Team:BYU Provo/Notebook/Cholera - Enzyme/September/Period1/Dailylog
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- | : | + | <font color="#333399" size="3" font face="Calibri"> |
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+ | <font size = "4"> | ||
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+ | : <u> '''Cholera Enzyme''' </u> </font> | ||
: [[Team:BYU Provo/Notebook/Cholera - Enzymes/March-April|March-April]] | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/March-April|March-April]] | ||
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: [[Team:BYU Provo/Notebook/Cholera - Enzymes/July-August|July-August]] | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/July-August|July-August]] | ||
- | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/September-October|September]] | + | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/September-October|September-October]] |
+ | |||
+ | : [[Team:BYU Provo/Notebook/Cholera - Enzymes/Protocols|Protocols]] | ||
</font> | </font> | ||
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- | + | <u>Protocol</u> | |
#Pellet 1-5 mL of overnight culture of recombinant E. coli culture by centrifugation at ≥ 12,000 × g for one minute. Resuspend pellet in 200 uL of provided Resuspension Solution. | #Pellet 1-5 mL of overnight culture of recombinant E. coli culture by centrifugation at ≥ 12,000 × g for one minute. Resuspend pellet in 200 uL of provided Resuspension Solution. | ||
#Lyse resuspended cells by adding 200 uL of Lysis solution. Immediately mix contents by gentle inversion 6-8 times, until the mixture becomes clear and viscous. Allow the Lysis reaction to proceed for approximately two minutes, but do not exceed five minutes. | #Lyse resuspended cells by adding 200 uL of Lysis solution. Immediately mix contents by gentle inversion 6-8 times, until the mixture becomes clear and viscous. Allow the Lysis reaction to proceed for approximately two minutes, but do not exceed five minutes. | ||
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#Qrr4/RFP PCR | #Qrr4/RFP PCR | ||
#piG91 miniprep | #piG91 miniprep | ||
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- | + | As well we set up phusion and Taq PCR for B. subtilis and phusion PCR for dspB | |
<u>Phusion PCR setup</u> | <u>Phusion PCR setup</u> | ||
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1 microliter diluted template DNA | 1 microliter diluted template DNA | ||
.5 microliter phusion polymerase | .5 microliter phusion polymerase | ||
- | + | ||
<br> | <br> | ||
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<font size="4"> '''9/5/2013''' </font> | <font size="4"> '''9/5/2013''' </font> | ||
- | I ran the PCR products from 9/4 on gel | + | I ran the PCR products from 9/4 on gel. There were no viable products. |
<br> | <br> | ||
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<font size="4"> '''9/6/2013''' </font> | <font size="4"> '''9/6/2013''' </font> | ||
- | + | We set up PCRs with Desi with a variety of conditions to test all of the primers that we have been using and the new primers for the iGem plasmid backbone for both DspB and Savinase. This will allow us to see if the DNA templates that we are using are viable or not. If some of the PCRs work, but not all of them, then we know that the problem is with our primers, not the DNA templates we are using. | |
- | - | + | |
+ | <br> | ||
+ | |||
+ | <font size="4"> '''9/9/2013''' </font> | ||
+ | |||
+ | We ran our PCR products from 9/6 on gel and got no results on any of them. This clearly shows that our DNA templates themselves are not viable. We will need to get new DNA templates to use for our DspB and Savinase. We ordered genomic DNA from Arabidopsis thaliana, which contains the DspB gene. We will also try to get purified Bacillus subtilis DNA from Dr. Robison's lab. | ||
+ | |||
+ | We set up new cholera overnights, seeding them with 50 ul of our previous overnights in 4 mL of SLB, and placed them in the 30°C incubator. | ||
+ | |||
+ | We set up sequencing on several of the Savinase and AmyA plasmids to check them: | ||
+ | 1. Savinase - Colony B with Forward primer | ||
+ | 2. Savinase - Colony B with Reverse primer | ||
+ | 3. Savinase - Colony D with Forward primer | ||
+ | 4. Savinase - Colony D with Reverse primer | ||
+ | 5. AmyA - Clone A with Forward primer | ||
+ | 6. AmyA - Clone A with Forward primer | ||
+ | 7. AmyA - Clone B1 with Forward primer | ||
+ | 8. AmyA - Clone B1 with Reverse primer | ||
+ | 9. AmyA - Clone B2 with Forward primer | ||
+ | 10. AmyA - Clone B2 with Reverse primer | ||
+ | 11. AmyA - Clone C with Forward primer | ||
+ | 12. AmyA - Clone C with Reverse primer | ||
+ | |||
+ | <br> | ||
+ | |||
+ | <font size="4"> '''9/11/2013''' </font> | ||
+ | |||
+ | We got the sequencing results back on our Savinase and AmyA plasmids from 9/9. None of the Savinase plasmids sequenced with our primers, indicating that none of the plasmids took up our target gene. AmyA Clone A had the best sequencing results of the AmyA plasmids, we will use this clone for our future work in cloning AmyA into the iGem backbone plasmid. | ||
+ | |||
+ | We worked today on getting our AmyA and DspB genes cloned into the iGem backbone plasmid. We set up PCRs for AmyA and Savinase using the following:<br> | ||
+ | <u>PCR Protocol</u> | ||
+ | 70 uL ddH20 | ||
+ | 20 uL 5X Phusion Buffer | ||
+ | 3 uL 10 mM dNTPs | ||
+ | 2 uL Forward primer | ||
+ | 2 uL Reverse primer | ||
+ | 1 uL Phusion polymerase | ||
+ | 2 uL template DNA | ||
+ | |||
+ | <u>Primers</u> | ||
+ | DspB Forward - BI258 | ||
+ | DspB Reverse - BI259 | ||
+ | AmyA Forward - BI260 | ||
+ | AmyA Reverse - BI268 | ||
+ | |||
+ | <br> | ||
+ | |||
+ | <font size="4">'''9/12/13'''</font> | ||
+ | |||
+ | We ran our PCR products from yesterday out on gel, the AmyA didn't work at all. We will have to check those primers and rerun the PCR for that. | ||
+ | |||
+ | We ran plasmid preps on Savinase Colony B and Colony D to see if we can get any kind of product out of them. See protocol page for protocol followed. We then set up PCRs using the purified plasmid prep as our template DNA, but when we ran it out on gel there wasn't any product. Our plasmids containing Savinase are completely unusable. | ||
+ | |||
+ | <br> | ||
+ | |||
+ | <font size="4">'''9/13/13'''</font> | ||
+ | |||
+ | We ran plasmid preps of the pIG91 and pJG648 plasmids. We then ran the digest for them and ran plate transformations in LB + CAM for AmyA/pIG91 Upper, AmyA/pIG91 lower, and DspB/pIG91. We then transformed DspB into pJG648, plated it to LB + AMP, and put it in the 37°C incubator. All work was done following the protocols listed on the protocols page. | ||
+ | |||
+ | We also purified our DspB and AmyA proteins today following the procedure listed on the protocols page. The purified proteins were placed in the -80°C freezer until ready for use. | ||
+ | |||
+ | <br> | ||
</font> | </font> |
Latest revision as of 21:09, 27 September 2013
Cholera - Enzymes Notebook: September 1 - September 14 Daily Log
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9/4/13 Today we set up new overnights of cholera by adding 4 mL of SLB and 50 uL of our previous overnight from 8/26/13 into a test tubes and placing in the 30° incubator overnight. We prepared two overnight cultures and one control.
Restriction Digest setup 7.5 uL H2O 4.0 uL Buffer 4 4.0 uL 10x BSA 20 uL DNA template 1.5 uL Xba 1 1.5 uL Spe 1 Digests Labelled
Phusion PCR setup 35 microliters ddH2O 10 microliters 5X phusion buffer 1.5 microliters 10mM dNTP's 1 microliter each primer 1 microliter diluted template DNA .5 microliter phusion polymerase Taq PCR setup 40 microliters ddH2O 5 microliters 10X TAQ buffer 1.5 microliters 10mM dNTP's 1 microliter each primer 1 microliter diluted template DNA .5 microliter phusion polymerase
9/5/2013 I ran the PCR products from 9/4 on gel. There were no viable products.
9/6/2013 We set up PCRs with Desi with a variety of conditions to test all of the primers that we have been using and the new primers for the iGem plasmid backbone for both DspB and Savinase. This will allow us to see if the DNA templates that we are using are viable or not. If some of the PCRs work, but not all of them, then we know that the problem is with our primers, not the DNA templates we are using.
9/9/2013 We ran our PCR products from 9/6 on gel and got no results on any of them. This clearly shows that our DNA templates themselves are not viable. We will need to get new DNA templates to use for our DspB and Savinase. We ordered genomic DNA from Arabidopsis thaliana, which contains the DspB gene. We will also try to get purified Bacillus subtilis DNA from Dr. Robison's lab. We set up new cholera overnights, seeding them with 50 ul of our previous overnights in 4 mL of SLB, and placed them in the 30°C incubator. We set up sequencing on several of the Savinase and AmyA plasmids to check them: 1. Savinase - Colony B with Forward primer 2. Savinase - Colony B with Reverse primer 3. Savinase - Colony D with Forward primer 4. Savinase - Colony D with Reverse primer 5. AmyA - Clone A with Forward primer 6. AmyA - Clone A with Forward primer 7. AmyA - Clone B1 with Forward primer 8. AmyA - Clone B1 with Reverse primer 9. AmyA - Clone B2 with Forward primer 10. AmyA - Clone B2 with Reverse primer 11. AmyA - Clone C with Forward primer 12. AmyA - Clone C with Reverse primer
9/11/2013 We got the sequencing results back on our Savinase and AmyA plasmids from 9/9. None of the Savinase plasmids sequenced with our primers, indicating that none of the plasmids took up our target gene. AmyA Clone A had the best sequencing results of the AmyA plasmids, we will use this clone for our future work in cloning AmyA into the iGem backbone plasmid. We worked today on getting our AmyA and DspB genes cloned into the iGem backbone plasmid. We set up PCRs for AmyA and Savinase using the following: 70 uL ddH20 20 uL 5X Phusion Buffer 3 uL 10 mM dNTPs 2 uL Forward primer 2 uL Reverse primer 1 uL Phusion polymerase 2 uL template DNA Primers DspB Forward - BI258 DspB Reverse - BI259 AmyA Forward - BI260 AmyA Reverse - BI268
9/12/13 We ran our PCR products from yesterday out on gel, the AmyA didn't work at all. We will have to check those primers and rerun the PCR for that. We ran plasmid preps on Savinase Colony B and Colony D to see if we can get any kind of product out of them. See protocol page for protocol followed. We then set up PCRs using the purified plasmid prep as our template DNA, but when we ran it out on gel there wasn't any product. Our plasmids containing Savinase are completely unusable.
9/13/13 We ran plasmid preps of the pIG91 and pJG648 plasmids. We then ran the digest for them and ran plate transformations in LB + CAM for AmyA/pIG91 Upper, AmyA/pIG91 lower, and DspB/pIG91. We then transformed DspB into pJG648, plated it to LB + AMP, and put it in the 37°C incubator. All work was done following the protocols listed on the protocols page. We also purified our DspB and AmyA proteins today following the procedure listed on the protocols page. The purified proteins were placed in the -80°C freezer until ready for use.
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