Team:Harvard/Template:NotebookDataAugust3

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(Created page with "<div style="display:none"> ==August 10== ===Team TolC=== =====MAGE OZ052 and OZ123===== *MAGE round 4a, time constants of 5.6s (OZ052) and 1.2s and 5.4s (OZ123). There appeared t...")
 
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==August 10==
==August 10==
===Team TolC===
===Team TolC===
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***numbered, from 1-6, 1-3 is colony 1, 4-6 is colony 2. 1,4=TT 2,5=RR, 3,6=ZR
***numbered, from 1-6, 1-3 is colony 1, 4-6 is colony 2. 1,4=TT 2,5=RR, 3,6=ZR
***PCR successful!! We have the real WN strain now. It should be ready for transformation tomorrow with the zif268 spec plasmid
***PCR successful!! We have the real WN strain now. It should be ready for transformation tomorrow with the zif268 spec plasmid
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[[File: 2011.08.10.WN1tt2rr3zrworks(labeled).png|thumb|none|Zeocin/rpoZ and TolC PCR of lambda red colonies 8/10/11]]
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[[File: HARV2011.08.10.WN1tt2rr3zrworks(labeled).png|thumb|none|Zeocin/rpoZ and TolC PCR of lambda red colonies 8/10/11]]
===Team Wolfe===
===Team Wolfe===
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'''Results'''
'''Results'''
*rpoZ was knocked out!
*rpoZ was knocked out!
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[[File: 2011.08.10.rpoz KO check(labeled).png|thumb|none|Zeocin/rpoZ PCR of lambda red colonies 8/10/11]]
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[[File: HARV2011.08.10.rpoz KO check(labeled).png|thumb|none|Zeocin/rpoZ PCR of lambda red colonies 8/10/11]]
*Reinoculated LB+zeo with culture 9 to use tomorrow for glycerol stocks and transformations
*Reinoculated LB+zeo with culture 9 to use tomorrow for glycerol stocks and transformations
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====Digestion of pSB4K5 Plasmid====
====Digestion of pSB4K5 Plasmid====
*Gel with yesterday's digestion product suggests that neither of the two restriction enzymes (Xba1 or Spe1) cut our plasmid. This was determined by comparing the band sizes to those obtained by midiporep of the pSB4K5 (whole) plasmid.
*Gel with yesterday's digestion product suggests that neither of the two restriction enzymes (Xba1 or Spe1) cut our plasmid. This was determined by comparing the band sizes to those obtained by midiporep of the pSB4K5 (whole) plasmid.
*Plan of action: We will use smaller reactions to increase the relative concentration of enzymes and we will use slightly more BSA buffer.
*Plan of action: We will use smaller reactions to increase the relative concentration of enzymes and we will use slightly more BSA buffer.
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[[File:2011.08.10.pSB4K5 digest(labeled).png|thumb|none|pSB4K5 digestion with Spe1  and Xba1]]
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[[File:HARV2011.08.10.pSB4K5 digest(labeled).png|thumb|none|pSB4K5 digestion with Spe1  and Xba1]]
'''Today's Digestion of pSB4K5 Plasmid'''
'''Today's Digestion of pSB4K5 Plasmid'''
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**1.5µL Spe1
**1.5µL Spe1
*Results: the size of the bands isn't what we expected (backbone should be ~3.4kb, insert ~1.2), but the comparison between the different digestions and the uncut plasmid does imply that the digestion we worked. We will go ahead and gel extract from the Spe+Xba digest and use both ligation and sequencing to be sure that this is indeed the plasmid we want.
*Results: the size of the bands isn't what we expected (backbone should be ~3.4kb, insert ~1.2), but the comparison between the different digestions and the uncut plasmid does imply that the digestion we worked. We will go ahead and gel extract from the Spe+Xba digest and use both ligation and sequencing to be sure that this is indeed the plasmid we want.
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[[File:2011.08.10.psb4k5 spexba digest(labeled).png|thumb|none|pSB4K5 digest with Spe1, Xba1, and both 8/10/11]]
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[[File:HARV2011.08.10.psb4k5 spexba digest(labeled).png|thumb|none|pSB4K5 digest with Spe1, Xba1, and both 8/10/11]]
===Team ZF===
===Team ZF===
====Mini library ligation results====
====Mini library ligation results====
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We checked our plates from our practice plate library assembly [[Lab_Notebook:_August#Practice_plate_oligo_pool|yesterday]], and we got colonies!!  Strangely, our 450 ul plate didn't have a huge number more colonies than the 50 ul plate.  Dan suggested that this was because we plated all the cells in a 450 ul volume, which may have sloshed around and taken cells with it.  Next time we should pellet the cells and resuspend in 100 ul and plate that.  Based on our colony numbers with 50 ul, we should probably plate with 100 ul in the future.
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We checked our plates from our practice plate library assembly yesterday, and we got colonies!!  Strangely, our 450 ul plate didn't have a huge number more colonies than the 50 ul plate.  Dan suggested that this was because we plated all the cells in a 450 ul volume, which may have sloshed around and taken cells with it.  Next time we should pellet the cells and resuspend in 100 ul and plate that.  Based on our colony numbers with 50 ul, we should probably plate with 100 ul in the future.
Due to the proliferation of colonies, we picked 90 colonies with the assistance of Will.  These 90 colonies should hopefully represent all 18 oligos in equal amounts.  We did colony PCRs on all 90 with the junction PCR protocol, and sent them out for sequencing today.  We saved these 90 colonies by adding LB/spec to each of the wells after suspending them in the 10 ul of water for the colony PCR.  We will eventually harvest and gather all 18 assembled plasmids from this step.
Due to the proliferation of colonies, we picked 90 colonies with the assistance of Will.  These 90 colonies should hopefully represent all 18 oligos in equal amounts.  We did colony PCRs on all 90 with the junction PCR protocol, and sent them out for sequencing today.  We saved these 90 colonies by adding LB/spec to each of the wells after suspending them in the 10 ul of water for the colony PCR.  We will eventually harvest and gather all 18 assembled plasmids from this step.
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====Library ligation optimization====
====Library ligation optimization====
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Dan suggests that we optimize the vector:insert ratio for our library assembly.  We will try using the following insert ratios (assuming a vector unit of 1): 1, 2, 3, 4, 8, 10, 16.  Unfortunately, today we did not have enough cut CB bottom plasmid to immediately begin the ligation and transformation, so we attempted to cut more CB bottom.  After performing a cut with Bsa-HF using the [[Lab_Notebook:_August#New_restriction_enzyme_protocol|previous protocol]], we performed a PCR purification on the product, only to find that there were only 3.4 ng/ul of cut plasmid present.  This is not enough to perform the ligation, and so we will have to try the CB bottom plasmid cut again tomorrow morning when the cultures have grown enough.  We can then do a ligation and transformation tomorrow and count colonies on Friday.
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Dan suggests that we optimize the vector:insert ratio for our library assembly.  We will try using the following insert ratios (assuming a vector unit of 1): 1, 2, 3, 4, 8, 10, 16.  Unfortunately, today we did not have enough cut CB bottom plasmid to immediately begin the ligation and transformation, so we attempted to cut more CB bottom.  After performing a cut with Bsa-HF using the previous protocol, we performed a PCR purification on the product, only to find that there were only 3.4 ng/ul of cut plasmid present.  This is not enough to perform the ligation, and so we will have to try the CB bottom plasmid cut again tomorrow morning when the cultures have grown enough.  We can then do a ligation and transformation tomorrow and count colonies on Friday.
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As stated in the earlier section, we should probably plate 100 ul of transformed bacteria to standardize everything and to keep colony counting fairly manageable.
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As stated in the earlier section, we should probably plate 100 ul of transformed bacteria to standardize everything and to keep colony counting fairly manageable.</div>
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<div id='811' style="display:none">
==August 11th==
==August 11th==
===Team Wolfe===
===Team Wolfe===
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*Since colonies are not near mid-log we may have to fill plate reader tomorrow and run then as well
*Since colonies are not near mid-log we may have to fill plate reader tomorrow and run then as well
====Gradient Plates====
====Gradient Plates====
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*Created 5 50 mL total gradient plates with 2x Kan in the wedge layer, 20ul of Bluejuice in each 25ml of LB+agar+Kan to mark it with a dye.
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*Created 5 50 mL total gradient plates with 2x Kan in the wedge layer, 20ul of Bluejuice in each 25ml of LB+agar+Kan to mark it with a dye.</div>
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==August 12th==
==August 12th==
===Team Wolfe===
===Team Wolfe===
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**Team ZF's "CJUN" protocol: pZE23G 2123R and pZE23G 3581F primers
**Team ZF's "CJUN" protocol: pZE23G 2123R and pZE23G 3581F primers
**Note well 5 is fainter but is probably due to a loading error where a small volume of sample was left out.
**Note well 5 is fainter but is probably due to a loading error where a small volume of sample was left out.
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[[File: 2011.08.12.cjun(labeled).png|thumb|none|EcNR2 selection strain colonies transformed with zif268 8/12/11]]
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[[File: HARV2011.08.12.cjun(labeled).png|thumb|none|EcNR2 selection strain colonies transformed with zif268 8/12/11]]
====Selection strain genotype confirmation====
====Selection strain genotype confirmation====
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====Isothermal assembly and transformation of GFP reporter====
====Isothermal assembly and transformation of GFP reporter====
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We ran our PCR product from [[#PCR to get out GFP| yesterday]] on a 1% agarose gel. We got an appropriate band at approximately 700 bp. (Unfortunately, we could not get the imaging software to work at the time, so no image is available)
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We ran our PCR product from yesterday on a 1% agarose gel. We got an appropriate band at approximately 700 bp. (Unfortunately, we could not get the imaging software to work at the time, so no image is available)
We performed a gel extraction on our GFP PCR product, with the following yields:
We performed a gel extraction on our GFP PCR product, with the following yields:
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====CB Bottom Digestion====
====CB Bottom Digestion====
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We digested our CB Bottom plasmid, using our usual recipe. We ran the digestion for 2 hours at 37*, 20 minutes at 65*, and then let the reaction sit at 4* overnight.
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We digested our CB Bottom plasmid, using our usual recipe. We ran the digestion for 2 hours at 37*, 20 minutes at 65*, and then let the reaction sit at 4* overnight.</div>
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====Western Blot results====
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==August 13th==
==August 13th==
===Team ZF===
===Team ZF===
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Combined with the sequencing results from [[#Check oligo pool sequencing results|before]], we are missing oligos 3, 13, 14, and 16.
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Combined with the sequencing results from before, we are missing oligos 3, 13, 14, and 16.
====Results of GFP transformation====
====Results of GFP transformation====
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====PCR purification of CB Bottom digestion product====
====PCR purification of CB Bottom digestion product====
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We performed a PCR purification on the CB Bottom digestion, with a yield of 68.96 ng/ul and a 260/280 of 1.85. This will be used in a ligation in the future.
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We performed a PCR purification on the CB Bottom digestion, with a yield of 68.96 ng/ul and a 260/280 of 1.85. This will be used in a ligation in the future.</div>
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==August 15==
==August 15==
===TolC===
===TolC===
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Yay!!!
Yay!!!
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[[File: 3AT.png|thumb|none|Selection strain with and without plasmid, and 3-AT 8/12/11]]
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[[File: HARV3AT.png|thumb|none|Selection strain with and without plasmid, and 3-AT 8/12/11]]
Interestingly, our 5-FOA concentrations did not seem very potent: 3-AT was more effective at retarding growth. We might drop the URA3 part of our selection and instead use higher amounts of 3-AT to distinguish between true hits and false positives.
Interestingly, our 5-FOA concentrations did not seem very potent: 3-AT was more effective at retarding growth. We might drop the URA3 part of our selection and instead use higher amounts of 3-AT to distinguish between true hits and false positives.
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[[File: 2011.08.12.EcNR2 3AT+5FOA.png|thumb|left|Selection strain without Zif268 with 3-AT and 5-FOA 8/12/11]]
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[[File: HARV2011.08.12.EcNR2 3AT+5FOA.png|thumb|left|Selection strain without Zif268 with 3-AT and 5-FOA 8/12/11]]
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[[File: 2011.08.12.Zif1 3AT+5FOA.png|thumb|none|Selection strain with Zif268 with 3-AT and 5-FOA 8/12/11]]
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[[File: HARV2011.08.12.Zif1 3AT+5FOA.png|thumb|none|Selection strain with Zif268 with 3-AT and 5-FOA 8/12/11]]</div>
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==August 16==
==August 16==
In prioritizing our work for the next two weeks, we decided to focus on three main experiments:
In prioritizing our work for the next two weeks, we decided to focus on three main experiments:

Latest revision as of 22:30, 19 September 2011