Team:Harvard/Template:NotebookDataJuly3

From 2011.igem.org

(Difference between revisions)
(Kan-ZFB-wp insertion)
(Transformation for OZ plasmids)
 
(4 intermediate revisions not shown)
Line 163: Line 163:
====Minipreps of colonies and controls====
====Minipreps of colonies and controls====
-
Our minipreps from [[#Colony minipreps|Saturday]] had low yields, especially for culture 85. We suspect this is why the PCR [[#Gel analysis of miniprep junction PCR|on Sunday]] did not work for this sample. Unfortunately, 85.3 and 85.4 did not grow even after being left in the shaker overnight. These were two cultures we made by picking new colonies from plate 85. This may have occurred because we did not actually pick the colony, or the colony was a cheater. Thus, we performed minipreps on 80.1, 80.2, 81.1, 81.4 (the controls, chosen for their wide range of concentrations after our first miniprep), and 85.1 and 85.2.  
+
Our minipreps from Saturday had low yields, especially for culture 85. We suspect this is why the PCR [[#Gel analysis of miniprep junction PCR on Sunday did not work for this sample. Unfortunately, 85.3 and 85.4 did not grow even after being left in the shaker overnight. These were two cultures we made by picking new colonies from plate 85. This may have occurred because we did not actually pick the colony, or the colony was a cheater. Thus, we performed minipreps on 80.1, 80.2, 81.1, 81.4 (the controls, chosen for their wide range of concentrations after our first miniprep), and 85.1 and 85.2.  
In order to figure our why our minipreps were resulting in unexpectedly low yields and increase our yields:
In order to figure our why our minipreps were resulting in unexpectedly low yields and increase our yields:
Line 180: Line 180:
====PCR of miniprep products====
====PCR of miniprep products====
-
We then ran a PCR for the cross-junction on all 6 (80.1, 80.2, 81.1, 81.4, 85.1, 85.2) samples, using [[#PCR of expression plasmid cross-junction|our usual cross junction protocol]].  
+
We then ran a PCR for the cross-junction on all 6 (80.1, 80.2, 81.1, 81.4, 85.1, 85.2) samples, using our usual cross junction protocol.  
{|
{|
Line 192: Line 192:
====Designing ultramers for Zif268, OZ052, and OZ123====
====Designing ultramers for Zif268, OZ052, and OZ123====
-
In preparation for designing our 96-well practice plate, we designed ultramers for our three positive controls Zif268, OZ052, and OZ123.  These ultramers contain the Type II binding sites as well as the F2/F3 fingers.  Since the [[Lab_Notebook#Design_of_Plate_Practice_Sequences|practice plate]] will contain oligos that encode for F1, we can use these three positive controls to practice and ensure that we secure the technique of using the Type II binding sites to swap in F1 into our expression plasmids.  The ultramers have not yet been ordered.
+
In preparation for designing our 96-well practice plate, we designed ultramers for our three positive controls Zif268, OZ052, and OZ123.  These ultramers contain the Type II binding sites as well as the F2/F3 fingers.  Since the practice plate will contain oligos that encode for F1, we can use these three positive controls to practice and ensure that we secure the technique of using the Type II binding sites to swap in F1 into our expression plasmids.  The ultramers have not yet been ordered.
===Team TolC===
===Team TolC===
Line 309: Line 309:
====Construction of OZ052 and OZ123: Joining the Finger with Homology regions====
====Construction of OZ052 and OZ123: Joining the Finger with Homology regions====
-
Previously, we did a PCR to [[Lab_Notebook:_July#Overlap_PCR_of_OZ052_and_OZ123|reassemble the ultramers]] for OZ052 and OZ123, but they only coded strictly for F1/F2/F3 and did not have any overhang homology with any surrounding code.  Thus, we performed PCR to add these homology overhangs so that we can integrate them with the omega subunit as well as the spec backbone to create a final expression plasmid.
+
Previously, we did a PCR to reassemble the ultramers for OZ052 and OZ123, but they only coded strictly for F1/F2/F3 and did not have any overhang homology with any surrounding code.  Thus, we performed PCR to add these homology overhangs so that we can integrate them with the omega subunit as well as the spec backbone to create a final expression plasmid.
The program we used was 55* annealing temperature, and a 15 second extension time.  Gel results pictured below.
The program we used was 55* annealing temperature, and a 15 second extension time.  Gel results pictured below.
Line 366: Line 366:
Our concentrations were better than they have been in the past; notably, after the addition of buffer P2, our solution actually turned a bright blue (indicating lysis of the cells), which we had not seen before.
Our concentrations were better than they have been in the past; notably, after the addition of buffer P2, our solution actually turned a bright blue (indicating lysis of the cells), which we had not seen before.
-
We then ran a PCR on our miniprep product, to check for our desired insert. We used our [[#PCR of expression plasmid cross-junction|usual protocol]] for a PCR of the expression plasmid cross-junction.   
+
We then ran a PCR on our miniprep product, to check for our desired insert. We used our usual protocol for a PCR of the expression plasmid cross-junction.   
{|
{|
Line 375: Line 375:
====Sending out our expression colonies for sequencing====
====Sending out our expression colonies for sequencing====
-
We sent out the samples from [[#Expression Plasmid Sequencing Results|yesterday]] that had no more than 1 SNP for reverse sequencing. In addition, we also sent out 78 and 79 for forward and reverse sequencing.  
+
We sent out the samples from yesterday that had no more than 1 SNP for reverse sequencing. In addition, we also sent out 78 and 79 for forward and reverse sequencing.  
*Reverse sequencing: 77.1, 77.3, 77.4, 78.1, 80.1, 80.2, 80.4, 81.1, 81.4, 82.1, 83.4, 84.1, 84.4, Zif268
*Reverse sequencing: 77.1, 77.3, 77.4, 78.1, 80.1, 80.2, 80.4, 81.1, 81.4, 82.1, 83.4, 84.1, 84.4, Zif268
*Forward and reverse sequencing: 781, 78.2, 78.3, 78.4, 79.1, 79.2, 79.3, 79.4
*Forward and reverse sequencing: 781, 78.2, 78.3, 78.4, 79.1, 79.2, 79.3, 79.4
Line 390: Line 390:
====Gel Extraction and Isothermal Assembly of OZ fingers+homology====
====Gel Extraction and Isothermal Assembly of OZ fingers+homology====
-
We ran a gel extraction of our PCR product from [[#Construction of OZ052 and OZ123: Joining the Finger with Homology regions|yesterday]], so that we could use it for isothermal assembly later.  Strangely, we got bands that were larger than our largest theoretical product.
+
We ran a gel extraction of our PCR product from yesterday, so that we could use it for isothermal assembly later.  Strangely, we got bands that were larger than our largest theoretical product.
{|
{|
Line 423: Line 423:
*Also replated the 7/20 lambda red culture to see if we can get any good cells (1.5mL).</div>
*Also replated the 7/20 lambda red culture to see if we can get any good cells (1.5mL).</div>
<div id="722" style="display:none">
<div id="722" style="display:none">
 +
==July 22nd==
==July 22nd==
===Team ZF===
===Team ZF===
Line 453: Line 454:
-
To this end, we redid the PCRs for everything in preparation for the resequencing, using the junction primers and [[#PCR of expression plasmid cross-junction|the previous protocol]].  The resulting gels can be observed below:
+
To this end, we redid the PCRs for everything in preparation for the resequencing, using the junction primers and the previous protocol.  The resulting gels can be observed below:
{|
{|
Line 468: Line 469:
====Transformation for OZ plasmids====
====Transformation for OZ plasmids====
-
Today, we took the results of the isothermal assembly from yesterday and did chemical transformation to introduce the plasmids into the Top 10 ChemComp bacteria, using [[Protocols#Cultures|our protocol for chemical transformations]]. They were left to recover for approximately 1.5 hours. We plated 2 dilutions, 10 ul and 50 ul, and left them overnight at 37* in the incubator.
+
Today, we took the results of the isothermal assembly from yesterday and did chemical transformation to introduce the plasmids into the Top 10 ChemComp bacteria, using [https://2011.igem.org/Team:Harvard/Protocols#Cultures our protocol for chemical transformations]. They were left to recover for approximately 1.5 hours. We plated 2 dilutions, 10 ul and 50 ul, and left them overnight at 37* in the incubator.
===Team Wolfe===
===Team Wolfe===

Latest revision as of 20:53, 4 August 2011