Acronym NA
Category
Marine Biotechnology
Title Å bygge et glasshus: Undersøkelse av grunnleggende komponenter i biomineralisering av cellevegg hos kiselalger - How to build a glass house: Revealing fundamental components of diatom cell wall biomineralization Programme National Programme
Instrument (FP6)
Contact Type (FP7)
Strand (Interreg)
NA
Theme (FP7)
Activity Area (FP6)
Regional Area (Interreg)
Action (COST)
NA
Specific Programme (FP7)
NA
Funding source National Coordinator Olav Vadstein Coordinator email olav.vadstein@ntnu.no
Coordinator institution
NTNU - Norwegian University of Science and Technology (Norway)
Institutions involved
NA
Start year 2018 End year 2022 Funding (€) € 985,770 Website https://prosjektbanken.forskningsradet.no/project/FORISS/276085?Kilde=FORISS&distribution=Ar&chart=bar&calcType=funding&Sprak=no&sortBy=date&sortOrder=desc&resultCount=30&offset=0&ProgAkt.3=FRIBIO2-FRIPRO%20forskerprosjekt%2C%20biologi&source=FORISS&projectId=274635 Summary Biomineralization, the formation of complex inorganic structures by organisms, is a widely distributed process in nature. One of the most spectacular examples of biomineralization is the diatom cell wall (frustule), which is a three-dimensional silica structure with intricate, species-specific patterns ranging from nano- to micrometer scale. While a number of proteins have been identified that take part in the deposition and patterning of silica within a specialized compartment (the silica deposition vesicle, SDV), the process as a whole is poorly understood. There is extensive interaction between the inside of the SDV and cytosolic factors such as the cytoskeleton, but the mechanisms of these interactions are unknown.
We have identified a gene family restricted to diatoms that encodes predicted transmembrane proteins with a yet uncharacterised domain. Several lines of evidence suggest that members of this protein family, termed Silicanins, are localized to the SDV membrane, and that they are involved in frustule biosynthesis. In this project, we aim to investigate the roles of the Silicanin-D subfamily in cell wall biomineralization, using state-of-the-art molecular, biochemical and imaging techniques.
We will generate deletion series of the Silicanin-D subfamily members using CRISPR/Cas9-based genome editing. Silica production and frustule patterning, structure and chemical composition will be analysed in these mutants as well as overexpression lines. The intracellular localization and dynamics of Silicanin-D members and their possible interaction with the cytoskeleton and other proteins will be studied. Finally, recombinant Silicanin-D proteins will be analysed for direct or indirect effect on silica formation activity.
The results from this project will increase knowledge on a fundamental process in the ecologically important diatoms, and could form the basis for a system to customize frustule structures for commercial applications.
Keywords
Bioprospecting;
Protein;
Biomimicry;
Genetic;
Bioproduct;
Engineering;
Genomic;
Marine Region
76
Not associated to marine areas
0
Marine Region Map
