Team:Edinburgh/Project

From 2011.igem.org

(Difference between revisions)

Latest revision as of 14:41, 28 July 2011

This page is obsolete. The project should be documented at the relevant subpages:

Designs

The general formats for the basic phage and cell display would be:

Promoter-RBS-LeaderSequence-Enzyme-(Linker?)-pVIII
Promoter-RBS-INP-(Linker?)-Enzyme

Actions that ought to be carried out

General

Make or acquire fusion-ready cellulases (e.g. <partinfo>BBa_K392006</partinfo>, <partinfo>BBa_K392007</partinfo>, <partinfo>BBa_K392008</partinfo>).

Since a simple test system is desired, make fusion-ready amylase, from E. coli's own malS gene.

Make or acquire spacer/linker sequences?
- Short linkers could be ordered as oligos. Berkeley 2009 made some longer linkers which we could order.

Phage display

Acquire M13 phage.

PCR from our [http://www.neb.com/nebecomm/products/productn4018.asp M13mp18] to get:
- pVIII mature protein
- pVIII leader sequence, coding for: MKKSLVLKASVAVATLVPMLSFA.

Make or acquire fusion-ready pIII gene? (optional)
- See <partinfo>BBa_K415138</partinfo> (complete) or <partinfo>BBa_K257001</partinfo> (sans leader sequence).
- Our final fusion will need the leader sequence followed by the gene of interest followed by pIII proper.

Cell display

Make or acquire fusion-ready cell-surface display parts.
- See Berkeley 2009 (but perhaps ignore them).
- Instead, <partinfo>BBa_K265008</partinfo> (ice nucleation protein) looks promising.
- The fliC gene seems to be the target for flagella display; note that the displayed protein has to be inserted into the middle of it.

Biorefinery

To add...

Completion

Fuse whatever enzymes to cell-display parts or pVIII or maybe pIII.

???

Profit!

@@ Line 1: / Line 1: @@
-A [[Project descriptions|project description]] and [[Safety/Proposals|safety proposal]] is supposed to be submitted by July 15.
+{{:Team:Edinburgh/tech/Navbox}}
+<html><script type="text/javascript" >$(document).ready(function() {
+	getMenus('home', 'home_project');
+}); </script></html>
+<div class="main_body">
+__NOTOC__
+'''This page is obsolete. The project should be documented at the relevant subpages:'''
-==Project abstract==
+* [[Team:Edinburgh/Phage Reactors 2.0|Phage Reactors]]
+* [[Team:Edinburgh/Cell Display|Cell Display]]
+* [[Team:Edinburgh/Biorefineries|Biorefineries]]
-This year we will create '''"bioreactors"''', consisting of scaffolds for various enzymes, to carry out reactions in an extracellular environment. The hope is that, by combining the activity of multiple '''synergistic''' enzymes in a small space, high efficiency will be achieved. At least 4 systems are being considered:
+==Designs==
-* As a baseline, use '''bacteria''' as the scaffold, and attach enzymes by cell-surface display techniques.
+The general formats for the basic phage and cell display would be:
-* As a modified version of the above, use bacteria, but concentrate the enzymes on a small part of it such as the '''flagella'''.
+* Promoter-RBS-LeaderSequence-Enzyme-(Linker?)-pVIII
+* Promoter-RBS-INP-(Linker?)-Enzyme
-* As a fairly novel concept, use '''M13 phage''' as the scaffold, and attach enzymes by phage-display techniques to the pVIII coat protein.
-* As a modified version of the above, attach multiple such phage to '''beads''' via the pIII protein, making a larger "reactor".
-As example systems, we will (probably!) use '''cellulases''' as our enzymes of interest.
-==Pages==
-* [[Team:Edinburgh/Phage Reactors 2.0|Phage Reactors]]
-* [[Team:Edinburgh/Cell Display|Cell Display]]
 ==Actions that ought to be carried out==
@@ Line 26: / Line 24: @@
 * Make or acquire fusion-ready cellulases (e.g. <partinfo>BBa_K392006</partinfo>, <partinfo>BBa_K392007</partinfo>, <partinfo>BBa_K392008</partinfo>).
-* If a simple test system is desired, make fusion-ready amylase? Or something else?
+* Since a simple test system is desired, make fusion-ready amylase, from ''E. coli's'' own ''malS'' gene.
 * Make or acquire spacer/linker sequences?
-** These are short enough that ordering them as oligos probably makes sense...
+** Short linkers could be ordered as oligos. [[Team:Edinburgh/Berkeley 2009 Parts|Berkeley 2009 made some longer linkers]] which we could order.
 ===Phage display===
@@ Line 35: / Line 33: @@
 * Acquire M13 phage.
-* Make or acquire fusion-ready pVIII gene.
+* PCR from our [http://www.neb.com/nebecomm/products/productn4018.asp M13mp18] to get:
-** Perhaps from <partinfo>BBa_K415151</partinfo>.
+** pVIII mature protein
-** Remember it has a leader sequence, coding for: MKKSLVLKASVAVATLVPMLSFA.
+** pVIII leader sequence, coding for: MKKSLVLKASVAVATLVPMLSFA.
-** Our final fusion will need the leader sequence followed by the gene of interest followed by pVIII proper.
 * Make or acquire fusion-ready pIII gene? (optional)
@@ Line 47: / Line 44: @@
 * Make or acquire fusion-ready cell-surface display parts.
-** See [https://2009.igem.org/Team:Berkeley_Wetlab/Cell_Surface_Display_Parts Berkeley 2009].
+** See [https://2009.igem.org/Team:Berkeley_Wetlab/Cell_Surface_Display_Parts Berkeley 2009] (but perhaps ignore them).
-** Maybe also see <partinfo>BBa_K265008</partinfo> (ice nucleation protein).
+** Instead, <partinfo>BBa_K265008</partinfo> (ice nucleation protein) looks promising.
 ** The ''fliC'' gene seems to be the target for flagella display; note that the displayed protein has to be inserted into the middle of it.
+===Biorefinery===
+:''To add...''
 ===Completion===
@@ Line 60: / Line 61: @@
-{{:Team:Edinburgh/Template:Navbox}}
+</div> <!-- /main_body-->
+<html></div> <!-- /mids --></html>