Decolourization of azo dyes in textile wastewater by microbial processes

Türgay, Orcun

January 2010

Decolorization of Azo dyes in synthetic wastewater composition which is similar to real textile wastewater was carried out by microbial process. Experiments were performed in two continuous systems. Experiments were performed under anaerobic conditions in order to break the nitrogen bond of the azo group (-N=N-). A synthetic dye solution which contained 200 mg/L Reactive Black 5, 200 mg/L Procion Red MX-5B and 1 g/L yeast extract was prepared. In this study, living microorganisms were used to degrade the dyes in wastewater. Rice husks which contain bacteria and fungi were used in the reactors of continuous systems. The parameters tested on continuous system were wastewater composition, the number of reactors, the amount of yeast extract in wastewater composition, the wastewater flowrate, washing the system with wood chips solution, addition of yeast extract solution.  Results have shown that increasing the number of reactors, the retention time, the amount of yeast extract and washing the system with wood chips solution had positive effects for degradation of the dyes from wastewater. When the flowrate was increased the retention time has decreased so degradation of dyes has decreased but although the flowrate increased twice, % degradation hasn’t decreased as the same ratio. Therefore this result showed that this process can be worked for faster flowrates. Microbial process is a promising technology which might be used to treat wastewater containing azo dyes with good performance.

Azo dyes

microbial

lignocellulosic material

textile wastewater

Microbiology

Mikrobiologi

The role of 6C RNA in gene regulation in mycobacteria

Dexin, Zhou

January 2021

The Actinomycetes, to which the Mycobacterium genus belongs contains many pathogens, such as Mycobacterium tuberculosis, which can cause tuberculosis, so it has become a focus area in modern molecular biology research. Mycobacteria contain many proteins and regulatory factors, including tRNA, ncRNA and sRNA, which can help bacteria better adapt to the environment. Among them, 6C RNA is a stem-loop non-coding RNA, widely found in mycobacteria. According to previous studies, it may be involved in the rapid growth of mycobacteria. We aimed to clone the 6C RNA promoter region into the pIGn plasmid carrying lacZ reporter gene and transform the construct into Mycobacterium marinum, a close relative of M. tuberculosis. Then we analyzed the β-galactosidase activity of the transformed strain under different stress conditions to study the change of 6C RNA expression. At the same time, we recorded the growth curve and analyze expression changes of 6C RNA in the exponential growth phase and stationary phase of the transformed strain. In addition, we tried to clone the 6C RNA overexpression vector and to study the changes of gene expression at different growth stages, which will help us to better understand the role of 6C RNA in M. marinum.

Microbiology

Mikrobiologi

Fitness and virulence of epidemic and non-epidemic clones of extensively drug-resistant (XDR) carbapenemase-producing Klebsiella pneumoniae

Allander, Lisa

January 2018

No description available.

Microbiology in the medical area

Search for the Argonaute protein that governs miRNA regulation in Dictyostelium discoideum

Åström, Miranda

January 2021

MicroRNAs are small non-coding RNAs that regulate gene expression through RNA interference. These small RNAs enact gene silencing by forming a RNA-inducing silencing complex together with the effector protein Argonaute. The function of the Argonautes in the social amoeba Dictyostelium discoideum is not yet fully understood. In this study, we look closer at Argonaute B by investigating if it is possible to extract the protein from the cells by the addition of a polypeptide protein tag called 3xFlag. At the same time, we also look into if Argonaute B is important for cell growth. Sequences of the 3xFlag tag with or without the Argonaute B gene (agnB) attached had previously been cloned into a vector and transformed into Dictyostelium discoideum cell. The 3xFlag::agnB sequence was confirmed in wild type and agnB knock-out strains through polymerase chain reaction. We then verified the expression of the fusion protein in the cells by western blot. The cell growth was measured by how the number of cells changed over time. The experiment suggested that Argonaute B is important for growth. Our result show that the construct 3xFlag::agnB sequenced had correctly been transformed into the strains and is highly expressed under tested conditions. We could also see that Argonaute B is an important factor in cell growth.

Argonaute proteins

RNA interference

miRNA

3xFLAG-tag

Microbiology

Mikrobiologi

Utvärdering av fyra screeningmetoder för identifiering av kolistinresistens hos Escherichia coli och Klebsiella pneumoniae / Evaluation of four screening methods for the detection of colistin-resistant Escherichia coli and Klebsiella pneumoniae

Axelsson, Emma

January 2020

Multiresistens hos gramnegativa bakterier är ett stort problem i stora delar av världen. Avsaknaden av nya preparat har resulterat i återintroduktion av ett tidigare stoppat antibiotikum, kolistin, men dessvärre kantas resistensbestämningen av flertalet problem. Kolistin är en positivt laddad molekyl som binder till lipid A i yttermembranet, vilket destabiliseras och resulterar i celldöd. Flertalet resistensmekanismer mot kolistin finns beskrivna och majoriteten resulterar i förändrad lipid A-struktur, vilket leder till försämrad kolistininbindning. Syftet med examensarbetet var att utvärdera fyra potentiella screeningmetoder för att upptäcka kolistinresistens och jämföra resultaten mot buljongspädning som referensmetod. De fyra screeningmetoderna var buljongeluering och diskdiffusion samt de kommersiellt tillgängliga screeningtesterna Superpolymyxin och Rapid polymyxin NP. Totalt analyserades 57 helgenomsekvenserade Enterobacterales, varav 28 Escherichia coli och 29 Klebsiella pneumoniae, där aktuella resistensmekanismer var kända. Samtliga isolat analyserades en gång per metod och utöver detta analyserades även tre kontrollstammar. Vid buljongspädning erhölls värde för minsta inhiberande koncentration (MIC) kolistin, vilket användes för klassificering som känslig (MIC ≤ 2 mg/l) eller resistent (MIC > 2 mg/l). De fyra screeningtesterna var designade för att upptäcka resistenta isolat och innehöll 2–4 mg/l kolistin. Resultaten från screeningtesterna var kvalitativa och känslighetskategoriserade isolaten. Sensitivitet och specificitet beräknades för metoderna. Högst sensitivitet (100 %) noterades för Superpolymyxin och Rapid polymyxin NP, och lägst specificitet (76 %) för buljongeluering. Med hänsyn till resultat, prevalens, hållbarhets-, tids- och kostnadseffektivitet drogs slutsatsen att Rapid polymyxin NP är bästa alternativet som screeningmetod av utvärderade metoder. / Infections due to multidrug resistant Gram-negative bacteria are a major problem in large parts of the world. Due to lack of treatment options, a previously banned antibiotic, colistin, has been reintroduced. Unfortunately, susceptibility testing of colistin is problematic and currently the only recommended method is broth microdilution (BMD). Colistin is a positively charged molecule that binds to lipid A at the negatively charged outer cell membrane, which leads to cell disruption. Several mutations causing colistin resistance have been identified, most of them cause alterations of lipid A, resulting in impaired colistin outer cell membrane interaction. The aim of this study was to evaluate four potential screening methods for colistin resistance and compare the results with BMD (reference method). The four screening methods were broth disk elution, disk diffusion and the commercially available tests Superpolymyxin and Rapid polymyxin NP. A collection of 57 whole genome sequenced Enterobacterales consisting of 28 Escherichia coli and 29 Klebsiella pneumoniae were included in the study. Reference results were obtained by BMD, where the estimated minimum inhibitory concentration (MIC) values were used for classification of the isolates as sensitive (MIC ≤ 2 mg/l) or resistant (MIC > 2 mg/l). Sensitivity and specificity were calculated for the methods. The highest sensitivity (100 %) was noted for Superpolymyxin and Rapid polymyxin NP, and the lowest specificity (76 %) for broth disk elution. Considering the results, prevalence, durability, time and cost efficiency, it was concluded that Rapid polymyxin NP is the best alternative as a screening method of evaluated methods.

Susceptibility testing

broth microdilution

colistin

Antibiotikaresistensbestämning

buljongspädning

kolistin

Microbiology

Mikrobiologi

Inventering av läroplan och kurslitteratur för Bioteknik

Jakobsson, Jens

January 2003

The criteria for the gymnasial course in Biotechnics (BI1209) are analysed and a detailed plan of the course is suggested. Course litterature is evaluated. / I arbetet görs en konkretisering av kursplanen för Bioteknik (BI1209). Alternativ till kurslitteratur analyseras utifrån denna konkretisering.

bioteknik

BI1209

kursplan

genteknik

mikrobiologi

kursböcker

naturvetenskap

Social Sciences

Samhällsvetenskap

Bioteknikkursen i NV3 Innehåll och metoder

Ekholm, Dag

January 2004

Utformning och innehåll i kursen bioteknik BI1209 i NV3 undersöks genom en enkät besvarad av 26 gymnasier. Arbetsformer, läromedel, laborationer, utvärdering kartläggs.

biologi

biologididaktik

bioteknik

genteknik

mikrobiologi

NV-programmet

Social Sciences

Samhällsvetenskap

Study of Putative RNA-Binding Proteins in Escherichia coli.

Lindholm, Axel

January 1900

No description available.

Microbiology in the medical area

Methanobacterium cauma sp. nov., a hydrogenotrophic, halotolerant methanogen from an active serpintinization system at Chimaera seep

Stephens, Aubree

January 2023

The archaeal branch of life represents some of the oldest life forms on Earth. Archaea are believed to have diverged from Prokaryotes roughly 3.5 billion years ago and it’s theorized that biological methane production started around this time as well. This would make methanogenesis one of the oldest metabolisms on our planet. Methanogenesis is a process that, so far, is known to be unique to archaea. Since their evolution, methanogens have had massive impacts on Earth’s climate and biology. Methane is an important part of the global carbon cycle, but is also a major greenhouse gas, making it a vital area of research. The methanogen studied in this thesis is referred to as the wild type (WT) and was isolated from an active serpentinization system at Chimaera seep in Çıralı, Antalya Gulf, Turkey. The Chimaera seep is a geological formation analogous to mid-ocean ridges, but exposed and above land. The research in this thesis focuses on the description of the WT, which is believed to be a new species. Describing the WT consisted of the characterization of extremes as well as optimal growth conditions. The WT was found to grow at initial pH levels of 9.0 and 9.5. It grew from 15 °C to 45 °C, but not at 47 °C and not at 12 °C, and had an optimum at 39 °C. The WT had measurable growth up to 40 g/L NaCl, and had its optimum at 0 g/L. The WT grew best with H2/CO2 substrate, but also grew well on formate.

methanogen

archaea

hydrogenotroph

halotolerant

Methanobacterium

Chimaera seep

methanogenesis

Microbiology

Mikrobiologi

The role of Fragile-X mental retardation-related protein 1 in Human Adenovirus 5 infection

Kaira, Yanina

January 2021

The Fragile X-related mental retardation 1 (FXR1) is an N6-Methyladenosine reader involved in mRNAs metabolism like mRNA splicing, stability, transport, and miRNA regulation. It is also important in transcription, cell proliferation, differentiation, translation, polysome assembly and stress granule assembly. The protein is present in all eukaryotic cells, but so far it has been specifically essential for correct neural function. Until now, FXR1 has not been investigated in the concept of Human Adenovirus infection but we have observed an upregulation of FXR1 during the late phase of the Human Adenovirus 5 (HAdV-5) infection and an upregulation of some late HAdV-5 proteins in HeLa cells overexpressing FXR1. Our results furthermore showed that a FXR1 knockdown resulted in a reduced level of some HAdV-5 proteins at the same time as HAdV-5 mRNA were stabilized, indicating that FXR1 might be involved in translation of HAdV-5 late genes. Further investigation of the mechanism behind FXR1 mediated translation, a Death-associated protein 5 (DAP5) was founded to have an overall effect on the translation of HAdV-5 late proteins. / Part of a post-doctoral research

Adenovirus

HAdV-5

FXR1

DAP5

NAT1

p97

Microbiology

Mikrobiologi