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Sökning: WFRF:(Herbst Harald)

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1.
  • Bergström, Gunnar, et al. (författare)
  • Durability testing for 100 year lifetime for buried non-pressure plastic pipes
  • 2006
  • Ingår i: Plastics Pipes XIII.
  • Konferensbidrag (refereegranskat)abstract
    • For plastics pipes used for underground drainage and sewerage there is at present no internationally accepted method for the evaluation of durability. This makes it difficult to make an objective assessment for both new materials and new pipe designs entering the market. This paper presents a possible future structure of such a durability evaluation for nonpressure pipes. Based on an experimental study of pipes made from a filled and an unfilled PP material and one made from an HDPE material different damage mechanisms and changes in pipe characteristics were observed when the pipes were exposed to long-term deflection and long term (one-year) ageing at +95 °C. A CAED methodology is also described which was used to investigate the distribution and time dependence of pipe stresses.
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2.
  • Johansson, Mikaela (författare)
  • Metaproteogenomics-guided enzyme discovery : Targeted identification of novel proteases in microbial communities
  • 2018
  • Doktorsavhandling (övrigt vetenskapligt/konstnärligt)abstract
    • Industrial biotechnology is a large and growing industry as it is part of establishing a “greener” and more sustainable bioeconomy-based society. Using enzymes as biocatalysts is a viable alternative to chemicals and energy intense industrial processes and is en route to a more sustainable industry. Enzymes have been used in different areas for ages and are today used in many industrial processes such as biofuels production, food industry, tanning, chemical synthesis, pharmaceuticals etc. Enzymes are today a billion-dollar industry in itself and the demand for novel catalysts for various present and future processes of renewable resources are high and perfectly in line with converting to a more sustainable society.Most enzymes used in industry today have been identified from isolated and pure cultured microorganisms with identified desirable traits and enzymatic capacities. However, it is known that less than 1% of all microorganisms can be can be obtained in pure cultures. Thus, if we were to rely solely on pure culturing, this would leave the 99% of the microorganisms that constitutes the “microbial dark matter” uninvestigated for their potential in coding for and producing valuable novel enzymes. Therefore, to investigate these “unculturable” microorganisms for novel and valuable enzymes, pure-culture independent methods are needed.During the last two decades there has been a fast and extensive development in techniques and methods applicable for this purpose. Especially important has been the advancements made in mass spectrometry for protein identification and next generation sequencing of DNA. With these technical developments new research fields of proteomics and genomics have been developed, by which the complete protein complement of cells (the proteome) and all genes (the genome) of organisms can be investigated. When these techniques are applied to microbial communities these fields of research are known as meta-proteomics and meta-genomics.However, when applied to complex microbial communities, difficulties different from those encountered in their original usage for analysis of single multicellular organisms or cell linages arises, and when used independently both methods have their own limitations and bottlenecks. In addition, both metaproteomics and metagenomics are largely non-targeting techniques. Thus, if the purpose is still to - somewhat contradictory – use these non-targeting methods for targeted identification of novel enzymes with certain desired activities and properties from within microbial communities, special measures need to be taken.The work presented in this thesis describes the development of a method that combinesmetaproteomics and metagenomics (i.e. metaproteogenomics) for the targeted discovery of novel enzymes with desired activities, and their correct coding genes, from within microbial communities. Thus, what is described is a method that can be used to circumvent the pure-culturing problem so that a much larger fraction of the microbial dark matter can be specifically investigated for the identification of novel valuable enzymes.
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