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Comparison of biotechnological procedures for pure proteins preparation
Bušanski, Patrik ; Langová, Denisa (referee) ; Brázda, Václav (advisor)
The production of recombinant proteins is a biotechnological process during which proteins are produced in foreign organisms by gen manipulation. To form a recombinant plasmid the gene encoding the desired protein is isolated and inserted into an expression vector. The plasmid is then transformed using physical or chemical method into a suitable host, where the recombinant gene is translated into amino acid sequence in the newly synthetized protein. The theoretical part of this bachelor thesis includes characteristics of proteins, methods of recombinant protein preparation and compares individual expression systems. Three isoforms of the p53 protein, which were synthesized in the E. coli microorganism, were selected for processing the experimental part. The transformed recombinant plasmid contained two tags for purification, HIS-tag and GST-tag, making it possible to compare the efficacy of the two purification methods. HIS-tag purification was found to work for all three isoforms better, with concentrations of recombinant proteins were several times higher than those of the GST-tag. The p53 proteins are about 50 kDa long, what was confirmed by sodium dodecyl sulfate polyacrylamide gel electrophoresis.
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Double expression systems with respect to parasitic protozoa
Gromyko, Anastasiia ; Verner, Zdeněk (advisor) ; Kraeva, Natalia (referee)
Protozoan parasite infections continue to pose a significant health challenge in developing countries, resulting in hundreds of thousands of deaths each year. These parasites exhibit a complex multi-stage life cycle and possess unique cellular structures. However, many of their biological processes remain poorly understood. Multigene expression is a promising approach to address this knowledge gap, as it enables the expression of functional protein complexes in vivo, the addition of fluorescent protein tags for visualization of protein localization within the cell, and the study of protein-protein interactions. This bachelor's thesis reviews the current knowledge on available systems and approaches for studying key model parasitic protozoan species. Keywords: expression systems, Trypanosoma brucei, Leishmania tarentolae, Entamoeba histolytica, Giardia intestinalis, Trichomonas vaginalis, Toxoplasma gondii, Plasmodium falciparum, pET-Duet, CRISPR-Cas9
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Inducible expression systems and their use in the study of parasitic organisms.
Horáčková, Vendula ; Doležal, Pavel (advisor) ; Fišer, Radovan (referee)
1 Abstract Inducible expression systems are systems with ability to switch expression of genes of interest on and off. Therefore, they are useful molecular tools for analysis of gene function. Nowadays, there are tens of various inducible expression systems available that differ from each other in level of regulation of gene expression, time of induction, possibilities of use, etc. This work is focused on three of them to illustrate common features of the inducible expression systems which regulate gene expression at the level of transcription. Firstly, systems based on regulation of lactose operon of Escherichia coli are mentioned. Secondly, systems which use regulatory elements of tetracycline resistance-encoding transposon Tn10 of E. coli are described. Third chapter is focused on systems regulated by agonists of ecdysone receptor. In the last chapter cases of use of inducible expression systems in the study of parasitic organisms are summarized.
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Comparison of biotechnological procedures for pure proteins preparation
Bušanski, Patrik ; Langová, Denisa (referee) ; Brázda, Václav (advisor)
The production of recombinant proteins is a biotechnological process during which proteins are produced in foreign organisms by gen manipulation. To form a recombinant plasmid the gene encoding the desired protein is isolated and inserted into an expression vector. The plasmid is then transformed using physical or chemical method into a suitable host, where the recombinant gene is translated into amino acid sequence in the newly synthetized protein. The theoretical part of this bachelor thesis includes characteristics of proteins, methods of recombinant protein preparation and compares individual expression systems. Three isoforms of the p53 protein, which were synthesized in the E. coli microorganism, were selected for processing the experimental part. The transformed recombinant plasmid contained two tags for purification, HIS-tag and GST-tag, making it possible to compare the efficacy of the two purification methods. HIS-tag purification was found to work for all three isoforms better, with concentrations of recombinant proteins were several times higher than those of the GST-tag. The p53 proteins are about 50 kDa long, what was confirmed by sodium dodecyl sulfate polyacrylamide gel electrophoresis.
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Inducible expression systems and their use in the study of parasitic organisms.
Horáčková, Vendula ; Doležal, Pavel (advisor) ; Fišer, Radovan (referee)
1 Abstract Inducible expression systems are systems with ability to switch expression of genes of interest on and off. Therefore, they are useful molecular tools for analysis of gene function. Nowadays, there are tens of various inducible expression systems available that differ from each other in level of regulation of gene expression, time of induction, possibilities of use, etc. This work is focused on three of them to illustrate common features of the inducible expression systems which regulate gene expression at the level of transcription. Firstly, systems based on regulation of lactose operon of Escherichia coli are mentioned. Secondly, systems which use regulatory elements of tetracycline resistance-encoding transposon Tn10 of E. coli are described. Third chapter is focused on systems regulated by agonists of ecdysone receptor. In the last chapter cases of use of inducible expression systems in the study of parasitic organisms are summarized.
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