Team:Tartu TUIT/Design

In the beginning, we intended to insert the four genes as a cassette to reduce the number of сloning and not to use an excessive amount of markers.We have chosen five different promoters to control the flux and try to maximise the yield of the final products.

We were planning to run the parallel assembly using Vegas, Gibson and CPEC methods. We had some trouble with the PCR: we did not manage to adjust the annealing temperature of the primers.

Another reason why we had to reject the initial plan was the inability to predict the activity of a particular gene and the rate of each reaction in the pathway. This restricted us in designing the experiments and forecasting the results.It also complicated the process of modelling.

To be able to track each step of the pathway we have decided to insert genes with alternating promoters one by one via centromeric plasmids with different selection markers. Non-identical selection will allow us to insert several genes simultaneously using double, triple and quadruple selection plates.

Used plasmids:

1. Plasmid 1
2. Plasmid 2
3. Plasmid
4. Plasmid

Based on our model we are planning to obtain 136 strains as a result of different combinations.

We are also planning to run a parallel experiment, following our second model (link) and perform a series of gene knockouts to increase the concentration of the Sedoheptulose-7-phosphate - the precursor of our pathway.

We have created primers to switch off TKL1, TAL1, NQM1, PHO13, PGI1.

Since it might be complicated to delete several genes at once, we have decided to first delete only TKL1 and TAL1. The deletion of these 2 genes has been proven to have some effect on the S7P concentration. This might help us to estimate the validity of our assumptions and determine whether it is reasonable to continue the knockouts further.

We are hoping to obtain 2 strains with the increased S7P concentration, that will prove our hypothesis and allow us to continue knock-outs to optimize S7P concentration.

After the creation of the strains we can proceed with measurements.

First of all, we will have to estimate the concentration of the precursor using HPLC in the wild-type and in 2 knockout strains.

In addition, we will have to approximate the activity of the enzymes in 4 test strains (all genes with pTDH3 promoter) with the help of HPLC.

Using the obtained results, we can choose the promoter combinations that are worth checking. Then we perform the same measurements with them and select a few relevant ones to continue the experiments with.

To maximize the yield of the final products we will have to optimize the growth conditions. Initially, we wanted to put our stains under the UV light to prove that they produce UV-absorbing compounds. We also hope that it might help to induce the production of the MAAs.

However, S. Churio proposed to also use the visible light.

A lot of specialists also noted that it is reasonable to try out different substrates to find an optimal composition. For example, R.Sommaruga and S.Churio have proposed to use nitrogen enriched media.One of the crucial qualities for the sunscreen compounds is photostability. Despite most science groups working on MAAs find them extremely photostable, we think it is necessary to test photostability of these compounds also in yeast extract.

Dr K.Lawrence has provided us with some guidelines on how to check for this property. We expect our idea to have some real applications in the future.In our opinion, our idea of combining MAAs with yeast extract can be fitting for the industry. After consulting with the scientists working with MAA, we have added some details to our long-term goals. The most popular advice was to incorporate more diverse MAAs with distinct absorption maxima to increase the effectiveness of the sunscreen. Unfortunately, the genes for a lot of the MAAs are still not identified. However, there are sources propose possible pathways for palythine and gaudasol. There is a way to produce gaudasol in yeast. We can repeat and modify this method and make a mix out of yeast extracts from 2 strains. Other pieces of advice were about the composition of the future sunscreen. For example, Dr R Garcesa proposed adding ascorbic acid to increase photostability.

Serviceability

Nowadays the demand for accessible, eco-friendly sunscreen became sensible. For example, Hawaii became the first US state that tries to ban certain types of sunscreens. Therefore, the creation of this sunscreen is justified. Mycosporine-like amino acids are proven to efficiently absorb UV A and B. A number of human studies were also conducted that have shown the superiority of these compounds over the synthetic filters, as it MAAs not only serve as UV absorbents, but also improve skin firmness (anti-wrinkle effect), smoothness and inhibit liquid peroxidation. https://mibellebiochemistry.com/app/uploads/2015/03/Helioguard-365_Mycosporine-like-amino-acids-from-red-algae-protect-against-premature-skin-aging-EuroCosmetics-09-06.pdf They also have a potential in wound healing, which can be beneficial as the product will not only be able to prevent sunburns but also heal them). Mycosporine-like amino acids are also considered harmless for human health. https://www.ewg.org/skindeep/ingredient/705167/PORPHYRA_UMBILICALIS_(RED_ALGAE)_EXTRACT/#.W4zwKJMzb-Y) We also could not find any information about MAAs being allergens.

Flexibility

Our goal was to make our system adjustable. It affected our choice of gene sequences. A wide variety of organisms produce Mycosporine-like amino acids. Throughout the cyanobacterial phyla, a lot of species synthesize shinorine from the sedoheptulose-7 phosphate. However, there exist 2 evolutionary different paralogous enzymes for the last reaction leading to the final products. https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3194895/ One of them is seryl transferase, and the other belongs to the ATP-grasp family. The latter allows the production of several MAA products, including shinorine and porphyra-334, and we have decided to work with it. This combination might be advantageous, since both compounds are useful in the sunscreen composition. The products and their yield is thought to be easily adjusted by the composition of the media.

Simplicity

The KISS principle is very popular with engineers from different backgrounds. It is important to make our system understandable and straightforward while avoiding the loss in functionality. For our team, that mostly consists of first-year bachelor students, it was especially important to account for the lack of the experience and try to design the project in the fashion that together with being applicable and of current interest, it could still be completed following basic protocols without using complicated methods. This approach has also some real-life applications. Eco-friendly cosmetics is a big trend in the industry right now, but a lot of this type of products belongs to small, young brands with limited laboratory capabilities and budgets. That is why simplicity and accessibility are so important in our case.

Robustness

It is important that the created system is able to work properly without frequent additional adjustments. This goal is harder to achieve with prokaryotic organisms, since they are prone to lateral gene transfer and aquire mutations a lot faster. When integrating foreign genes to prokaryotes, in our case S. cerevisiae, DNA is inserted into the chromosomal genome. Acquired properties are therefore stable for many generations. Moreover, yeast are less susceptible to the changes in the environment and stress factors. https://www.genwaybio.com/technologies/protein-expression/yeast-expression

6.Innovativeness

The novelty of our project is the use MAAs enriched yeast extract. This allows to skip the purification step and therefore get the maximum possible yield. The yeast extract itself is a popular cosmetics ingredient, that is used as a moisturiser and to nourish the skin. It is already used in the after sun care products. http://www.naturalislife.com/nio-active.html http://www.naturalislife.com/nio-active.html