Talk:Team:IvyTech-South Bend

From 2010.igem.org

(Difference between revisions)
 
(63 intermediate revisions not shown)
Line 5: Line 5:
<body>
<body>
-
         <!-- Begin Header -->
+
          
 +
<!-- Begin Header -->
         <div id="header">
         <div id="header">
<p>  
<p>  
-
<img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/IvyTechLogo.png" align="left"><img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/igem1.png" align="left"><img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/2010.png" align="left"><img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/sb.png" align="left">
+
<img src="https://static.igem.org/mediawiki/2010/2/2d/IvyTech-South_Bend_logo.png" align="left"><img src="https://static.igem.org/mediawiki/2010/7/76/Igem1.png" align="left"><a href="https://2010.igem.org/Team:IvyTech-South_Bend/Team">
 +
<img src="https://static.igem.org/mediawiki/2010/d/d7/2010.png"align="left"></a><img src="https://static.igem.org/mediawiki/2010/a/a3/Sb.png" align="left">
<br clear="all">
<br clear="all">
     <p/>
     <p/>
<p>  
<p>  
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/home.png"></a>   
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend"> <img src="https://static.igem.org/mediawiki/2010/f/f3/Home1.png" width=12%></a>   
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Team"> <img src="team.http://bob.ivytech.edu/~rchamberlin1/IGEM/png"></a>     
+
 
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Project"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/project.png"></a>    
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Project"> <img src="https://static.igem.org/mediawiki/2010/5/58/Image-_SBProject.PNG" width=11%></a>     
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Parts"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/parts.png"></a>  
+
<width=80%><a href="https://2010.igem.org/Team:IvyTech-South_Bend/Parts"> <img src="https://static.igem.org/mediawiki/2010/7/79/Parts.png" width=15%></a>  
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Modeling"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/modeling.png"></a>
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Modeling"> <img src="https://static.igem.org/mediawiki/2010/0/0b/Image-SBModeling.PNG" width=11%></a>
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Notebook"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/notebook.png"></a>
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Notebook"> <img src="https://static.igem.org/mediawiki/2010/9/95/Notebook.png" width=11%></a>
-
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Saftey"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/safety.png"></a>
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Safety"> <img src="https://static.igem.org/mediawiki/2010/8/84/Safety.png" width=11%></a>
-
<a href="https://2010.igem.org/Talk:Team:IvyTech-South_Bend"> <img src="http://bob.ivytech.edu/~rchamberlin1/IGEM/plan.png"></a>
+
<a href="https://2010.igem.org/Talk:Team:IvyTech-South_Bend"> <img src="https://static.igem.org/mediawiki/2010/f/f7/Plan.png" width=12%></a>
-
<p/>
+
-
 
+
<a href="https://2010.igem.org/Team:IvyTech-South_Bend/Team"><img src="https://static.igem.org/mediawiki/2010/3/32/Team.png" width=12%></a>  
-
</div>
+
        <p/>
-
<!-- End Header -->
+
              </div>
 +
             
 +
<a href="https://2010.igem.org/wiki/index.php?title=Talk:Team:IvyTech-South_Bend&action=edit&section=new"><size=4><b> Add an Entry </b></size></a>
 +
 
 +
 
 +
<!-- End Header -->
</body>
</body>
</html>  
</html>  
Line 30: Line 37:
 +
{|align="left" width=500px id="template" style="text-align: center; font-weight: bold; font-size: large; color: #f6f6f6; padding: 5px;
-
{|align="justify"
+
== 6/14/10 TWADDLE ==
-
|== 6/14/10 TWADDLE ==
+
-
In summary we have decided to pursue a mercury sequesting IGEM to be built from available parts, possibly. 1) Mercury transporter K205044 2) a glutathione part: possibly BBa_J61213 BBa_T20205 BBa_K289001 BBa_K289002 BBa_K289003... Our task is to evaluate the gluthione parts for one that we can couple to the mercury transporter:
+
In summary we have decided to pursue a mercury sequesting IGEM to be built from available parts, possibly. 1) Mercury transporter K205044 2) a glutathione part: possibly BBa_J61213 BBa_T20205 BBa_K289001 BBa_K289002 BBa_K289003... Our task is to evaluate the gluthione parts for one that we can couple to the mercury transporter:
-
-|
+
 
-
|== 6/21/10 TWADDLE ("da coach") ==
+
== 6/21/10 TWADDLE ("da coach") ==
O.k. summary of our change of direction:
O.k. summary of our change of direction:
Line 42: Line 49:
Since we have found some good examples of IGEMs that have been created to detect and/or sequester heavy metals we decided to shift gears and build a IGEM that can detect enteric bacteria:  The idea is to build a device that can be use to sense bacteria in lake water.  Lake Michigan beaches are susceptible to closure because of high E.coli counts.  If we could develop an IGEM based upon the quorum sensing protein, autoinducer 2, the we could detect, indirectly the presence, even potentially the amount of bacteria in the water.
Since we have found some good examples of IGEMs that have been created to detect and/or sequester heavy metals we decided to shift gears and build a IGEM that can detect enteric bacteria:  The idea is to build a device that can be use to sense bacteria in lake water.  Lake Michigan beaches are susceptible to closure because of high E.coli counts.  If we could develop an IGEM based upon the quorum sensing protein, autoinducer 2, the we could detect, indirectly the presence, even potentially the amount of bacteria in the water.
-
|== 6/21/10 Joseph Hull(Joe) ==
+
== 6/21/10 Joseph Hull(Joe) ==
-
How about we use the British Columbia 2009 stop light bacteria device by manipulating this device with a AI-1 or AHL promoter to change this device to be sensitive to presence of AI-1
+
How about we use the British Columbia 2009 stop light bacteria device by manipulating this device with a  
 +
AI-1 or AHL promoter to change this device to be sensitive to presence of AI-1
-
|== 6/21/10 Chamberlin ("da geek") ==
+
== 6/21/10 Chamberlin ("da geek") ==
Possible promoter LuxR is a constitutively expressed protein that can bind AHL. When bound to AHL it can stimulate transcription from the right hand lux promoter (pLuxR). In the natural system, this promoter controls transcription of the LuxI enzyme leading to a positive feedback loop that increases transcription from the right hand lux promoter. In addition controlling the transcription of luxI, the promoter also controls transcription of luciferase. 1 BBa_R1062Promoter, Standard (luxR and HSL regulated -- lux pR)
Possible promoter LuxR is a constitutively expressed protein that can bind AHL. When bound to AHL it can stimulate transcription from the right hand lux promoter (pLuxR). In the natural system, this promoter controls transcription of the LuxI enzyme leading to a positive feedback loop that increases transcription from the right hand lux promoter. In addition controlling the transcription of luxI, the promoter also controls transcription of luciferase. 1 BBa_R1062Promoter, Standard (luxR and HSL regulated -- lux pR)
-
|}
+
 
 +
 
 +
== 6/23/10 Cassidy ==
 +
 
 +
If we're going for the AHL aspect like Joe proposed what about checking into the utilization of...
 +
 
 +
Part:BBa_I729004 (DNA AVAILABLE/EXPERIENCE: NONE) Sensitive AHL Receiver This AHL receiver contains mutant LuxR.(I45F) It can express GFP more at AHL 10nM compared with wild type. (Ref. Collins, C. H., Arnold, F. H. & Leadbetter, J. R. Directed evolution of Vibrio fischeri LuxR for increased sensitivity to a broad spectrum of acyl-homoserine lactones. Mol. Microbiol. 55, 712–723 (2005))
 +
 
 +
or maybe...
 +
 
 +
 
 +
Part:BBa_I729005 (DNA AVAILABLE/EXPERIENCE: WORKS!) AHL Reporter and Quencher GFP and aiiA are repressed Lux promoter GFP and aiiA induced by AHL. GFP will express if the amount of AHL exeed the capability of aiiA.
 +
 
 +
== LB plates plus antibiotics - Joice P==
 +
 
 +
"**Be sure agar is not to hot Cool to 55 degrees C. before starting procedure if agar is hot**"
 +
 
 +
1)Ampicillin- add 1 ml ampicillin (at 100 mg/ml) per liter of agar to obtain a final concentration of 100 ug/ml. Can mark with red line to signify amp.
 +
 
 +
2)Kanamycin- add 1ml kanamycin stock (at 50 mg/ml) per liter of agar to obtain a final concentration of 50 ug/ml. Can mark with green line to signify Kanamycin.
 +
 
 +
3) Tetracycline- add 1ml tetracycline stock (at 15 mg/ml)per liter of agar to obtain a final concentration of 15 ug/ml.Can mark with black line to signify tetracycline.
 +
 
 +
4)Chloramphenicol-add 1ml chloramphenicol stock (at 25 mg/ml)per liter of agar to obtain a final concentration of 100 ug/ml. Can mark plates with a single purple line to signify chloramphenicol.
 +
 
 +
--[[User:Joice2872|Joice2872]] 19:37, 30 June 2010 (UTC)
 +
 
 +
== How to determine volumes to obtain a certain concentration Joice P ==
 +
 
 +
Use the following formula to determine amount of stock solution to use for any amount. Buy make sure units match!!
 +
'''C'''1'''V'''1 ='''C'''2 '''V'''2 so '''C''' = concentration and '''V''' = volume
 +
To convert mg/ml to ug/ml multiply by 1000
 +
 
 +
 
 +
An example: stock solution of A at 100 mg/ml. You want 150 ml at 100 ug/ml. Use the '''C'''1'''V'''1 for what you want, and the '''C'''2'''V'''2 for what you have.
 +
Just Plug n Chug. (100 ug/ml)(150ml) = (100000 ug/ml)(x)
 +
15000=100000x
 +
 
 +
x = 0.15ml, or 150 ul (again remember you have to convert mg/ml to ug/ml, by multiplying by 1000)--
 +
 
 +
--[[User:Joice2872|Joice2872]] 19:38, 30 June 2010 (UTC)
 +
 
 +
== 6/28/10 Joseph Hull(Joe)  ==
 +
 
 +
Preparing SOB-
 +
SOB BROTH(DRY MEDIA) CatNo. S0221  Lot: S022130D0901
 +
 
 +
Scale: Mad by Adventurer Pro AV64
 +
s/n: 8030391129  Error+ .67%
 +
Calibrated by Cassidy
 +
 
 +
 
 +
1) I used 4 - 250 mL capped elenmyer flasks
 +
 
 +
2) in two of them I added 6.97 grams of SOB media powder to 250 mL DI water
 +
 
 +
3)the mixed and dissolved on the hot plate
 +
 
 +
4) once dissolved, I separated the 2 - 250 mL SOB media into 4 - 250 mL elenmyer flasks and autocalved for one hour
 +
 
 +
== Richard Lab:Electroporation of E. coli  ==
 +
 
 +
This protocol is for the typical electro-transformation of E. coli done in the Richard Lab.
 +
 
 +
The consensus electroporation protocol should be consulted if deviating from the procedure outlined here.
 +
Procedure
 +
 
 +
1. Chill the # electroporation cuvettes by floating them in an ice bath.
 +
 
 +
2. Remove # vials containing 100μl electro-competent cells from the -80°C freezer and thaw them with the iced cuvettes.
 +
 
 +
3. Prepare # micro-centrifuge tubes containing 900μl SOB media.
 +
 
 +
4. Turn on electroporator and set voltage to either 1.25 kV (1mm cuvettes).
 +
 
 +
5. Add add 5μL of ligated DNA sample to 100μl thawed electrocompetent cells on ice. Swirl tip around gently in cells to mix DNA and cells.
 +
 
 +
6. Place cells back on ice to ensure they remain cold.
 +
 
 +
7. Pippette 100μL of cell-DNA mixture to cuvette.
 +
 
 +
8. Wipe off excess moisture from outside of cuvette.
 +
 
 +
9. Place cuvette in chamber of electroporator.
 +
 
 +
10. Pulse the cells by pressing button on electroporator twice.
 +
 
 +
11. Quickly use a pipette to remove the electroporated cell suspension from the cuvette and add it to a tubes containing 1ml SOB.
 +
 
 +
12. Let cells recover at room temperature for 30-60 minutes.
 +
 
 +
13. Plate 100μl of eletroporated cells onto prewarmed LB-agar plate supplemented with appropriate antibiotic. Incubate plate overnight at 37°C.
 +
 
 +
--[[User:Rchamberlin|Rchamberlin]] 19:59, 30 June 2010 (UTC)
 +
 
 +
== Big Picture Revisited ==
 +
 
 +
So, am I correct in summarizing:
 +
 
 +
We are going to marry the BC stoplight/jammer device(s) with a device that is sensitive to AL2.
 +
 
 +
It may be possible to put this into E.coli, even though E.coli is making and sensitive to AL2: E.coli grown in dilute solution (plantonic form) should be green and as the concentration of bacteria, AL2, rises actually, then the color of the bacteria should shift from green to yellow to red.  That of course is the ideal.
 +
 
 +
We could also build an AHL sensitive system but that will set us up to detect another type of bacteria....--[[User:Geotwaddle|Geotwaddle]] 20:11, 30 June 2010 (UTC)
 +
 
 +
== New idea? ==
 +
 
 +
Can we merry stoplight idea with the AL2 sensor? New idea??--[[User:Joice2872|Joice2872]] 20:02, 7 July 2010 (UTC)
 +
 
 +
== pGlo transformation successful ==
 +
 
 +
Our bacteria did take up the pglo plasmid after I placed 1 mL on LB amp/ara plate. We will now continue by transforming and cell banking more bacteria with the pglo plasmids while we await parts from the registry.
 +
--[[User:Joice2872|Joice2872]] 18:53, 21 July 2010 (UTC)
 +
 
 +
== Parts Needed and Found ==
 +
 
 +
We have identified 4 parts that we will need for the project.
 +
Two parts are in the 2010 distributions:
 +
 
 +
''' Plate 2 - 20A 
 +
BBa_I729006'''
 +
 
 +
(pSB1A3)AHL reporter and aiia device
 +
 
 +
T9002
 +
S01656
 +
 +
Express LuxR and aiiA constantly. AiiA degrades AHL as signaling molecule. Express GFP when the AHL concentration exceed the capacity of aiiA,.
 +
 
 +
'''Plate 1 - 1F
 +
BBa_I13453'''
 +
 
 +
(pSB1A3)Pbad promoter
 +
 
 +
I13453
 +
 +
PBad promoter from I0500 without AraC.
 +
Usage and Biology
 +
Has been used as a second promoter in a system containing BBa_I0500 (PBad+AraC). In this system, it showed behavior qualitatively indistinguishable from the BBa_I0500 copy of PBad. Has not been tested independent of AraC. A second part, BBa_I13458, should allow decoupling of PBad and AraC.
 +
See this OpenWetWare article on pBAD and lac promoters for additional usage and biology information
 +
Characterization
 +
For the 2009 iGEM competition, British_Columbia characterized BBa_I13453 in the context of a pBAD promoter family. For the results of this characterization, see here.
 +
 +
I have asked Professor T to order  '''pBAD strong BBa_K206000''' and '''pBAD weak BBa_K206001''' that were submitted by British Columbia 2009.
 +
 
 +
--[[User:Rchamberlin|Rchamberlin]] 12:13, 22 July 2010 (UTC)
 +
 
 +
Plasmids
 +
From partsregistry.org
 +
 
 +
< Back to Catalog
 +
 
 +
Plasmids are circular, double-stranded DNA molecules typically containing a few thousand base pairs that replicate within the cell independently of the chromosomal DNA. Plasmid DNA is easily purified from cells, manipulated using common lab techniques and incorporated into cells. Most BioBrick parts in the Registry are maintained and propagated on plasmids. Thus, construction of BioBrick parts, devices and systems usually requires working with plasmids.
 +
 
 +
Note: In the Registry, plasmids are made up of two distinct components:
 +
 
 +
1. the BioBrick part, device or system that is located in the BioBrick cloning site, between (and excluding) the BioBrick prefix and suffix.
 +
2. the plasmid backbone which propagates the BioBrick part. The plasmid backbone is defined as the sequence beginning with the BioBrick suffix, including the replication origin and antibiotic resistance marker, and ending with the BioBrick prefix. [Note that the plasmid backbone itself can be composed of BioBrick parts.]
 +
 
 +
Many BioBrick parts in the Registry are maintained on more than one plasmid backbone!
 +
To construct, assemble, or operate BioBrick parts, you are probably looking for a plasmid backbone ... not a plasmid. Please go to the Plasmid backbones collection to see all available plasmid backbones.
 +
 
 +
However, the Registry does have a small collection of plasmids. These are largely legacy parts and not useful for construction of BioBrick parts, devices and systems. However, we include them here for completeness.
 +
 
 +
--[[User:Rchamberlin|Rchamberlin]] 19:07, 28 July 2010 (UTC)
 +
 
 +
== Usage and extraction ==
 +
 
 +
Usage
 +
 
 +
The Distribution Kit Plates contain dried DNA of hundreds of parts that are available in the Registry up to 2009. While there is not enough DNA for assembly, you will be able to transform the DNA into cells and then make your own glycerol stocks of any part that you wish.
 +
[edit] Linearized Plasmid Backbone Instructions
 +
 
 +
In addition to the DNA plates the Distribution Kit also contains a set of linearized plasmid backbones:
 +
 
 +
    * pSB1C3
 +
    * pSB1T3
 +
    * pSB1A3
 +
 
 +
These plasmid backbones have been prepared via PCR and purified. All you need to do is cut with EcoRI, PstI and DpnI to leave two ends ready to be ligated to a Biobrick™ part. Use these backbones to send your parts to the Registry when shipping your parts before the Jamboree.
 +
 
 +
    * NOTE: The linearized plasmid backbones need to be cut by EcoRI and PstI restriction enzymes prior to use.
 +
 
 +
 
 +
You can find instructions on how to use AND make your own linearized plasmid backbones on the protocol page.
 +
[edit] DNA Kit Plate Instructions
 +
 
 +
To use the DNA in the Distribution Kit you may follow these instructions:
 +
 
 +
1. With a pipette tip, punch a hole through the foil cover into the corresponding well to the Biobrick™-standard part that you want. Make sure you have properly oriented the plate. We recommend that you do not remove the foil cover, as it could lead to cross contamination between the wells.
 +
 
 +
2. Add 10uL of diH2O (deionized water)
 +
 
 +
3. Pipette 1 or 2uL of the resuspended DNA transform into your desired competent cells, plate bacteria with the appropriate antibiotic* and grow overnight.
 +
 
 +
4. Pick a single colony and inoculate broth (again, with the correct antibiotic) and grow for 18 hours.
 +
 
 +
5. Use the resulting culture to miniprep the DNA AND make your own glycerol stock (for further instruction on making a glycerol see this page). We recommend using the miniprepped DNA to run QC tests, such as restriction digests and sequencing.
 +
 
 +
* To know which antibiotics to use, look at the plasmid that the part is in. The naming scheme for plasmids is specifically designed to indicate antibiotic resistance.
 +
 
 +
--[[User:Rchamberlin|Rchamberlin]] 19:51, 28 July 2010 (UTC)
 +
 
 +
== AHL Promoter ==
 +
 
 +
Hello Twaddle. Will this work?
 +
http://partsregistry.org/partsdb/get_part.cgi?part=BBa_K131010
 +
--[[User:DonKuyk|DonKuyk]] 20:22, 9 August 2010 (UTC)

Latest revision as of 19:43, 7 October 2010

Add an Entry


Contents

6/14/10 TWADDLE

In summary we have decided to pursue a mercury sequesting IGEM to be built from available parts, possibly. 1) Mercury transporter K205044 2) a glutathione part: possibly BBa_J61213 BBa_T20205 BBa_K289001 BBa_K289002 BBa_K289003... Our task is to evaluate the gluthione parts for one that we can couple to the mercury transporter:

6/21/10 TWADDLE ("da coach")

O.k. summary of our change of direction:

Since we have found some good examples of IGEMs that have been created to detect and/or sequester heavy metals we decided to shift gears and build a IGEM that can detect enteric bacteria: The idea is to build a device that can be use to sense bacteria in lake water. Lake Michigan beaches are susceptible to closure because of high E.coli counts. If we could develop an IGEM based upon the quorum sensing protein, autoinducer 2, the we could detect, indirectly the presence, even potentially the amount of bacteria in the water.

6/21/10 Joseph Hull(Joe)

How about we use the British Columbia 2009 stop light bacteria device by manipulating this device with a AI-1 or AHL promoter to change this device to be sensitive to presence of AI-1

6/21/10 Chamberlin ("da geek")

Possible promoter LuxR is a constitutively expressed protein that can bind AHL. When bound to AHL it can stimulate transcription from the right hand lux promoter (pLuxR). In the natural system, this promoter controls transcription of the LuxI enzyme leading to a positive feedback loop that increases transcription from the right hand lux promoter. In addition controlling the transcription of luxI, the promoter also controls transcription of luciferase. 1 BBa_R1062Promoter, Standard (luxR and HSL regulated -- lux pR)



6/23/10 Cassidy

If we're going for the AHL aspect like Joe proposed what about checking into the utilization of...

Part:BBa_I729004 (DNA AVAILABLE/EXPERIENCE: NONE) Sensitive AHL Receiver This AHL receiver contains mutant LuxR.(I45F) It can express GFP more at AHL 10nM compared with wild type. (Ref. Collins, C. H., Arnold, F. H. & Leadbetter, J. R. Directed evolution of Vibrio fischeri LuxR for increased sensitivity to a broad spectrum of acyl-homoserine lactones. Mol. Microbiol. 55, 712–723 (2005))

or maybe...


Part:BBa_I729005 (DNA AVAILABLE/EXPERIENCE: WORKS!) AHL Reporter and Quencher GFP and aiiA are repressed Lux promoter GFP and aiiA induced by AHL. GFP will express if the amount of AHL exeed the capability of aiiA.

LB plates plus antibiotics - Joice P

"**Be sure agar is not to hot Cool to 55 degrees C. before starting procedure if agar is hot**"

1)Ampicillin- add 1 ml ampicillin (at 100 mg/ml) per liter of agar to obtain a final concentration of 100 ug/ml. Can mark with red line to signify amp.

2)Kanamycin- add 1ml kanamycin stock (at 50 mg/ml) per liter of agar to obtain a final concentration of 50 ug/ml. Can mark with green line to signify Kanamycin.

3) Tetracycline- add 1ml tetracycline stock (at 15 mg/ml)per liter of agar to obtain a final concentration of 15 ug/ml.Can mark with black line to signify tetracycline.

4)Chloramphenicol-add 1ml chloramphenicol stock (at 25 mg/ml)per liter of agar to obtain a final concentration of 100 ug/ml. Can mark plates with a single purple line to signify chloramphenicol.

--Joice2872 19:37, 30 June 2010 (UTC)

How to determine volumes to obtain a certain concentration Joice P

Use the following formula to determine amount of stock solution to use for any amount. Buy make sure units match!! C1V1 =C2 V2 so C = concentration and V = volume To convert mg/ml to ug/ml multiply by 1000


An example: stock solution of A at 100 mg/ml. You want 150 ml at 100 ug/ml. Use the C1V1 for what you want, and the C2V2 for what you have. Just Plug n Chug. (100 ug/ml)(150ml) = (100000 ug/ml)(x) 15000=100000x

x = 0.15ml, or 150 ul (again remember you have to convert mg/ml to ug/ml, by multiplying by 1000)--

--Joice2872 19:38, 30 June 2010 (UTC)

6/28/10 Joseph Hull(Joe)

Preparing SOB- SOB BROTH(DRY MEDIA) CatNo. S0221 Lot: S022130D0901

Scale: Mad by Adventurer Pro AV64 s/n: 8030391129 Error+ .67% Calibrated by Cassidy


1) I used 4 - 250 mL capped elenmyer flasks

2) in two of them I added 6.97 grams of SOB media powder to 250 mL DI water

3)the mixed and dissolved on the hot plate

4) once dissolved, I separated the 2 - 250 mL SOB media into 4 - 250 mL elenmyer flasks and autocalved for one hour

Richard Lab:Electroporation of E. coli

This protocol is for the typical electro-transformation of E. coli done in the Richard Lab.

The consensus electroporation protocol should be consulted if deviating from the procedure outlined here. Procedure

1. Chill the # electroporation cuvettes by floating them in an ice bath.

2. Remove # vials containing 100μl electro-competent cells from the -80°C freezer and thaw them with the iced cuvettes.

3. Prepare # micro-centrifuge tubes containing 900μl SOB media.

4. Turn on electroporator and set voltage to either 1.25 kV (1mm cuvettes).

5. Add add 5μL of ligated DNA sample to 100μl thawed electrocompetent cells on ice. Swirl tip around gently in cells to mix DNA and cells.

6. Place cells back on ice to ensure they remain cold.

7. Pippette 100μL of cell-DNA mixture to cuvette.

8. Wipe off excess moisture from outside of cuvette.

9. Place cuvette in chamber of electroporator.

10. Pulse the cells by pressing button on electroporator twice.

11. Quickly use a pipette to remove the electroporated cell suspension from the cuvette and add it to a tubes containing 1ml SOB.

12. Let cells recover at room temperature for 30-60 minutes.

13. Plate 100μl of eletroporated cells onto prewarmed LB-agar plate supplemented with appropriate antibiotic. Incubate plate overnight at 37°C.

--Rchamberlin 19:59, 30 June 2010 (UTC)

Big Picture Revisited

So, am I correct in summarizing:

We are going to marry the BC stoplight/jammer device(s) with a device that is sensitive to AL2.

It may be possible to put this into E.coli, even though E.coli is making and sensitive to AL2: E.coli grown in dilute solution (plantonic form) should be green and as the concentration of bacteria, AL2, rises actually, then the color of the bacteria should shift from green to yellow to red. That of course is the ideal.

We could also build an AHL sensitive system but that will set us up to detect another type of bacteria....--Geotwaddle 20:11, 30 June 2010 (UTC)

New idea?

Can we merry stoplight idea with the AL2 sensor? New idea??--Joice2872 20:02, 7 July 2010 (UTC)

pGlo transformation successful

Our bacteria did take up the pglo plasmid after I placed 1 mL on LB amp/ara plate. We will now continue by transforming and cell banking more bacteria with the pglo plasmids while we await parts from the registry. --Joice2872 18:53, 21 July 2010 (UTC)

Parts Needed and Found

We have identified 4 parts that we will need for the project. Two parts are in the 2010 distributions:

Plate 2 - 20A BBa_I729006

(pSB1A3)AHL reporter and aiia device

T9002 S01656

Express LuxR and aiiA constantly. AiiA degrades AHL as signaling molecule. Express GFP when the AHL concentration exceed the capacity of aiiA,.

Plate 1 - 1F BBa_I13453

(pSB1A3)Pbad promoter

I13453

PBad promoter from I0500 without AraC. Usage and Biology Has been used as a second promoter in a system containing BBa_I0500 (PBad+AraC). In this system, it showed behavior qualitatively indistinguishable from the BBa_I0500 copy of PBad. Has not been tested independent of AraC. A second part, BBa_I13458, should allow decoupling of PBad and AraC. See this OpenWetWare article on pBAD and lac promoters for additional usage and biology information Characterization For the 2009 iGEM competition, British_Columbia characterized BBa_I13453 in the context of a pBAD promoter family. For the results of this characterization, see here.

I have asked Professor T to order pBAD strong BBa_K206000 and pBAD weak BBa_K206001 that were submitted by British Columbia 2009.

--Rchamberlin 12:13, 22 July 2010 (UTC)

Plasmids From partsregistry.org

< Back to Catalog

Plasmids are circular, double-stranded DNA molecules typically containing a few thousand base pairs that replicate within the cell independently of the chromosomal DNA. Plasmid DNA is easily purified from cells, manipulated using common lab techniques and incorporated into cells. Most BioBrick parts in the Registry are maintained and propagated on plasmids. Thus, construction of BioBrick parts, devices and systems usually requires working with plasmids.

Note: In the Registry, plasmids are made up of two distinct components:

1. the BioBrick part, device or system that is located in the BioBrick cloning site, between (and excluding) the BioBrick prefix and suffix. 2. the plasmid backbone which propagates the BioBrick part. The plasmid backbone is defined as the sequence beginning with the BioBrick suffix, including the replication origin and antibiotic resistance marker, and ending with the BioBrick prefix. [Note that the plasmid backbone itself can be composed of BioBrick parts.]

Many BioBrick parts in the Registry are maintained on more than one plasmid backbone! To construct, assemble, or operate BioBrick parts, you are probably looking for a plasmid backbone ... not a plasmid. Please go to the Plasmid backbones collection to see all available plasmid backbones.

However, the Registry does have a small collection of plasmids. These are largely legacy parts and not useful for construction of BioBrick parts, devices and systems. However, we include them here for completeness.

--Rchamberlin 19:07, 28 July 2010 (UTC)

Usage and extraction

Usage

The Distribution Kit Plates contain dried DNA of hundreds of parts that are available in the Registry up to 2009. While there is not enough DNA for assembly, you will be able to transform the DNA into cells and then make your own glycerol stocks of any part that you wish. [edit] Linearized Plasmid Backbone Instructions

In addition to the DNA plates the Distribution Kit also contains a set of linearized plasmid backbones:

   * pSB1C3
   * pSB1T3
   * pSB1A3 

These plasmid backbones have been prepared via PCR and purified. All you need to do is cut with EcoRI, PstI and DpnI to leave two ends ready to be ligated to a Biobrick™ part. Use these backbones to send your parts to the Registry when shipping your parts before the Jamboree.

   * NOTE: The linearized plasmid backbones need to be cut by EcoRI and PstI restriction enzymes prior to use. 


You can find instructions on how to use AND make your own linearized plasmid backbones on the protocol page. [edit] DNA Kit Plate Instructions

To use the DNA in the Distribution Kit you may follow these instructions:

1. With a pipette tip, punch a hole through the foil cover into the corresponding well to the Biobrick™-standard part that you want. Make sure you have properly oriented the plate. We recommend that you do not remove the foil cover, as it could lead to cross contamination between the wells.

2. Add 10uL of diH2O (deionized water)

3. Pipette 1 or 2uL of the resuspended DNA transform into your desired competent cells, plate bacteria with the appropriate antibiotic* and grow overnight.

4. Pick a single colony and inoculate broth (again, with the correct antibiotic) and grow for 18 hours.

5. Use the resulting culture to miniprep the DNA AND make your own glycerol stock (for further instruction on making a glycerol see this page). We recommend using the miniprepped DNA to run QC tests, such as restriction digests and sequencing.

  • To know which antibiotics to use, look at the plasmid that the part is in. The naming scheme for plasmids is specifically designed to indicate antibiotic resistance.

--Rchamberlin 19:51, 28 July 2010 (UTC)

AHL Promoter

Hello Twaddle. Will this work? http://partsregistry.org/partsdb/get_part.cgi?part=BBa_K131010 --DonKuyk 20:22, 9 August 2010 (UTC)