Team:HKUSTers/Project

From 2008.igem.org

(Difference between revisions)
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! Name of test !! Purpose !! Circuit involved
! Name of test !! Purpose !! Circuit involved
|-
|-
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| T7 polymease proudction test || Check the T7 polymease production circuit using IPTG as inducer and GFP as  reporter || [[Image:T7_production_test.PNG]] ||  
+
| T7 polymease production test || Check the T7 polymease production circuit using IPTG as inducer and GFP as  reporter || [[Image:T7_production_test.PNG]] ||  
|-
|-
| GFP test || Check if the intact T7 promoter and GFP is functional|| [[Image:GFP_test.PNG]] ||  
| GFP test || Check if the intact T7 promoter and GFP is functional|| [[Image:GFP_test.PNG]] ||  
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| Adjacent bidirectional promoters test || Evaluate if two promoters in opposite directions can function properly if they are placed adjacently  || [[Image:Adj_promoters_test.png]] ||  
| Adjacent bidirectional promoters test || Evaluate if two promoters in opposite directions can function properly if they are placed adjacently  || [[Image:Adj_promoters_test.png]] ||  
|-
|-
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| Truncated promoter test || Stimulate the condition in the overlapped version, where the first two non-essential base pairs of cl434 promoter are altered. We want to know if the cl434 can still function under such condition.|| [[Image:Truncated_promoter_test.PNG]] ||  
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| Truncated promoter test || Stimulate the condition in the overlapped version, where the first two non-essential base pairs of cl434 promoter are altered. We want to know if the cl434 can still function under such conditions.|| [[Image:Truncated_promoter_test.PNG]] ||  
|-
|-
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| Left/right induction test || To see weather the overlapped promoter can be driven to both directions || [[Image:Left_right_test.png‎]]  ||  
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| Left/right induction test || To see whether the overlapping promoter can drive transcription of both directions || [[Image:Left_right_test.png‎]]  ||  
|}
|}
===Strain and vector used===
===Strain and vector used===
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* '''Strain''': ''e. coli'' BBa_V1001  DH5a, with genotype  
+
* '''Strain''': ''E. coli'' BBa_V1001  DH5a, with genotype  
   F-φ80dlacZΔM15 Δ(lacZYA-argF)U169 deoR recA1 endA1 hsdR17(rk- mk+ phoA supE44 λ- thi-1 gyrA96 relA1)
   F-φ80dlacZΔM15 Δ(lacZYA-argF)U169 deoR recA1 endA1 hsdR17(rk- mk+ phoA supE44 λ- thi-1 gyrA96 relA1)
* '''Vector''': pUC18+ λ-''InCh''2
* '''Vector''': pUC18+ λ-''InCh''2
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The advantages of this approach include:
The advantages of this approach include:
* No risk of >1 copy of target gene in our machine, so as to give a sharp output instead of "blurred" output caused by multiple copies
* No risk of >1 copy of target gene in our machine, so as to give a sharp output instead of "blurred" output caused by multiple copies
-
* Stable integration of a single copy of the plasmid fragment
+
* Stable integration of a single copy of the construct DNA fragment
-
* Most ordinary ''e. coli'' strains and a variety of pBR322-derived Amp-resistant plasmid can be used  
+
* Most ordinary ''E. coli'' strains and a variety of pBR322-derived Amp-resistant plasmids can be used  
* λ-phage as the only specialized vector required
* λ-phage as the only specialized vector required
-
* Source: λ ''InCh'' a simple E.Coli plasmid-chromosome shuttle system Boyd, D., Weiss, D. S., Chen, J. C. & Beckwith, J
+
* Source:  
 +
Boyd D., Weiss D.S., Chen J.C., Beckwith J.,
 +
Towards single-copy gene expression systems making gene cloning physiologically relevant: Lambda InCh, a simple Escherichia coli plasmid- chromosome shuttle system
 +
(2000) Journal of Bacteriology, 182 (3), pp. 842-847.

Revision as of 22:42, 29 October 2008

HK Harbour-1-2.jpg


Randomness.JPG


Randomness is everywhere!

381184220 4cfce0c86a.jpg

You may not have realized it, but randomness is very important even outside the casino. It plays an important role in mathematics, statistics, engineering, computer science and even medicine. Randomness is often needed in reducing bias. Here are some examples of natural occuring random events:

  • Random motions of molecules that explains phenomena in thermodynamics and properties of gases
  • Random genetic mutations that lead to diversity of life and makes natural selection possible

True Randomness?

There are various scientific or social areas in which randomness is required for fair analysis. When random numbers are needed, they are usually generated by computers. The computers may use information say, time, and long complicated mathematical processes to generate the number. So, is this true randomness?? The result may actually just be determined by the time at which the generation is kicked start. It is still not absolutely random.

Therefore, we have decided to design a . . .

Name ran3.jpg

This is going to be biologists' random generator. It is not just a biological slot machine, but a random number generator. The cell will have an either 0 or 1 state. By using more than 1 cell, a multi-digit binary number can be generated. The results cannot be controlled or altered by humans. It is true randomness!!! (yes, ideally)


The Design

"Making the dice"

We "tell" our cells to start making the "dice"--T7 polymease by applying a pulse of IPTG. IPTG can activate the araC/pBAD promoter which leads to transcription of T7 promoter.

IPTG.PNG width=400 height=78

"Throwing the dice"


T7P2.jpg
The core part of the randomizer consists of a pair of overlapping T7 promoters having similar binding affinities. The T7 polymerase binds absolutely randomly onto either the left or the right promoter to give an either 0 or 1 signal eventually, i.e. a mutually exclusive binding event. There are two operators on the sides of the promoters, they are c1434 and TetR operators.

Reciprocal inhibiton

Then there are TetR and C1434 repressor repressor genes on both sides respectively. A repressor protein can be produced to interrupt transcription on the other side of the circuit. For example, say, the T7 polymerase binds onto the promoter on the left side. The TetR repressor on the left, which was coded by TetR repressor gene, will bind to TetR operator on the right and repress transcription of right side of the promoter. Thus, the intial random event (binding of polymease) can be captured and amplified in a postive feedback circuit.
HKUSTers mutual repression.PNG

Final outcome

  • Continous production of GFP if the polymease binds to the left of overlapped T7 promoter
  • Continous production of RFP if the polymease binds to the right of overlapped T7 promoter

Greenred.jpg
The signal output is shown by green or red fluorescent protein (GFP/RFP) respectively.




Construction details

Testing

Testing of the components of circuit
Name of test Purpose Circuit involved
T7 polymease production test Check the T7 polymease production circuit using IPTG as inducer and GFP as reporter T7 production test.PNG
GFP test Check if the intact T7 promoter and GFP is functional GFP test.PNG
Adjacent bidirectional promoters test Evaluate if two promoters in opposite directions can function properly if they are placed adjacently Adj promoters test.png
Truncated promoter test Stimulate the condition in the overlapped version, where the first two non-essential base pairs of cl434 promoter are altered. We want to know if the cl434 can still function under such conditions. Truncated promoter test.PNG
Left/right induction test To see whether the overlapping promoter can drive transcription of both directions Left right test.png

Strain and vector used

  • Strain: E. coli BBa_V1001 DH5a, with genotype
 F-φ80dlacZΔM15 Δ(lacZYA-argF)U169 deoR recA1 endA1 hsdR17(rk- mk+ phoA supE44 λ- thi-1 gyrA96 relA1)
  • Vector: pUC18+ λ-InCh2

Integration system

We have chosen the λInCh system as the vehicle for intergration. Lambda phage inCh.png

The success rate for recombination is about 1 in 1000 cells. Ampicillin is used to screen for the second recombination event and temperatute of 42 degree Celsius is used to screen for the third recombination event. (Such temperature deactivates the cl857 repressor and hence activates the harmful gene of λ-phage introduced in second recombination event, killing the host cells.)

The advantages of this approach include:

  • No risk of >1 copy of target gene in our machine, so as to give a sharp output instead of "blurred" output caused by multiple copies
  • Stable integration of a single copy of the construct DNA fragment
  • Most ordinary E. coli strains and a variety of pBR322-derived Amp-resistant plasmids can be used
  • λ-phage as the only specialized vector required


  • Source:

Boyd D., Weiss D.S., Chen J.C., Beckwith J., Towards single-copy gene expression systems making gene cloning physiologically relevant: Lambda InCh, a simple Escherichia coli plasmid- chromosome shuttle system

(2000) Journal of Bacteriology, 182 (3), pp. 842-847.