Team:Peking/Parts

Peking iGEM 2017

Favorite Basic Part



Bxb1 gp35

This year, our team has selected a series of recombinases through litera-ture searches and characterized a number of them. Here we present the best characterized recombinase - Bxb1 gp35 (BBa_K2243012) as our best basic part for the award.
With well-behaved inversion performance, Bxb1 gp35 can invert the target DNA sequence efficiently, thus changing the function of the circuit accord-ing to our demands, and can be designed and used by other iGEM teams in their project/research.

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Figure 1. Schematic of the standard approach used for recombinase characterization.

How we characterized and improved the part

Using our standard approach to characterize recombinases (Figure 1), we selected two different vectors and a series of RBS to express Bxb1 to in-vert the constitutive promoter BBa_J23119 and change the fluorescence. Through the screening procedure, we improved the performance of Bxb1 gp35 and obtained a number of well-behaved matches, among which Bxb1 gp35 recombinase works particularly well. (See more in Results)


Properties

Through the fine tuning, we improved the performance of Bxb1 gp35 effi-ciently. Here we present some of the well-tested behaviors of this recom-binase, which indicates the excellent properties of Bxb1 gp35.

High efficiency of inversion under most conditions

Whether with computer-designed RBS or widely used RBS from the iGEM registry, Bxb1 exhibited a relatively high efficiency in inverting the target promoter.

Low leakage through tuning

Through our tuning procedure and exhaustive characterization, we ob-tained a series of response curves to the concentration of inducer, in which relatively low leakage (no inducer) and high inversion efficiency (proper in-ducer concentration) were found. This property meets our requirements well, indicating that Bxb1 gp35 can change the DNA accurately according to our needs.

Potential for controlling the downstream circuit

In addition to inverting the promoter to change the gene expression, we al-so used the improved Bxb1 expression plasmid to invert a unidirectional terminator (See more in Results), thus opening or closing the expression of a downstream reporter gene.

Table of Basic Parts we submitted


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Composite Part



Best Composite Part

Our team constructed many composite parts for the expression of the re-porter and the recombinase. Here we present a list of them, and introduce the best-performing part: Bxb1 attB_ ECK120034435_Bxb1 attP, as our best composite part.

Function of Bxb1 attB_ECK120034435_Bxb1 attP

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Figure 1. Schematic of the Bxb1 attB_ECK120034435_Bxb1 attP composite part as integrated into the GFP expression plasmid.

Our best composite part consists of the Bxb1 gp35’ target sites attB/attP and one well-behaved unidirectional terminator (ECK120034435) between them. This construct can be regarded as an outstanding biological switch for RNA polymerase, because of its high ratio between forward and re-verse terminator strength. What’ more, we can express Bxb1 gp35 to change the direction of the terminator and switch on/off the expression of downstream genes.

Excellent performance

High ratio between forward and reverse terminator strength. (Over 1000-fold)

The terminator ECK120034435 is the best-performing unidirectional termi-nator in our library, and its Ts ratio is higher than 1000-fold, which indicates that it can potentially be used as an RNAP switch in our circuit.

No latent reactivity to transcription.

Unlike some other terminators we observed and characterized, ECK120034435 has no latent promoter reactivity under most conditions, and won’t start transcription even if ligated with recombinase reaction sites. Thus, this terminator can be used as our controller to improve the predictability of our constructed circuit.

Robustness under different conditions.

When we introduced one or two pairs of attB/P sites on both sides of ECK120034435 to construct the controller that can be inverted by recom-binase, the great performance of this unidirectional terminator was robust. This property shows its potential utility in constructing more complex con-trol circuits in our sequential logic circuitry.

Ability to control expression through the recombinase.

With the excellent performance in opening/closing the transcription pro-cess, we have proved that our best composite part can be inverted by Bxb1 gp35 to obviously change the GFP expression, which shows that this construct is potentially a great control unit for gene expression under the control of recombinases.



Composite Parts Table

maybe need another card

Background

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Improvement



Though there are already many recombinase parts in the iGEM registry, quantitative characterization data on them is very limited, and what's more, there is no single standard characterization method for serine recom-binases. In addition, even though the attL/R sites formed by the recom-binase inversion are not recognized by the recombinases which create them, we successfully achieved the "reset" process using fusions of the recombinases and their recombination directionality factors (RDF).

Improvement of TP901-1

There is no submitted TP901-1 integrase part in the iGEM registry. Moreo-ver, the only data for TP901-1 was obtained through the dimerization of split integrase, which did not work so well. Additionally, there appears to be no quantitative information to evaluate the RDF of TP901-1.
This year we submitted the TP901-1 (BBa_K2243000) coding region as a basic part, and obtained detailed data to evaluate the inversion efficiency of TP901-1 integrase with different RBSs and vectors through our stand-ard characterization method. This opens the possibility to tune and improve its performance further to meet our design requirements.
We also used our composite part BBa_K2243035, comprising the unidirec-tional terminator ECK120034435 flanked by attB/P sites, as the reporter to evaluate the performance of TP901-1, which broadens the prospects to use TP901-1 to control gene expression.
We also constructed the fusion protein BBa_K2243014, comprising TP901-1 integrase and its RDF(BBa_K1733000), and tested its ability to invert DNA through attL/R sites. (See more in Results)


Improvement of Bxb1 gp35

Some characterization data of Bxb1 gp35 (BBa_K907000) is already available in the iGEM registry, but it is still limited because the RBS plays a significant role in recombinase expression and performance according to our modelling and observations. Without proper RBSs, Bxb1 may exhibit very high leaky expression (even approaching the induced expression level).
This year, our team constructed an RBS library to improve the efficiency of Bxb1 gp35. We obtained a number of well-behaved matches (from BBa_K2243002-BBa_K2243005), and measured their corresponding transfer curves against the concentration of inducer. Through our im-provements, Bxb1 showed a very high efficiency of nearly 95% and low leakage of inversion.
Additionally, we used our composite parts (BBa_K2243023 and BBa_K2243024), comprising the unidirectional terminator ECK120034435 flanked by attB/P sites as the reporter to evaluate the performance of Bxb1 gp35, which broadens the prospects to use Bxb1 to control gene expres-sion.
Finally, we fused Bxb1 gp47 (BBa_K907001) with Bxb1 gp35 and tested its ability to reinvert the DNA sequence flanked by its specific attL/R sites.


Improvement of phi31 integrase

Though there are quite a few parts related to phiC31 integrase, there is no systematic standard characterization of it. The only relevant information we found comprises fluorescent images that show the performance of phiC31 in plants, which is not quantitative and accurate.
Our team used our standard reporter (BBa_K2243008) to characterize phiC31, and selected a few well-behaved phiC31 translational units which can achieve very high inversion efficiencies with low leakage. Through these data, we will be able to make use of phiC31 in our future designs more efficiently and accurately. Additionally, we used our composite part (BBa_K2243031), consisting of the unidirectional terminator ECK120034435 flanked by attB/P sites, as the reporter to evaluate the per-formance of Bxb1 gp35, which broadens the prospects to use Bxb1 to con-trol gene expression.