Team:ETH Zurich/Wetlab/Chemostat Selection

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Chemostat selection


1. Goal

The goal of our project is to find the minimal genome that is able to support survival of E. coli. In the previous section, we have introduced the method we want to apply for reducing the genome. However, manually selecting for those bacteria that have successfully reduced their genomes is obviously impossible. Therefore, we have to find a mechanism that automatically selects cells possessing a reduced genome.


2. Idea

Our idea is to set up a continuous bacterial culture in which cells possessing a reduced genome overgrow those maintaining more chromosomal DNA.

However, bacteria with a smaller genome do not automatically grow faster than those containing more DNA. Therefore, we want to introduce a constraint that renders DNA synthesis the limiting factor of the growth rate. In this scenario, reducing chromosomal DNA would speed up replication leading to fastest growth of those cells with the smallest genome. Hence, we would not have to look for bacteria with reduced genomes, but let them find us!


3. Method

3.1 Chemostat

A chemostat is the instrument of choice for setting up a continuous culture. It is characterized by a continuous influx of medium, and an efflux of bacterial culture of the same volume. Since the optical density of the continuous culture is kept constant, the volume of influx/efflux per time is solely determined by the growth rate of bacteria. Under these conditions, slowly growing cells will be washed out of the culture, while the fastest growing clone will take the lead and finally dominate the entire culture.



3.2 Growth constraint

As mentioned above, we want to introduce a constraint that renders DNA synthesis the limiting factor of the growth rate. DNA synthesis in bacterial cells is accomplished using the following biosynthetic pathway:



The thymidylate synthase catalyzes the methylation of dUMP to yield dTMP. Phosphorylation then converts dTMP into dTTP, one of the four building blocks of DNA. In contrast to the other three nucleotides DNA is made of, dTTP is exclusively used for DNA, but not RNA synthesis. Therefore, impairing the activity of the thymidylate synthase should interfere quite specifically with DNA synthesis.

Our idea is to knockout the thymidylate synthase of the E. coli strain we use for genome reduction and then add thymidine to the continuous culture in a concentration that renders DNA synthesis the limiting factor for the growth rate.

The underlying assumptions are that a thymidylate synthase knockout slows down DNA replication and that a decreased replication rate results in a slower growth rate. Escartin et al. showed that an E. coli strain expressing an enzymatically less active thymidylate synthase shows a significantly lower incorporation rate of radioactively labeled thymidine into DNA indicating a reduced replication velocity. The same strain grows poorly in thymidine-deprived growth media. Other reports support that a decreased replication rate results in a slower growth rate and decreased replicative fitness. Therefore, we conclude that a smaller genome in an otherwise identical thymidylate synthase knockout background leads to faster DNA replication and, hence, confers a growth advantage.