Life sciences (LIFE) // Life Sciences (LIFE)

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https://odr.chalmers.se/handle/20.500.12380/10

Vi bedriver forskning och utbildning − och driver innovation − för att möjliggöra ett biobaserat samhälle och förbättra människors hälsa. Våra områden innefattar både grundläggande och tillämpad forskning inom life sciences.
På institutionen för life sciences, LIFE, (tidigare biologi och bioteknik) utforskar vi hur biologiska system och innovativa teknologier kan användas för att omvandla biomassa till livsmedel, läkemedel, material, kemikalier och bränslen. Vi utvecklar och använder avancerade experimentella tekniker och beräkningsmodeller för att undersöka hur biomolekyler, levande celler och organismer fungerar och interagerar. Vi banar väg för nya metoder för att förutse, förebygga, diagnosticera och behandla sjukdomar.

Läs mer om våra utbildningar

För forskning och forskningspublikationer, se https://research.chalmers.se/organisation/biologi-och-bioteknik/

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We conduct research, innovation, and education to enable a biobased society and improve human health. Our topics cover both basic and applied aspects of life sciences.
At the Department of Life Sciences, LIFE, (former Biology and Biological Engineering) we explore how biological systems and innovative technologies can be used to convert biomass into foods, pharmaceuticals, materials, chemicals and fuels. We develop and apply advanced experimental and computational technologies to discover how biomolecules, living cells and organisms function and interact. We pioneer new methods for the prediction, prevention, diagnostics and treatment of diseases.

Studying at the Department of Life Sciences at Chalmers

For research and research output, please visit https://research.chalmers.se/en/organization/biology-and-biological-engineering/

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    3D Bioprinting Meniscus for Future Tissue Replacement in Osteoarthritis Affected Knee Joints
    (2020) Pettersson, Ida; Olsson Widjaja, Amanda; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Gatenholm, Paul; Simonsson, Stina
    Progressive cartilage defects in human knee joints are a worldwide health issue that exposes a great burden on society as well as on single individuals. Sudden traumas to the knees can induce tears in the structures of the joints such as the articular cartilage and the meniscus. Lesions in the cartilage tissue of the knee joints have a high probability to eventuate in osteoarthritis (OA). The emerging technique of 3D bioprinting tissue is a novel approach for cartilage repair and regeneration. The choice of bioink and cell type are important factors that considerably impact the resulting cartilage repair potential after the process of 3D bioprinting. Induced pluripotent stem cells possess the ability to differentiate into almost any cell type and their potential in future regenerative medicine is of great interest. The present study has investigated the possibility of 3D bioprinting chondrocytederived human induced pluripotent stem (iPS) cells into meniscus structures with initiated cartilage regeneration. A combination of nanofibrillated cellulose (NFC) and alginate (A) was used as bioink. At first, the bioink was subjected to optimization to augment printing properties and cell viability during and after bioprinting. The composition of nanofibrillated cellulose and alginate originated from a ratio of 60/40 NFC/A (% w/w) that was compared with one ratio of 48/52 NFC/A (% w/w) and one ratio of 80/20 NFC/A (% w/w). The optimization of bioink involved measurements of printability, rheology, and cell viability. The formation of microtissues enabled differentiation of iPS cells toward extracellular matrix (ECM) producing cells prior to 3D bioprinting. 3D bioprinted menisci, as well as cultured microtissues, were analyzed with LIVE/DEAD assay, immunohistochemical analysis, and quantitative reverse transcription polymerase chain reaction (qRT PCR). The work also comprised an in vivo assay of 3D bioprinted constructs transplanted subcutaneously in mice to enable the evaluation of tissue formation in a realistic milieu. Induced pluripotent stem cells further modified to express green fluorescence protein under the aggrecan promotor have been subjected to a screening of a library of small Food and Drug Administration (FDA) approved molecules. Changes in intensity indicated induction or inhibition of the synthesis of aggrecan. Moreover, the screening highlighted molecules included in the induction or inhibition of aggrecan production. These molecules will be subjected to further investigations to evaluate their possible contribution in future OA-treatments. The prevailing work demonstrates the feasibility of utilizing microtissues formed by iPS cells for the 3D bioprinting of cartilage tissue. The culturing of iPS cells as microtissues has proven to induce differentiation and synthesis of components included in the ECM, both in vitro and in vivo. Simultaneously, the study has included a comparison of three bioinks that resulted in an optimized protocol for the production of the bioink composed of 60/40 NFC/A (% w/w). This optimized bioink fulfilled the requirements of being printable while supporting cell viability.
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    A CRISPR approach to manipulating NK cell receptor ligand expression
    (2018) Kristensson, Linnea; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Natural killer (NK) cells are important innate lymphocytes in the immune system and have been considered to be vital in fighting cancer, virus infections as well as regulating immune responses. The activity of NK cells is regulated via a complex signaling between inhibitory and activating receptors. Ligands for most of the ac-tivating receptors have been discovered but no endogenous ligand for one of the important natural cytotoxicity receptors, NKp46 has been identified. Therefore, the long term aim of this thesis project was to define ligand candidates for the acti-vating receptor NKp46 with intermediate aims to manipulate expression of NK cell activating receptor ligands in the K562 cell line using a CRISPR approach. The result from the performed cytotoxicity assays demonstrated the importance of the activating receptors NKp30 and DNAM-1 in elimination of K562 cells and the expression of the complementary ligands NCR3LG1, PVR and NECTIN2 was confirmed using RT-qPCR. The successful creation of a Cas9-expressing K562 cell line was demonstrated, including verification of Cas9 protein expression using both flow cytometry and western blot. Following that, a constructed plasmid with the gRNA for the B7-H6 gene, NCR3LG1, was generated and shown to create a cleavage and mutation within the gene. The engineered cell line was ultimately shown to have a reduced expression of the B7-H6 protein, indicating the successful knockout of the NCR3LG1 gene.
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    A kinetically-constrained FBA-model of the synthesis of aromatic amino acid-derived products in Saccharomyces cerevisiae
    (2015) Janasch, Markus; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    During the last decades the research interest for creating a more sustainable and environmentallyfriendly society and industry has increased dramatically. The employment of icroorganisms to create valuable compounds such as fuels and chemicals from renewable resources has gained high popularity. With directed modifications in the metabolism of these microorganisms, metabolic engineering seeks to optimize the properties of these organisms for an efficient bioprocess to produce valuable compounds. One characteristic of metabolic engineering is the extensive use of computational models to predict the behavior of the metabolism and thereby identifying suitable targets for genetic interventions in an in silico to in vivo progress. Flux Balance Analysis (FBA) is a popular analysis method for metabolic models, as it only requires the underlying stoichiometric network of the metabolism modelled. With FBA the optimal flux distribution, given a certain objective to be maximized, can be calculated with linear programming algorithms. As FBA only takes the stoichiometry and reaction directionality into account, further physiological constraints have to be included in the framework to increase the predictive strength of the simulations. In this thesis, an expanded form of FBA, that includes kinetic enzyme parameters as additional constraints on the system, was used to analyze a metabolic model of the popular industrially-used organisms Saccharomyces cerevisiae, that included, additionally to the native metabolism, also recombinant enzymatic steps to form the plant secondary metabolites resveratrol and naringenin from the aromatic amino acids phenylalanine and tyrosine. Resveratrol and naringenin have been found to be beneficial to human health by offering anti-inflammatory, anti-carcinogenesis and anti-oxidant properties. The kinetically-constrained model was successfully used to estimate the impact of introducing recombinant pathways on the protein pool in the cell as well as to identify the enzymatic steps offering the highest control over the flux towards these products. This might be used in metabolic engineering to estimate the efficiency of metabolic pathways in the context of the whole metabolism form a protein cost point of view.
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    A Modular Toolkit to Enable Intein-mediated Enzyme Fusions
    (2024) Storm, Linus; Chalmers tekniska högskola / Institutionen för life sciences; Chalmers University of Technology / Department of Life Sciences; Larsbrink, Johan; Widén, Tove
    In second generation biorefineries, lignocellulosic biomass is fermented by microbes to higher-value products. Hydrolysis of the substrate is necessary to break it into fragments that the microbes can utilize. Enzymatic hydrolysis is often preferred, but a bottleneck is the high costs of enzyme cocktails since lignocellulosic polymers require several types of enzymes to be degraded. Fusion enzymes have been produced to increase conversation rates, but the methods for creating them are either complex or limited. This project aimed to circumvent some of these limitations by creating a modular toolkit to produce any fusion enzymes, where the fusion is split intein-mediated in vitro. For evaluation of the toolkit, an α-xylosidase (BoGH3B) and a β-glucosidase (BoGH31A) involved in xyloglucan (XyG) degradation, were chosen. The toolkit was developed to completion and consists of eight types of parts, excluding the protein of interest. Three assemblies were confirmed by sequencing, proving that the toolkit works. Aside from the toolkit-mediated assemblies, the enzymes on their own were expressed and tested in different combinations for XyG degradation. This was done to compare with the split intein-fused enzymes. However, when it came to expressing the protein assemblies the yield was low, and no fusion could be observed. Thus, the possibly synergistic effect of fusing BoGH3B and BoGH31A could not be investigated. A lot of research is still needed to determine the usefulness of split inteins for creating enzyme fusions. For future work, some experiments need redoing, and new experiments with different linkers and configurations of the assemblies could be performed.
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    A platform for Acetyl-CoA synthesis using xylose as feedstock in Saccharomyces cerevisiae
    (2015) Englund Örn, Oliver; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Global rise in temperature and diminishing oil reserves has stimulated a market of alternative replacements to traditional petroleum based products. An alternative is the use of a bio refinery capable of converting biomass to the normally petroleum based products. The baker yeast Saccharomyces cerevisiae is an attractive cell factory as its existing large-scale infrastructures for bioethanol production. However, it cannot utilize xylose, an otherwise unusable part of the plant biomass, which represents of utmost importance in the bio-refinery development. To also have a strain capable to produce a wide range of products, it could be used as a platform to base a bio refinery upon. Therefore, the aim of this study is to generate platform strains capable of forming acetyl-CoA, an intermediate metabolite in many of the cells metabolic reactions and also for many other industrially relevant bio-chemicals. With this goal in mind, the metabolism of S. cerevisiae was engineered. The genes encoding an isomerase-based xylose assimilation pathway (RTG, XI, XKS), and a phosphoketolase pathway (XPK, PTA), were cloned into the yeast strain CEN.PK113-5D to enable the yeast to take up and convert xylose into acetyl-CoA. The functionality of this synthetic pathway were evaluated for the production of 3-hydroxypropionic acid via introduction of ACC1** and MCR genes into the engineered strains. By characterisation of all the engineered strains on glucose growth we found increase of acetate production in strains with the phosphoketolase pathway expressed, indicating the in vivo activity of this pathway. However, expression of the xylose assimilation pathway through genome integration did not render the strains able to grow on xylose, suggesting the low efficiency of the assembled xylose assimilation pathway. To overcome this adaptive laboratory evolution is recommended.
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    A Rolling Circle Amplification-Based Methodology for Making Long, SequenceRepeating, DNA Duplexes
    (2018) Dekoning, Nora; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    In vitro studies of sequence-specific DNA-protein interactions using techniques where long DNA molecules is needed are currently limited by the size of synthesized DNA molecules, or is restricted to the commercially available DNA. For single molecule DNA imaging techniques using for instance nanochannels confinement, the small sized molecules make the interactions difficult to detect. The commercially available DNA, on the other hand, does not allow any freedom in choosing or changing the DNA sequence. Therefore, a method for producing long DNA molecules containing a sequence of choice would alleviate these limitations and greatly improve the possibility to study DNA-protein interactions. The general concept of this paper was to create long, double-stranded DNA molecules with a sequence that is specifically designed to interact with the protein internal host factor. To make such molecules, three experimental procedures were developed, building on the single-stranded DNA products from a rolling circle amplification (RCA) reaction. The first experimental procedure was based on the presumed perfect annealing of smaller complementary strands to the single-stranded RCA product. The second experiment assumed that single-stranded gaps would be present in the duplex after annealing, hence the addition of a polymerisation reaction. In the third experiment, the RCA was run for 24 hours, to allow double-stranded product to be formed in the RCA. The DNA strands were visualized using fluorescence microscopy, with the goal of studying them and their protein interactions in nanochannels. To be able to use this detection method, an external fluorescent dye, YOYO, is used in the main aim of the project. However, as these types of dyes change the native structure of DNA, an extra aim was to use the fluorescent base analogue tC incorporated into one of the duplex strands, leaving the native structure intact. All three experimental procedures were shown to be capable of producing apparently double-stranded DNA molecules, that were larger than 100 kilo-base pairs albeit with a broad size distribution. This shows that the main aim in terms of procuing DNA molecules has been completed. The tC-containing DNA molecules were not visible under the microscope with the settings used, but appears to be promising.
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    A Step Toward Personalized Cancer Treatment Simultaneous Detection of Multiple Types of Chemotherapyinduced DNA Damage Using Single Molecule Imaging
    (2022) Foss, Ebba; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering; Westerlund, Fredrik; Akwasi Aning, Obed
    Chemotherapy is commonly used to treat cancer today, either alone or more commonly as part of combination therapy. Response to a certain chemotherapeutic agent is highly individual, both in terms of treatment efficacy and the extent to which healthy cells are affected. For several drugs, induced DNA damage provides the main cytotoxic effect, and a method for evaluating this damage could therefore prove a powerful tool in treatment planning. In this thesis, a single molecule imaging approach is used to assess chemotherapy-induced DNA damage, allowing visualisation of damage sites on individual DNA strands. While previous studies have focused on one damage type, or collective damage without distinction between types, a novel modification to pre-existing techniques that allows for this distinction has recently been demonstrated. In this thesis, the alkylating agent temozolomide was used to illustrate how different damage types can be distinguished with a single molecule imaging approach. This is done using repair enzymes associated with different DNA repair pathways. The repair enzymes sequentially incorporate spectrally distinct fluorescent nucleotides at the damage site which are then visualized as fluorescent spots of two different colours on individual DNA molecules. This distinction could be shown with high repeatability in terms of colour ratio. While both enzymes used separately clearly repaired the treated DNA, there appeared to be an overlap when applying them sequentially. This could suggest a problem with enzyme specificity. Further exploration of this issue is needed to verify the feasibility of single molecule imaging for the purpose of simultaneous detection of chemotherapy-induced DNA damage types.
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    Accelerated shelf life tests of wheat tortillas A study of microbial and textural deterioration in wheat tortilla
    (2018) Nilsson, Fredrik; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    This study tried to shorten the time required for shelf life studies in product development of wheat tortillas, by developing accelerated shelf life test (ASLT) models for microbial and textural shelf life. ASLTs speed up product degradation by exposure to extreme environmental conditions and in this case were temperature and relative humidity (RH) used. The samples were divided into four storage groups: 3°C and 70% RH, 20°C and 30% RH, 27°C and 80% RH as well as 40°C and 80% RH. Texture was determined with a fold/roll-method, an instrument and by a sensory panel. Microbial concentrations were determined by a laboratory company. Gas composition inside the bags, tortilla pH, water content and water activity were measured to determine possible links to the shelf life. It was not possible to calculate an ASLT model for the microbial growth because of unknown starting number of microbes. The microbial tests however showed that a high temperature and humidity caused the number of bacteria to rapidly increase above what is considered acceptable. Microbial ASLTs thus seem possible, but more tests with a lower detection limit are needed to create a model. To avoid bad taste from nonpathogenic bacterial growth, consumers are recommended to avoid storing the tortillas in high temperature and/or humidity. Textural ASLTs also seem possible in regards of rollability and foldability, but more tests are needed to precisely determine the accelerating factor. Stickiness and translucency seems to deteriorate much slower than rollability and foldability under normal storage conditions. It is therefore suggested to be enough to check that freshly baked tortillas meet the quality requirements of stickiness and translucency. Tortillas seemed to lose textural quality at the same rate, or slower, in refrigerator compared to room conditions. Longer shelf life studies are therefore suggested, to verify if this is the case. If so, storage in a refrigerator could possibly prolong shelf life of wheat tortillas. Changes in the modified atmosphere inside the bags seems to correlate with textural degradation. A study with atmospheric air instead would therefore be interesting as an attempt to determine if it retards textural degradation in wheat tortillas.
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    Acidophilic fungal beta-glucosidase(s) for biorefinery applications
    (2024) Danielsson, Albin; Wray, Ingrid; Chalmers tekniska högskola / Institutionen för life sciences; Chalmers University of Technology / Department of Life Sciences; Olsson, Lisbeth; Christopher, Meera
    Lignocellulose is a promising substrate for the production of chemicals and materials. In traditional biorefineries, it is first pretreated to disrupt its structure, thereby yielding acidic fractions. Therefore, enzymes from acid-tolerant organisms would be advantageous for their bioconversion. In this study, we have investigated beta-glucosidases (BGLs) from the fungi Talaromyces sp1. ASS 358-9 (Talaromyces-358), which thrives in highly acidic conditions and can utilize inhibitor-rich liquor from spruce pretreatment for growth and enzyme production. Since BGLs are crucial for biomass saccharification, we are studying the properties of differentially expressed Talaromyces-358 BGLs, aiming to find robust enzymes for biorefinery use that can withstand harsh environments like high temperatures and low pH levels. Culturing Talaromyces-358 in various liquid media revealed glucose as the most favorable substrate, significantly enhancing BGL activity over 15 days, while spruce liquor, though initially inhibitory, eventually supported significant enzyme production. The BGLs exhibited peak activity at 80°C and maintained considerable activity at 90°C, with optimal pH ranging from 4 to 6, demonstrating adaptability to harsh conditions. Enzyme activity was measured using substrates such as glucose, glucose-spruce, spruce, xylan, and xylan-spruce, with temperature measurements taken from 30°C to 90°C at pH 4, and pH measurements taken from 2 to 9 at 50°C. However, there was little to no BGL activity observed at neutral and basic pH levels.
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    Adaptive evolution of Yarrowia lipolytica
    (2017) Hellgren, John; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    We need renewable resources to allow sustainable production of fuels. By using lipid accu-mulating yeast, biodiesel can be produced in a sustainable way from resources that were previously not used, for example lignocellulose-based sources such as agricultural waste. However, for this process to be profitable, the tolerance of the yeast needs to be improved. This project aims to improve the tolerance of the oleaginous yeast Yarrowia lipolytica to-wards osmotic and saline stress by using the method adaptive laboratory evolution. This method has previously been shown to be efficient in constructing strains to tolerate new conditions without the need of prior knowledge. After evolving Y. lipolytica for 220 gen-eration in minimal medium containing 1.4 M NaCl, an improved performance in the same medium was observed, along with evolved cross-tolerance towards low pH. This indicates that this adaptive evolution of Y. lipolytica resulted in improved ionic tolerance rather than pure osmotic tolerance. The evolved strains were sent for whole genomic sequencing to find out which mutations that caused this phenotype. During this project, two previous CRISPR/Cas9 strategies were combined and adapted for efficient markerless reverse en-gineering. When genome data arrives, this strategy will be used for reconstruction of can-didate mutations to find out which mutations are important for the observed phenotype. The gained knowledge from this evolution experiment can later be used for constructing a robust industrial strain that efficiently converts lignocellulose-based material to biodiesel, allowing sustainable production of fuels.
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    Adaptive laboratory evolution of Saccharomyces cerevisiae for increased tolerance towards compounds of industrial interest
    (2016) Malina, Carl; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Over the last decades, microbial production of fuels and chemicals has become an increas-ingly attractive alternative to petroleum-based production. This has created a demand cell factories able to produce a wide range of compounds. The yeast Saccharomyces cere-visiae is widely used in biotechnology with successful applications in the production of both bulk and fine chemicals. However, in order to reach the full potential of yeast as a cell factory challanges still remain. These include creating strains tolerant to stress conditions, such as inhibition at the high product titers required in industrial production. Traits conferring these properties are often complex and encoded by several genes. In order to obtain strains with improved tolerance, adaptive laboratory evolution (ALE) is often used. This thesis was part of an ongoing project of ALE for increased tolerance towards compounds with potential industrial applications. The work in this thesis can be divided into two main parts. The first part was screening for tolerance of S. cerevisiae towards four diols and two diamines by microplate cultivation. For both the diols and diamines, clear trends of decreasing fitness as compound concentration was increased was seen. For the diols tested, it seems increasing toxicity correlates with increasing chain length and branching. The second part was characterization of pimelic acid tolerant strains from ALE, by shake flask cultivation and HPLC analysis of metabolites. In addi-tion, the genomes of 21 strains were resequenced. Results from the shake flask cultures showed that, in presence of pimelic acid, most strains have an impaired growth on non-fermentable carbon sources. Furthermore, HPLC analysis of metabolites revealed that glycerol and acetate accumulated during cultivation while ethanol was slowly consumed, implicating a defective respiratory system. Through genome resequencing, in total 47 genes were found to be mutated across all of the evolved strains.
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    Aggregation av Parkinsonproteinet -synuklein (vildtyp och sjukdomsvarianterna A30P och A53T) samt interaktion med liposomer
    (2017) Lorentzon, Emma; Olsson, Anna; Sundvall, Nathalie; Tingvall Gustafsson, Johanna; Torell Björkman, Agnes; Vånder, Frida; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Parkinsons sjukdom ¨ar en vanlig ˚aldersrelaterad neurodegenerativ sjukdom, som leder till b˚ade motoriska och kognitiva problem. Sjukdomen karakt¨ariseras av ab-normal ansamling av proteinaggregat, kallade Lewykroppar, inneh˚allande amyloida fibrer. Dessa fibrer best˚ar till stor del av proteinet α-synuklein, som fr¨amst ˚aterfinns i de presynaptiska nervterminalerna, d¨ar det interagerar med bland annat fosfolipider och andra molekyler. Syftet med projektet ¨ar att studera hur tre varianter av α-synuklein, vildtyp samt tv˚a sjukdomsalstrande mutationer, A30P och A53T, aggregerar samt interage-rar med liposomer. Liposomerna best˚ar av DOPC, DOPS, DOPE och kolesterol f¨or att efterlikna synaptiska vesiklar i hj¨arnan. Proteinstruktur samt aggregationskinetik in¨arvaro av liposomer unders¨oktes m.h.a. cirkul¨ar dikroism och fluorescenspektro-skopi. Studien visar att samtliga α-synukleinvarianter interagerar med liposomerna. Vildtypen och A53T-mutanten uppvisar en likartad strukturell f¨or¨andring, i form av en ¨okning av α-helixstruktur, i n¨arvaro av liposomer, medan A30P-mutanten uppvisade l¨agre grad av strukturf¨or¨andring. Aggregationskinetiken f¨or samtliga proteinvarianter inhiberas av de syntetiska liposomerna, vilket observeras m.h.a. tioflavin T fluorescens. Prov inneha˚llande enbart protein aggregerar snabbare ¨an i n¨arvaro av liposomer. Slutsatsen ¨ar att samtliga varianter av α-synuklein interagerar med membran-modellen, som inducerar en f¨or¨andring av deras sekund¨arstruktur. Aggregationen f¨or samtliga proteinvarianter inhiberas i n¨arvaro av membranmodellen.
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    Aggregation of α-synuclein in primary neuron models of Parkinson’s disease
    (2024) Allgén, Elin; Borg, Olivia; Chalmers tekniska högskola / Institutionen för life sciences; Chalmers University of Technology / Department of Life Sciences; Esbjörner Winters, Elin; Ghaeidamini, Marziyeh; Agholme, Lotta; Esbjörner Winters, Elin
    Parkinson’s disease (PD) is the second most prevalent neurodegenerative disorder, characterized by the progressive loss of dopaminergic neurons, leading to impaired motor function. In PD pathology, substantial evidence suggest that the neuronal loss is caused by the protein α-synuclein (α-syn) which aggregates into insoluble amyloid fibrils Mutations in the SNCA gene, encoding α-syn, can accelerate disease progression by enhancing the protein’s propensity to aggregate. Synthetic amyloid fibrils called pre-formed fibrils (PPFs) have recently been developed as a valuable tool for studying disease progression in vitro, by effectively induce endogenous aggregation in cells. In this project, five α-synuclein variants were studied: wild-type (WT) and pathological mutants A30P, E46K, H50Q, and A53T. The study aimed to characterize the biophysical properties of PFFs, identify differences among the variants, and assess their ability to induce endogenous α-syn aggregation and potential neurotoxicity. PFFs were generated and characterized using atomic force microscopy (AFM), circular dichroism (CD), and Thioflavin T fluorescence spectroscopy (ThT Assay). Cellular assays with primary cortical cultures from rat and mouse were then employed to evaluate cellular health, viability, and α-syn aggregation. This thesis demonstrated that within a given experiment PFFs could be generated and sonicated in a reproducible manner. Biophysical characterization revealed differences among the α-syn variants, including distinct morphologies, variations in monomer conversion to PFFs, and differences in fluorescence intensity and molar ellipticity. Furthermore, all α-syn variants induced endogenous aggregation in both cell models, with distinct aggregation patterns observed across variants and between models. E46K PFFs caused the highest level of aggregation in the mouse model without affecting cellular health, whereas A53T PFFs led to the highest aggregation in the rat model and impaired dendritic networks. H50Q induced minimal aggregation in both models, but negatively affected dendritic networks, suggesting potential neurotoxicity. Notably, aggregates induced by E46K displayed a distinct morphology compared to other variants. These findings highlight the complexity of α-syn pathology and suggest that different α-syn variants contribute uniquely to PD progression
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    Altered immune phenotype in patients with cirrhosis results in impaired vaccine-induced immunity following COVID-19 vaccination
    (2022) Blick, Elin; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Nygård, Yvonne; Martner, Anna
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    Anaerobic Digestion using Mini Reactors. Validation and optimization of analytical instruments for anaerobic bioprocesses
    (2020) Larsson, Yrsa; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Franzén, Carl-Johan; Habagil, Moshe
    I vattenreningsverk används anaerob nedbrytning för biologisk stabilisering av slamvattnet. I den anaeroba nedbrytningen skapas metan och koldioxid med andra ord biogas. Biogasen tas tillvara och kan användas som grön energikälla, men produktionen är inte alltid pålitlig i vilka mängder biogas som produceras. För att optimera och utveckla biogasproduktionen används småskaliga biogasreaktorer i laboratoriemiljöer. Fram tills idag så är det främst semikontinuerliga reaktorer som kommer till användning som behöver manuell matning och dataavläsning varje dag. VIVAB i Varberg har investerat i automatiska reaktorer som ska förenkla laborativa undersökningar med mindre spill, automatisk avläsning och ta bort det vardagliga manuella momentet. Målet med arbetet under den här rapporten, har varit att möjliggöra en ersättning av de semikontinuerliga reaktorerna med de optimerade automatiska reaktorerna. Vid uppstart av de automatiska reaktorerna uppkom flera problem, som upptäcktes via höga värden på de organiska fettsyrorna och låg biogasproduktion. Optimering av reaktorutformningen skedde genom följande korrigeringar. Identifiering och eliminering av gasläckor, utbyte av delar av utrustningen och utformning av ett rör som möjliggör utflöde från reaktorn. Reaktorerna var sammankopplade med en PLC controller som via en skärm tillät enkla förändringar av reaktorerna vad gäller matning, temperatur, mixning och kalibrering av gasmätare och flödespump. Resultat från reaktorerna sparades i realtid i PLC controller som registrerade mätdata från reaktorerna varje gång gasmätaren läste av gasproduktion. Gasmätaren uppvisade i några fall fel resultat då gasmätningsutrustningen fastnat och inte läste av biogasproduktionen. För att undvika utelämning av resultat sammankopplades ytterligare en gasmätare, μ-Flow som kunde påvisa uteblivna data och bidra till en pålitlig kalibrering av gasmätaren. De automatiska reaktorerna fungerade efter optimeringen mer eller mindre självgående med undantag för matning av slam var 4–5 dag. Detta innebär en stor minskning i arbetsbelastning vid laborationer och analyser vid optimering och utveckling av biogasproduktion som i efterhand kan appliceras på storskalig biogasproduktion.
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    Analysis of avenanthramides in oats with Ultra High Performance Liquid Chromatography
    (2016) Astner, Martin; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Avenanthramides have been shown to have beneficial properties such as strong antioxidant activity and anti-inflammatory effects in humans, and are a key defence molecule for oats. The goal of this project was to create and validate a method for quantification of avenanthramides in oats that would take less than 20 minutes. A new extraction method and new liquid chromatography method were tested, as well as the introduction of an internal standard to improve quantification. We found that the internal standard selected was not stable during extraction and that it was necessary to use an external standard curve. We found that the liquid chromatography method was reproducible for standard compounds and that we could get separation of the three main avenathramides in oats for a total run time of 15 minutes. The extraction component of the method requires further work to improve recovery and stability before this method can be used for quantification of avenanthramides in oats.
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    Antimicrobial silk
    (2016) Floderus Savonen, Lotta; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    Spider silk has shown potential for use as a biomaterial. If fused to antimicrobial peptides (AMPs), recombinant spider silk could be used for medical applications and reduce the need to use conventional antibiotics to battle infections. Recombinant spider silk 4RepCT was fused to the AMPs Magainin I, Lactoferricin and a synthetically derived AMP referred to as WGR. Polystyrene disks were coated with the AMP-silk fusion proteins and the disks were incubated with cultures of Staphylococcus aureus and Escherichia coli, to test the AMP-silks antimicrobial activity. All AMP-silk fusion proteins significantly decreased bacterial adhesion of S. aureus to the disks after 48 hours of incubation compared to uncoated disks. The Mag- and WGR-silks were e↵ective already after 24 hours. The recombinant silk itself seemed to have an antimicrobial e↵ect by reducing bacterial adhesion of both bacterial strains to the polystyrene disks. Results indicated that addition of the AMPs improved this e↵ect on S. aurues, but not on E.coli.
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    Användning av svenska makroalger som substrat för bioetanolproduktion
    (2015) Davidsson, Christoffer; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    This project investigates Saccharina latissima seaweeds, harvested in Sweden, as substrate for bioethanol fermentation. Saccharina latissima is also called sugar kelp and contains large amounts of the polysaccharide laminarin which was the target of interest in this project. The seaweed was milled before mixed with strong base followed by acid to extract the laminarin into a solution. After extraction, three methods for hydrolysing the laminarin into glucose were evaluated: sulphuric acid and autoclaving, commercial laminarinase enzyme, and enzymes from the naturally occuring bacterium Pseudoalteromonas sp. After hydrolysis fermentation was performed in small batches with a commercial strain of brewers' yeast. The results show that both sulphuric acid and enzymes from Pseudoalteromonas sp. did release glucose, which was successfully fermented into ethanol.
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    Artbestämning och karaktärisering av laktosväxande vildjäst från Nigeria
    (2022) Good, Johanna; Bellot Avendaño, Gelmy; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Geijer, Cecilia; Persson, Karl
    During cheese production, whey is a residual product, containing disaccharide lactose and other nutrients and minerals. Large quantities of whey must be disposed of yearly, which becomes costly since it requires further processing. The possibility of using microorganisms to convert this cheap and available resource into valuable bioproducts is an attractive approach. However, few known yeasts can perform this task without extensive genomic engineering. The discovery of yeast species that naturally produce valuable biochemicals could increase the value of whey in the industry. Therefore, from a large collection of wild Nigerian yeast isolates, our research sought to identify new yeast species that can grow on lactose. This was done by identifying species with DNA sequence data from a collection of ~6000 wild Nigerian yeast strains, were ~230 was found to grow on lactose. One representative isolate from 15 selected species were chosen for cultivating, HPLC-analysis, and literature review. The species were selected based on findings in literature such as usage in industry, bioproduct formation and biohazard level. The selected species include Apiotrichum mycotoxinovorans, Candida orthopsilosis, Candida pseudointermedia, Clavispora lusitaniae, Cutaneotrichosporon curvatum, Cyberlindnera fabianii, Kodamaea ohmeri, Meyerozyma caribbica, Meyerozyma carpophila, Moesziomyces antarcticus, Papiliotrema flavescens, Rhodotorula mucilaginosa, Trichosporon insectorum, Vishniacozyma taibaiensis and Yarrowia lipolytica. The literature research of this study revealed that all yeast species may have industrial potential, but more research is needed, especially for C. pseudointermedia, M. carpophila and V. taibaiensis, for which information was lacking. Species that produced fatty lipids deemed of special interest, due to the potential for future use in biotechnology. The result from the cultivation showed that half of the species grew well on lactose medium, which was backed up by the HPLC analysis. M. antarcticus was the only species which had greater growth in lactose medium than in glucose medium, and which also, shown trough the HPLC analysis, produced products that differed from other species. Although a few species showed good potential, further research is needed to determine if the species is suitable future industrial usage.
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    Assessment of fermentability of steam-pretreated spruce tips, needles and branches for bioethanol applications
    (2018) Asp, Tobias; Chalmers tekniska högskola / Institutionen för biologi och bioteknik; Chalmers University of Technology / Department of Biology and Biological Engineering
    The production of bioethanol from fermentation-based bioprocesses utilizing ligno-celluosic feedstocks is an option for replacing fossil based fuels. By using genetically modified yeasts that co-consume glucose and xylose, it is possible to ferment lingo-cellulosic materials such as spruce for bioethanol production. In this project the fermentability of spruce tips, needles and branches, pretreated by acid-catalyzed steam explosion according to a design of experiments plan, was evaluated in terms of ethanol titer, rate and yield as well as cell viability. In order to ferment the spruce tips, needles and branches, suÿcient cell concentrations are needed. A preculture method was developed where enough cells were produced and harvested in the same physiological state in di˙erent batches for simultaneous saccharification and co-fermentation. A anaerobic shake flask system was used to ferment the spruce tips, needles and branches. Final ethanol titers of up to 10 g l-1, average volumetric ethanol production rates of up to 0.35 g l-1 h-1 and final yields of ethanol on available glucose and on available glucose together with xylose of up to 0.19 gEthanol gGlucose-1 and 0.16 gEthanol gGlucose+Xylose-1 respectively were observed. The final cell concentrations, colony forming units and growth rates observed were all fairly low values of up to 3.00 x 105 cells ml-1, 1.19 x 107 CFU ml-1 and 2.36 x 10-2 h-1 respectively. Even though there may be some indications on preferable pretreatment conditions in terms of fermentability, more testing and experiments are required to make statisti-cally significant recommendations.However, trends observed in this project points to either high temperature and short time or low temperature and long time as prefer-able pretreatment process conditions. Materials pretreated under these conditions showed the highest final titers and yields.