Team:Edinburgh/Data

From 2011.igem.org

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(Phage Display System)
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==Phage Display System==
==Phage Display System==
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[[Image:Edinburgh-Data-Phage-Display.png|thumb|center|710px|The completed system should contain:<br>]]
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[[Image:Edinburgh-Data-Phage-Display.png|thumb|center|710px|The completed system should contain:<br>
&nbsp; A '''promoter''' (<partinfo>BBa_K523000</partinfo>) controlling:<br>
&nbsp; A '''promoter''' (<partinfo>BBa_K523000</partinfo>) controlling:<br>
&nbsp; &nbsp; an '''Endoglucanase&mdash;pVIII''' fusion<br>
&nbsp; &nbsp; an '''Endoglucanase&mdash;pVIII''' fusion<br>

Revision as of 19:36, 2 September 2011

Data Page

The iGEM rules require us to have simple illustrations of how our devices work and where the Parts function in the system; and links to the Registry for the parts/constructs for which we have produced data.

See the sample Data page.

Cell Surface Display System

The completed system should contain:
  A promoter (<partinfo>BBa_K523000</partinfo>) controlling:
    an INP—Endoglucanase fusion (<partinfo>BBa_K523008</partinfo> + <partinfo>BBa_K523011</partinfo>)
    an INP—β-glucosidase fusion (<partinfo>BBa_K523008</partinfo> + <partinfo>BBa_K523010</partinfo>)
    an INP—Exoglucanase fusion (<partinfo>BBa_K523008</partinfo> + <partinfo>BBa_K523009</partinfo>)
  Ribosome Binding Sites are indicated as green ovals.

Cellulose degradation is shown at top. In reality, tens of thousands of enzymes will cover the outer membrane in random places.

A test system to prove that <partinfo>BBa_K523008</partinfo> can be used to carry proteins to the outer membrane uses a fusion to Yellow Fluorescent Protein (YFP) or the E. coli amylase "malS" instead.

Phage Display System

The completed system should contain:
  A promoter (<partinfo>BBa_K523000</partinfo>) controlling:
    an Endoglucanase—pVIII fusion
    a β-glucosidase—pVIII fusion
    an Exoglucanase—pVIII fusion
  Ribosome Binding Sites are indicated as green ovals. "Signal" means a periplasmic signal sequence, directing the protein to the periplasm to be assembled into the phage.

A test system uses a fusion of pVIII to E. coli amylase "malS" instead.