Revision as of 10:11, 8 August 2011

Introduction
Our Project
Tools
- Gibson Assembly
- MITOMI
Notebook
- Protocols
- May
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- October
Considerations
- Human Practices
- Safety
Acknowledgements
- Sponsors
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Assembly Sequence

TODO: describe here the sequence of assembly for our plasmids: what plasmids we build; where the parts came from; 
what had to be done. For example, why did we have to rebuild J61002 from scratch?

This page will probably become very technical, in which case we will move it and replace by a succinct outline. 
The goal of this page is to keep everybody on the assembly team up to date on the ugly details of everybody's work.
Leave nothing out!

Reporter Plasmid

The reporter plasmid contains the mutated TetR operator coupled to a LacI inverter, so that in presence of TetR the reporter gene is activated. Two reporter plasmids are built: one that contains and RFP reporter, and one that contains a Lysis gene, to lyse the cells that contain valid combinations of TetR and pTet mutants, in order to recover their DNA. Their structure is illustrated below.

Backbone template assembly

The first step of assembly was to make a J61002 backbone, containing pTet and RFP. We took the J61002 plasmid from the registry, containing ampicillin resistance, RFP and a ColE1 replication origin (medium copy number). By PCR, we then added the pTet promoter in front of RFP. Finally, the pTet-RFP and the backbone (plasmid without RFP) were assembled thank to Gibson.( vincent, please confirm this!). This was our first successful Gibson assembly.

Vincent, please document this step. What template did you use, what primers, etc? Please include links to the 
sequences of the template, of the expected product, and if possible a table that summarizes that all, 
like Nadine did.

Part used for Gibson assembly	Amplified from which template	Features added by extension PCR
J61002 backbone	J61002 plasmid - from delivery kit	none
pTet-RFP	J61002 plasmid - from delivery kit	pTet

The product of this assembly is the J61002-pTet-RFP 'backbone' plasmid. It contains an ampicillin resistance gene, as well as RFP repressed by pTet. This plasmid is used as a template for the second step of assembly, in which the LacI inverter and reporter genes are introduced.

Adding the inverter and reporter

The second step is to add the LacI inverter and reporter gene into the backbone. Let's run through the elements one by one. We need:

The backbone, which already contains the pTet promoter
the LacI coding region, repressed by the pTet promoter
a pLac promoter...
...that represses expression of a reporter gene either RFP or the Lysis cassette.

TODO: - illustrate which parts are copied from where.
      - lookup biobrick numbers.
      - illustrate Gibson overhangs

The backbone is copied from the previously-assembled J61002-pTet-RFP. The RFP gene is not included in this copy; this allows the same PCR primers and products to be used for the assembly of both plasmids. The LacI coding region is copied from the Repressilator plasmid. In the case of the RFP plasmid, RFP is copied from the J61002-pTet-RFP plasmid, making a fragment separate from the backbone. In the case of the Lysis plasmid, the lysis device is copied from the T4 Lysis device plasmid, from the iGEM gene distribution. In both cases, the pLac promoter is introduced by the primer, using an overhang.

Part used for Gibson assembly	Amplified from which template	Features added by extension PCR
J61002-pTet backbone	J61002 pTet-RFP plasmid - from previous assembly	none
LacI	Repressilator plasmid	Degradation tag (ssrA) and terminator (rrnB)
Plac-RFP	J61002 pTet-RFP plasmid - from previous assembly	Plac
Plac-lysis	T4 lysis plasmid	Plac

TetR plasmid

This assembly was quite tricky, as we had to test 3 plasmids before succeeding.

We first took the J23019 plasmid from the registry and designed plasmids, but we never succeeded in amplifying something during PCRs. We assumed that probably the plasmid is not exactly the one described in the registry and went on with plasmid number 2.
Our second choice was pSB3C5, as we could partially reuse the primers designed for J23019. But the PCR results were very weak and the assembly failed.
So finally we used pSB3K1, which is really similar to pSB3C5, designed new primers and succeeded in doing the Gibson assembly!

We amplified this backbone, and added

Part used for Gibson assembly	Amplified from which template	Features added by extension PCR
pSB3K1 backbone	pSB3k1 plasmid - from registry	none
Pconst-TetR	Repressilator plasmid	Constitutive promoter (pConst)

@@ Line 60: / Line 60: @@
 The '''backbone''' is copied from the previously-assembled J61002-pTet-RFP. The RFP gene is '''not''' included in this copy; this allows the same PCR primers and products to be used for the assembly of both plasmids. The '''LacI''' coding region is copied from the Repressilator plasmid. In the case of the '''RFP''' plasmid, RFP is copied from the J61002-pTet-RFP plasmid, making a fragment separate from the backbone. In the case of the '''Lysis''' plasmid, the lysis device is copied from the T4 Lysis device plasmid, from the iGEM gene distribution. In both cases, the '''pLac''' promoter is introduced by the primer, using an overhang.
-{| border="1" align="left" style="text-align:center;"
+{|
-!align=left| Part used for Gibson assembly
+! Part used for Gibson assembly
-!align=left| Amplified from which template
+! Amplified from which template
-!align=left| Features added by extension PCR
+! Features added by extension PCR
 |-
 | J61002-pTet backbone
@@ Line 81: / Line 81: @@
 | Plac
 |}
 == TetR plasmid ==

Team:EPF-Lausanne/Our Project/Assembly

From 2011.igem.org