Difference between revisions of "Team:Valencia UPV/Part Collection"

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Revision as of 10:17, 2 October 2018

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Part Collection

Introduction

Assembly methods using type IIS restriction enzymes (methods based on the Golden Gate technology) have a great advantage over those using Type II: The reaction is performed in a single step, without the need for gel band purification which decreases the efficiency of the assembly and is time consuming. In addition, with the Golden Gate technology it is possible to make assemblies with more than two pieces and the backbone in a single reaction. For these reasons, the Golden Gate technology is very well adapted to Printeria because its automation is less complicated than in other assembly methods.

It is because of these advantages that the Golden Gate technology is increasingly used. However, finding collections of parts in the same standard optimized for E. coli and well characterized is very complicated. That's why we decided to create our collection of basic parts: promoters, RBS, CDS and a terminator. This collection is based on some of the most used parts in E. coli from the Registry of Standard Biological Parts. To create this collection we used the Golden Braid 3.0 standard (link to that page). In addition, to give value to this collection, we have made a characterization of these parts.

In our collection we have represented different types of basic parts so that, combining them, we can create composite parts (transcriptional units) of different types: constitutive, inducible, repressible, depending on another construction, to implement a more complex circuit, ...

Basic Parts

All our basic parts are in the plasmid BBa_P10500 and are compatible with BioBricks as they do not contain any illegal sites for RFC10. They have not sites for the type IIS restriction enzymes BsaI and BsmBI. For information on how these parts have been designed, see our design page (link).

Promoters

With respect to promoters, we found three constitutive promoters of different strengths, a strong promoter for T7 phage DNA polymerase and a promoter for the sigma 32 subunit of E. coli DNA polymerase. In addition, in our collection there are three promoters regulated by a transcription factor: the inducible pBad, positively regulated by AraC in the presence of L-arabinose, and the inducible and repressible lux promoters, respectively positively and negatively regulated by LuxR in the presence of Acyl-homoserine-lactone.

Part Original BioBrick Description
BBa_K2656004 BBa_J23106 Constitutive promoter
BBa_K2656005 BBa_J23102 Constitutive promoter
BBa_K2656007 BBa_J23101 Constitutive promoter
BBa_K2656000 BBa_I719005 Strong promoter for T7 phage DNA polymerase
BBa_K2656001 BBa_K338001 Promoter for the sigma 32 subunit of E. coli DNA polymerase
BBa_K2656006 BBa_K2442101 pBad minimal promoter: positively regulated by AraC in the presence of L-arabinose
BBa_K2656002 BBa_R0061 Lux repressible promoter: negatively regulated by LuxR in the presence of Acyl-homoserine-lactone.
BBa_K2656003 BBa_R0062 Lux inducible promoter: positively regulated by LuxR in the presence of Acyl-homoserine-lactone.

RBS

Regarding the RBS, we have selected 5 from the Registry of Standard Biological Parts, with different strengths.

Part Original BioBrick Description
BBa_K2656008 BBa_J61100 Weak RBS
BBa_K2656009 BBa_B0030 Strong RBS
BBa_K2656010 BBa_B0032 Weak RBS
BBa_K2656011 BBa_B0034 Strong RBS
BBa_K2656012 BBa_J61101 Weak RBS

CONTACT US igem.upv.2018@gmail.com