ABSTRACT
Marine plastic debris is widely recognized as a global environmental issue. Small microplastic particles, with an upper size limit of 20 µm, have been identified as having the highest potential for causing damage to marine ecosystems. Having accurate methods for quantifying the abundance of such particles in a natural environment is essential for defining the extent of the problem they pose. Using an optical micro-Raman tweezers setup, we have identified the composition of particles trapped in marine aggregates collected from the coastal surface waters around the subtropical island of Okinawa. Chemical composition analysis at the single-particle level indicates dominance by low-density polyethylene, which accounted for 75% of the small microplastics analysed. The smallest microplastics identified were (2.53 ± 0.85) µm polystyrene. Our results show the occurrence of plastics at all test sites, with the highest concentration in areas with high human activities. We also observed additional Raman peaks on the plastics spectrum with decreasing debris size which could be related to structural modification due to weathering or embedding in organic matter. By identifying small microplastics at the single-particle level, we obtain some indication on their dispersion in the ocean which could be useful for future studies on their potential impact on marine biodiversity.
ABSTRACT
Plastic products contribute heavily to anthropogenic pollution of the oceans. Small plastic particles in the microscale and nanoscale ranges have been found in all marine ecosystems, but little is known about their effects upon marine organisms. In this study, we examine changes in cell growth, aggregation, and gene expression of two symbiotic dinoflagellates of the family Symbiodiniaceae, Symbiodinium tridacnidorum (clade A3), and Cladocopium sp. (clade C) under exposure to 42-nm polystyrene beads. In laboratory experiments, the cell number and aggregation were reduced after 10 days of nanoplastic exposure at 0.01, 0.1, and 10 mg/L concentrations, but no clear correlation with plastic concentration was observed. Genes involved in dynein motor function were upregulated when compared to control conditions, while genes related to photosynthesis, mitosis, and intracellular degradation were downregulated. Overall, nanoplastic exposure led to more genes being downregulated than upregulated and the number of genes with altered expression was larger in Cladocopium sp. than in S. tridacnidorum, suggesting different sensitivity to nano-plastics between species. Our data show that nano-plastic inhibits growth and alters aggregation properties of microalgae, which may negatively affect the uptake of these indispensable symbionts by coral reef organisms.
ABSTRACT
Dinoflagellates are some of the most common eukaryotic cells in the ocean, but have very unusual nuclei. Many exhibit a form of closed mitosis (dinomitosis) wherein the nuclear envelope (NE) invaginates to form one or more trans-nuclear tunnels. Rather than contact spindles directly, the chromatids then bind to membrane-based kinetochores on the NE. To better understand these unique mitotic features, we reconstructed the nuclear architecture of Polykrikos kofoidii in 3D using focused ion beam scanning electron microscopy (FIB-SEM) in conjunction with high-pressure freezing, freeze-substitution, TEM, and confocal microscopy. We found that P. kofoidii possessed six nuclear tunnels, which were continuous with a reticulating network of membranes that has thus far gone unnoticed. These membranous extensions interconnect the six tunnels while ramifying throughout the nucleus to form a "nuclear net." To our knowledge, the nuclear net is the most elaborate endomembrane structure described within a nucleus. Our findings demonstrate the utility of tomographic approaches for detecting 3D membrane networks and show that nuclear complexity has been underestimated in Polykrikos kofoidii and, potentially, in other dinoflagellates.
Subject(s)
Chromosome Segregation/physiology , Dinoflagellida/physiology , Nuclear Envelope/physiology , Spindle Apparatus/physiology , Dinoflagellida/metabolism , Endoplasmic Reticulum/physiology , Microscopy, Confocal , Microscopy, Electron, Scanning/methods , Microscopy, Electron, Transmission , Mitosis/physiologyABSTRACT
We examine the origin of harpoon-like secretory organelles (nematocysts) in dinoflagellate protists. These ballistic organelles have been hypothesized to be homologous to similarly complex structures in animals (cnidarians); but we show, using structural, functional, and phylogenomic data, that nematocysts evolved independently in both lineages. We also recorded the first high-resolution videos of nematocyst discharge in dinoflagellates. Unexpectedly, our data suggest that different types of dinoflagellate nematocysts use two fundamentally different types of ballistic mechanisms: one type relies on a single pressurized capsule for propulsion, whereas the other type launches 11 to 15 projectiles from an arrangement similar to a Gatling gun. Despite their radical structural differences, these nematocysts share a single origin within dinoflagellates and both potentially use a contraction-based mechanism to generate ballistic force. The diversity of traits in dinoflagellate nematocysts demonstrates a stepwise route by which simple secretory structures diversified to yield elaborate subcellular weaponry.
