ABSTRACT
Diatoms contribute 20% of global primary production and form the basis of many marine food webs. Although their species diversity correlates with broad diversity in cell size, there is also an intraspecific cell-size plasticity owing to sexual reproduction and varying environmental conditions. However, despite the ecological significance of the diatom cell size for food-web structure and global biogeochemical cycles, our knowledge about genes underpinning the size of diatom cells remains elusive. Here, a combination of reverse genetics, experimental evolution and comparative RNA-sequencing analyses enabled us to identify a previously unknown genetic control of cell size in the diatom Thalassiosira pseudonana. In particular, the targeted deregulation of the expression of the cell-wall protein silacidin caused a significant increase in valve diameter. Remarkably, the natural downregulation of the silacidin gene transcript due to experimental evolution under low temperature also correlated with cell-size increase. Our data give first evidence for a genetically controlled regulation of cell size in T. pseudonana and possibly other centric diatoms as they also encode the silacidin gene in their genomes.
Subject(s)
Cell Wall/metabolism , Diatoms/metabolism , Proteins/metabolism , Cell Size , Cell Wall/genetics , Diatoms/cytology , Diatoms/genetics , Gene Expression Regulation , Genome , Proteins/geneticsABSTRACT
Diatoms are unicellular algae of enormous biodiversity that occur in all water habitats on earth. Their cell walls are composed of amorphous biosilica and exhibit species-specific nanoporous to microporous and macroporous patterning. Therefore, diatom biosilica is a promising renewable material for various applications, such as in catalysis, drug-delivery systems, and biophotonics. In this study, diatom biosilica of three different species (Stephanopyxis turris, Eucampia zodiacus, and Thalassiosira pseudonana) was used as support material for gold nanoparticles using a covalent coupling method. The resulting catalysts were applied for the oxidation of d-glucose to d-gluconic acid. Because of its high specific surface area, well-established transport pores, and the presence of small, homogeneously distributed gold nanoparticles on the surface, diatom biosilica provides a highly catalytically active surface and advanced accessibility to the active sites. In comparison to those of the used reference supports, higher catalytic activities (up to 3.28 × 10-4 mmolGlc s-1 mgAu -1 for T. pseudonana biosilica) and slower deactivation were observed for two of the diatom biosilica materials. In addition, diatom biosilica showed very high gold-loading capacities (up to 45 wt %), with a homogeneous nanoparticle distribution.