our pLAT sample was a mixture of pIG12 and pIG13, which according to the parts database are the same plasmid, taken from two different colonies.
 +
Having set our vector and inserts to digest, we started a low-melt gel with Jordan’s help. Low melt gels follow a slightly different protocol than normal gels, and use a smaller dock. Our dock was broken so our gel didn’t set very well. Because we don’t have time today, tomorrow we’ll run our vector and insert on the low-melt gel to see what happens.
 +
KK, KP
 +
Our PCR from last time gave us very dim bands as products so we did PCR clean up and added all three of the samples together into one column. We also set up restriction digests for the cleaned PCR insert of Cro and for the plasmid pIG13 with pstI and ecoRI. This should place the Cro insert right after pBAD in pIG13. I also worked a bunch on the QS construct updating the primers document from last year and working on a document that has the sequence for the entire construct as it should appear in pJG78. Need to redo sequencing for the primers BI222, BI227, and BI247.
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CH
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<br>
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<font size="4"> '''5/9/13''' </font>
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Our low melt gel had holes in the bottom of the first few wells, so the already low-concentration plasmid was diluted between 4 wells. Our vector’s well was viable, and the vector stayed in the well.
KK, KP
KK, KP
 +
 +
<br>
 +
 +
<font size="4"> '''5/10/13''' </font>
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We were able to cut out our vector from the low melt gel, but our insert was not visible. So, today, we made preparations to run our CRO insert on a low melt gel again. I made the low melt gel and set it to cool, and to remain in the fridge over the weekend. Kelton and Clarice performed the PCR cleanup of a second CRO insert PCR reaction that we ran. The PCR was more successful this time - the bands were much more clearly visible, in all three of our Lambda samples (see the photo that Kelton will upload).
 +
 +
Today we did a PCR cleanup on our Cro PCR products. We also set up a slow melt gel so we can try again on Monday to get a cutout of the insert in order to combine our plasmid and insert. We already have the plasmid, we just have to wait on the insert because it wasn’t visible in our first slow melt gel. Here is a picture of our second PCR product run on a 1 kb ladder gel:
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KK, KP,CH
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 +
CH 5/13/13
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Set up ligations for pIG12/13 + Cro both treated with pstI and ecoRI. Figured out the primers we need for sequencing the region where cro will be inserted (IG57 and IG58).
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<br>
{{TeamBYUProvoFooter}}
{{TeamBYUProvoFooter}}

Latest revision as of 23:03, 27 September 2013


Cholera Detection May-June Notebook: May 1 - May 14 Daily Log



Cholera Detection
March-April
May-June
July-August
September-October

5/1/2013

KK Over the break we did little Lab work. Kelton was in Rexburg, and Clarice and I didn’t have the necessary primers to continue working. Today the primers came! We submitted primers for all the genes that have been cloned into pIG78 with pIG78 for sequencing. (I believe we included the primers for all the genes). We also have primers for working with CRO in the pBAD plasmid. Today our assignment was to make goals and set plans for what we hope to accomplish by the end of the term. Our plans are to be submitted by Friday. Our plans are spelled out in a table we’re printing, but they include understanding (via sequencing) what is ocurring in the plasmid by May 13th, correcting our system by May 29th, and demonstrating that we can induce Lambda into lysis through expression CRO. We will place CRO on the pBAD plasmid with the pBAD promoter (or on pLAT with a pBAD promoter), and the pBAD promoter is induced by arabinose.

KP Today we were trained in Cholera handling safety and we made our plans and goals for a summer full of success.

CHFirst day of new semester. Our First assignment is due Friday which is a detailed plan for the semester. Need to think about the web page and register for the team. Explained the whole process of plasmid modification to Kendal and Kelton. Figured out plan to modify pLat (pIG12 or pIG13) so that cro will be inserted right after pBAD (using restriction sites PstI and ecoRI). List of primers we are using for sequencing: IG11- pLat MCS forward BI219- hap rev. BI220- GFP for. BI222-GFP rev. BI225- RFP for. BI227- Qrr4 rev. BI228- Lux O for. BI229- Lux U rev. BI230- CqsS for. BI247- CqsS rev. middle BI248- LuxO for. middle



5/3/13

KP Today Kendall and I did PCR for the first time. Jordan and Clarice showed us how to do it. We did PCR on our E. Coli that has our lysogenic lambda encased within. We also froze down our lambda e. coli samples for future use.

KK Kelton and I worked with Jordan today to PCR amplify the CRO gene from π9907-infected E.Coli. We boiled the E.Coli to use as template and then followed the PCR protocol as outlined. Jordan actually was performed most of the protocol so that we could learn. Our control was E.Coli that had not been infected with lambda.


5/6/13

We ran a gel of our PCR product that we had created over the weekend. This was the first time I had ever done so, so it was fun and interesting! To make the gel, we mix 100 mL of TAE buffer with 1 gram of agar and heat in the microwave. The agar powder needs to completely dissolve. That mixture, with ethidium bromide, is added to the gel dock, and let set for about 20 minutes, or if you set the gel in the fridge it is a little less time. The CRO gene is about 300 base pairs. However, when we ran our PCR product against the ladder and against our negative control, our PCR product matched the control and did NOT match the length that indicates 300 base pairs. So, we know that our PCR reaction failed. It may be because we used a colony that did not include that lambda prophage.

Today we did the PCR reaction to amplify CRO again, but this time we amplified CRO from colonies that had been infected with our three distinct strains of Lambda. We will check our product tomorrow.

KK, KP

PCR amplified Cro from one of our lamda phage ecoli. It didn’t give us a product so we need to redo it. Froze down lamda phage Ecoli strains in -80. (220ul DMSO added to 1.3ml saturated overnight culture) IGM46 = 23281 IGM47 =9901 IGM48 =9907 Figured out that the vector we need for our Cro insert is pIG12 or pIG13. Obtained this strain from the -80. Did PCR clean up on the PCRs we set up last time turns out no good. Redid the PCR this time having a reaction for each of the three strains (IGM46, IGM47, and IGM48) and a control.

CH


5/8/13

We did a few different procedures today. We started out by doing a PCR purification for BI7701, BI7707, and BI23.... It was successful, but our concentration was very low (11.9). We also set up another PCR for BI7701, BI7707, and BI23... It will be done tomorrow. Today we also did a digest of our plasmid and our cro insert.

Having confirmed that our CRO insert was indeed PCR amplified (see picture above; very faint lines about 500 base pairs; wells 1-3 represent three strains of lambda, while 4 is a negative control), we performed a PCR cleanup on ALL 3 of our samples, in an attempt to isolate concentration of CRO insert possible. On the spectrophotometer our A260 reading gave us a concentration of 11.9 ng/microL. Following that we ran a digest of our CRO insert and pLAT plasmid with pBAD promoter using restriction enzymes PST1-HF and ECOR1-HF. Our pLAT sample was a mixture of pIG12 and pIG13, which according to the parts database are the same plasmid, taken from two different colonies. Having set our vector and inserts to digest, we started a low-melt gel with Jordan’s help. Low melt gels follow a slightly different protocol than normal gels, and use a smaller dock. Our dock was broken so our gel didn’t set very well. Because we don’t have time today, tomorrow we’ll run our vector and insert on the low-melt gel to see what happens. KK, KP

Our PCR from last time gave us very dim bands as products so we did PCR clean up and added all three of the samples together into one column. We also set up restriction digests for the cleaned PCR insert of Cro and for the plasmid pIG13 with pstI and ecoRI. This should place the Cro insert right after pBAD in pIG13. I also worked a bunch on the QS construct updating the primers document from last year and working on a document that has the sequence for the entire construct as it should appear in pJG78. Need to redo sequencing for the primers BI222, BI227, and BI247. CH


5/9/13

Our low melt gel had holes in the bottom of the first few wells, so the already low-concentration plasmid was diluted between 4 wells. Our vector’s well was viable, and the vector stayed in the well. KK, KP


5/10/13

We were able to cut out our vector from the low melt gel, but our insert was not visible. So, today, we made preparations to run our CRO insert on a low melt gel again. I made the low melt gel and set it to cool, and to remain in the fridge over the weekend. Kelton and Clarice performed the PCR cleanup of a second CRO insert PCR reaction that we ran. The PCR was more successful this time - the bands were much more clearly visible, in all three of our Lambda samples (see the photo that Kelton will upload).

Today we did a PCR cleanup on our Cro PCR products. We also set up a slow melt gel so we can try again on Monday to get a cutout of the insert in order to combine our plasmid and insert. We already have the plasmid, we just have to wait on the insert because it wasn’t visible in our first slow melt gel. Here is a picture of our second PCR product run on a 1 kb ladder gel: KK, KP,CH

CH 5/13/13 Set up ligations for pIG12/13 + Cro both treated with pstI and ecoRI. Figured out the primers we need for sequencing the region where cro will be inserted (IG57 and IG58).