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BASF Agricultural Solutions Belgium

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Stage-onderwerp 2012-2013: Molecular and physiological characterization of SnRK1 related genes in dark stress conditions

Abstract Bachelor Project FBT 2020-2021: Fine mapping of a transcription factor binding site involved in the regulation of a gene in wheat
Wheat is the dominant crop in temperate countries being used for human food and livestock feed and is therefore critical for mankind. It is estimated that there will be around nine billion people by 2050 and many of them will be dependent on wheat production. Therefore, the global wheat production must increase by 50 % to 60 % to feed all these people. One way to increase wheat production is by developing hybrid seeds and using heterosis as tool to increase yield. Hybrid production in autogamous plants requires a method to block self-pollination. A system that has been used for production of hybrids in many crop plants including maize, rice and sorghum is based on cytoplasmic male sterility (CMS), a mitochondrially-encoded trait, coupled with one or more nuclear genes able to suppress CMS in F1 plants. The aim of this study is to identify protein-DNA interaction of a specified gene(s) in wheat by using Yeast one-hybrid (Y1H) assay as a screening method and Saccharomyces cerevisiae as a model organism. Y1H assays involve two components which are DNA baits and protein preys. Briefly, a DNA bait is placed upstream of Y1H reporter gene, HIS3. Each DNA bait reporter construct is integrated into a fixed location within the yeast genome to generate “DNA bait-strains”, ensuring that the DNA bait is incorporated into yeast chromatin. A plasmid that expresses a protein of interest (POI)  fused to the activation domain of the yeast GAL4 transcription factor (GAL4-AD) is then introduced into the DNA bait-strain, and when the protein binds the promoter, the Gal4-AD moiety activates reporter gene expression. Activation of the HIS3 reporter is visualized by growth on media lacking histidine and containing the competitive inhibitor 3-amino-1,2,4-triazole (3-AT). As controls, yeast was transformed with empty pGADT7 AD vector. In this project, a set of 23 bait strains with point mutation(s) in the bait sequence have been studied. In total, eight bait-strains with mutations in the bait sequence were identified as having strong effects on the expression of the HIS3 reporter and therefore on the binding of the POI to the bait sequence. We hypothesize that the corresponding nucleotides in the bait sequence constructs are involved in the regulation of specified gene(s).
 
Abstract Bachelor Project FBT 2019-2020Identification of optimal mutations in a herbicide target gene
The competition between weeds and crops is a worldwide problem in agriculture. In order to increase the production, new crops tolerant to herbicides need to be developed. The aim of this study is to identify the optimal herbicide tolerance in a plant target gene (PTG) by using Saccharomyces cerevisiae as model organism and screening tool. The yeast cells are plated on a growth medium with various concentrations of herbicide in order to identify new and potentially optimal mutations of the PTG. Part of the screenings was for spontaneous mutants and a part was with chemically induced mutations using two different mutagens. As chemical mutagen A and mutagen B were used in screenings as prior art. The experiments show that mutagen B rendered fewer colonies than with mutagen A treatment whereas the latter increased numbers of herbicide tolerant colonies considerably. In total, 201 mutations were found of which 83 % are on known positions. The sort of mutations is different for spontaneous and chemical induced colonies. The base changes in DNA, induced by mutagen A, is mainly a replacement of thymine to adenine while the most common spontaneous mutation is from thymine to cytosine. The amino acid phenylalanine mutates preferably in leucine and isoleucine due to chemical mutagen A and in serine when it is a spontaneous mutation. The different mutations will be further investigated to confirm the herbicide tolerance of the PTG and to determine the half maximal inhibitory concentration (IC50) and resistance factor. The strongest mutations can be used to develop herbicide resistance in crops by either genetically modified (GM) or targeted genome optimization (TGO) techniques.
 
Abstract Bachelor Project FBT 2018-2019THE USE OF A YEAST THREE-HYBRID SYSTEM AS A TOOL FOR SCREENING RNA-PROTEIN INTERACTIONS

BACKGROUND: Triticum aestivum or common wheat is the third most cultivated cereal in the world after maize and rice. It is an important source of food for the population, as wheat has a high content of carbohydrates and protein. While 700 million tons of wheat is being produced annually, the demand for this cereal is still increasing due to its versatility. BASF Agricultural Solutions NV is responding to this demand by producing new cultivars of wheat and hybrid wheat. To improve hybrid wheat production, BASF is looking for superior characteristics to introduce to its hybrid wheat lines. In this project, BASF is working on an RNA-protein interaction in wheat.

OBJECTIVE: The aim of this study is to identify new pentatricopeptide repeat proteins (PPR) that interact with the BASF mRNA. This RNA-protein interaction is at the molecular basis to increase the commercial production of hybrid wheat.

METHODS: A yeast three-hybrid system in Saccharomyces cerevisiae is used to screen RNA- protein interactions. The vectors pGADT7 AD and pRS426, respectively containing a cDNA library and the BASF mRNA, are transformed into yeast strain YBZ-1. Interaction between the protein coded by the cDNA and the BASF mRNA activates the expression of HIS3 and lacZ reporters present in the YBZ1 genome. The HIS3 qualitative selectable marker is used to select transformed YBZ-1 colonies that contain the desired RNA-protein interaction. The cDNA in these colonies is PCR-amplified, send for sequencing and identified using the Blastn tool.

RESULTS: The quality check of the first and second batch of the cDNA library showed that the insert frequency of cDNA inserts in the pGADT7 AD vector was low. The frequency promised by Creative Biolabs was above 90%, while the maximum insert frequency found during the quality check was 42% for the second batch. Insert frequency for the first batch was even lower with a maximum of 8%. Plasmids from the first and second batch that are positive for a cDNA insert were sequenced. The results for the first batch showed sequences from Triticum aestivum. Sequencing results from the second batch of the cDNA library showed sequences for Gossypium hirsutum or cotton indicating that the wrong library was sent.

CONCLUSION: This project has been stalled by the poor quality of the cDNA library that was provided. The combination of a low insert frequency and cDNA present from other plants does not facilitate the search for new pentatricopeptide repeat proteins in wheat. Still, the yeast three- hybrid system seems to be a promising tool to find new RNA-protein interactions since positive controls showed interactions that where be detected both qualitatively and quantitatively. A third cDNA library can be ordered from another external company which will be used to identify new proteins capable of binding to the BASF mRNA. Another future perspective is to create a homemade cDNA library from wheat mRNA to ensure proper quality.

 
Abstract traineeship advanced bachelor of bioinformatics 2017-2018Setting up a framework for bringing routine data analysis to Oilseeds Breeding

Data is everywhere, it can start in the lab where callus material is checked for insertions, and continues in the greenhouse where lots of plants are screened for breeding value. To keep a clear view in this sea of data, a custom package with data analysis scripts was created based on the scripting language R. This approach worked fine, but now a more robust and user friendly way of working is needed when we want to scale up. This is what this traineeship is about. The project consists of three steps: first step is to make the R scripts robust and easy maintainable, second is to introduce standardized Rmarkdown (simple formatting syntax based on markdown that enables the user to output reports in different formats like html, pdf,…) and third is to create a (graphical) user interface where users are shielded from coding. The main focus of this project is that every user should be capable of doing routine data analysis in R as independent as possible.

To make the scripts robust, a new R package was initiated by my coach that contained new functions and updates from the ones used in the past. Scripts were designed according to a standard lay out, with a header, parameter section and the relevant analysis section. Next, these scripts were turned into Rmarkdown templates. By replacing the analysis section by a compile report section, the user can now use the parameters to parameterize a Rmarkdown template stored in the background of the R package which results in an html compiled report that opens automatically after compilation. Another advantage of using these Rmarkdown templates is the short code a user needs to go through. The old scripts contained dozens of lines, the new ones contain maximum 50 lines which makes it very readable for a user to run the code line by line.

Further, the templates allow all output files to be stored automatically, and can be easily retrieved by any other user, either to review, or to use the results to select the right plants in the greenhouse.

Because the user experience is top priority and the IT background is limited, we decided to create a small user interface that could both open a new template via parameter specification, and load existing analyses. A collection of buttons, colors and pop-up screens guide the users. The green arrow indicates the start button for the user friendly ‘Workflow for routine data analysis.’ 

Of course, all these changes apply to the aesthetics of the project. The real smartness is behind the scenes. One example is the create function which generates a template directory where a copy of the script and the results are stored. This is managed using unique identifiers created by R code to prevent users from browsing through the data structure or to put intelligence in folder names. Users should use the interface to retrieve the data. During creation of a new analysis an entry is added to a structured file that acts as a database. This file registers all the user entered parameters in yaml format and scans the folder structure to see if a Rmarkdown report is already available or not. Lastly, the functionality automatically opens the selected analysis template in the Rstudio IDE framework such that the user can directly run the appropriate code on the specified data.

User training is another part of this project. Users will need to learn to switch from a Windows to a Linux environment, and guidelines for data storage are needed. Therefore, we created a series of documentation called vignettes in R terminology. These are Rmarkdown files with example code combined with the explanation about how to use this code. Per analysis template, there is a vignette available that explains all of the hidden code. Furthermore, some vignettes were added on how to do the data management and how a new developer could start and add a new template.

For the future, the plan is to embed this workflow into the bigger picture, with the ultimate goal to get rid of the import and export of data. Now data from different databases is first exported to excel and then imported in R. In the future, these will need to be linked to databases which will increase again the efficiency.

 

Abstract bachelorproef 2015-2016Unravelling DELLA’s protein-protein interactions via co-Immunoprecipitation in wheat protoplasts

Bayer CropScience aims at delivering solutions to produce enough food, feed, fiber and renewable raw materials for the growing world population on the limited land available. Therefore, new strategies need to be designed to increase the yield. In the Trait Research department at the innovation center of Bayer CropScience, researchers are trying to find genetic ways to improve crop yield. Crop yield is a complex trait which itself is influenced by  several other traits in the plants, and is a consequence of the many interactions in the complex molecular regulations in a plant. Therefore it is important to identify the participating genes and understand how they work together in molecular signal transduction pathways. (Matthew Reynolds, 2012)

A major step forward in increasing yield was delivered by the Green Revolution, which took place in wheat and rice. In the Green Revolution, new improved wheat varieties were discovered. The new varieties were shorter because they contained mutations in genes that controlled the height of plants. These genes are known as Reduced Height (Rht) genes.  A benefit of these Rht genes has been an increase in grain yield through an improvement of the harvest index (Peter Hedden, Green Revolution Genes, 2010). The Rht genes were isolated more than a decade ago and were shown to encode DELLA proteins (Peng J. R., 1999). DELLA proteins are nuclear transcription regulators that help the plant to divide its energy and resources between the defense system and growth. This by regulating the cross-talk between several (hormone) signaling pathways. DELLAs alter the functioning of those pathways via regulation of gene transcription and protein interactions that stimulate the function of the other protein, inhibit it or even lead it to degradation (Sun, 2011).

The objective of this project is to build on the knowledge from the Green Revolution and find out more about the function, including the interacting partners of DELLA proteins, in wheat. To clarify these mechanisms, a technique has been developed to study the protein-protein interactions of DELLA, called co-Immunoprecipitation (co-IP). Before the interacting partners of DELLA can be identified, first an entire workflow has to be followed. To start, the wild type Rht-B1a gene is being introduced in wheat protoplast, combined with a Green Fluorescent Protein (GFP) reporter to visually confirm the transformation. Next, the efficiency of transient protoplast transformation can be improved to produce sufficient material for protein extraction. Because DELLA regulates in the nucleus, the nuclear membrane must be degraded to get out the protein. Finally, after the protein extraction the co-IP can start. The co-IP can be optimized by eluting with 1% SDS instead of 0,2 M glycine, after changing the incubation periods. To analyze the protein after co-IP an SDS-PAGE followed by Western blot is done. The protein-protein interacting partners can be determined by Mass Spectrometry (MS/MS).

In summary, this work results in the optimization of a method to study protein-protein interactions. The methods combine a transient protoplast transformation system followed by a co-IP to efficiently identify the interaction partners of a target protein, DELLA, but can also be used for any other protein of interest. Therefore the method will be an important research tool for discovery of new leads that can be used for genetic improvement of crops.

 
Samenvatting eindwerk 2013-2014:
Characterization and comparison of SnRK1 related genes in response to stress in two Arabidopsis thaliana ecotypes
Ever since the origin of the world, plants are one of the most important food sources for humans and animals. Plants are constantly confronted by multiple types of stress. Different types of stress result in both specific and convergent responses that modulate plant growth and development.
Arabidopsis research is the first step in an exciting future of plant improvement. The purpose of this project is to learn about the gene expression of the model organism Arabidopsis thaliana under certain stress conditions. In the future this can be useful to develop genetic modified plants that are more resistant to certain environmental stress. This would make it possible to grow plants under non-ideal conditions, and could eventually reduce loss of yield in the future if there is for example, a long period of drought, or a cold winter threatening the yield.
The first objective of this project is the molecular and phenotypic characterization of SnRK1 related genes in response to stress, using Arabidopsis thaliana as a model organism. The second objective is the molecular and phenotypic comparison of SnRK1 related genes in response to stress in two different Arabidopsis thaliana ecotypes.
For the phenotypic characterization, of both Arabidopsis ecotypes, several genotypes are grown in vitro where certain stress conditions can be simulated.  Arabidopsis is grown on a germination medium in a petri plate. The medium components can be adjusted to specific stress conditions. The plants are analyzed by taking pictures of the plates on specific time points; the leaf area is measured and the relative growth rate is calculated. Then a comparison can be made between control plates, plants which are not exposed to any stress and plants that are exposed to stress. By testing different genotypes (wild type, knock out and overexpression of the SnRK1 related gene) it can be determined whether SnRK1 related genes play a role in the survival of certain stress conditions.
A phenotypic characterization is also done on Arabidopsis growing in soil. Soil approximates more the natural environment of plants than in vitro experiments but has also several disadvantages compared with in vitro experiments.
The molecular characterization is done on gene level. To study the gene expression, different genotypes (wild type, knock out and overexpression of the SnRK1 related genes) of Arabidopsis are grown in soil and RNA is extracted from fresh leaf material. After cDNA synthesis, qPCR analysis is done.
The results of the phenotypic characterization show us that the tested SnRK1 related genes do not contribute to a better stress recovery for the stress treatments tested in this project. The results also show that Arabidopsis ecotype 1 generally shows a better stress recovery for al stress treatments than Arabidopsis ecotype 2.
The results of the molecular characterization show us that tested target gene 3 is induced a lot more by darkness than tested target genes 1 and 2.

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Technologiepark 38
9052 Zwijnaarde (Gent)
+32-9.243.07.18
Belgium

Contacts

Traineeship supervisor
Dos Santos Tome Filipa
Traineeship supervisor
Karel Van De Velde
Traineeship supervisor
Korneel Vandenbroucke
Traineeship supervisor
Ruud Derijcker
Traineeship supervisor
Pieter Ouwerkerk
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