Embryogenesis is one of the most delicate biological processes which requires precise control in various levels, including molecular distribution and gene expression, cellular orientation and specification, and tissue dynamics giving rise to proper morphology. The diverse animal morphology can be resulted from the difference during early embryonic cleavages. Spiral cleavage is a conserved embryonic patterning strategy used in the majority of the animal clade Spiralia. The specific cell positioning during cell division and quadrant-based clonal domain formation make the embryos with the blastomeres orientated in a spiral manner when viewing from the animal pole. Although spiral cleavage is conserved in many phyla, the detailed cellular, molecular and biophysical mechanisms for this left-right symmetry breaking event remain unclear.
Here I studied the early development of the prototypic annelid spiral-cleaver Platynereis dumerilii, which performs two unequal embryonic cleavages followed by the first dextral spiral cleavages, and compared the mechanisms to other spiralians or to other cleavage types. First, I described the morphology of each cell cycle from the zygote until 64-cell stage by imaging the fluorescently labeled fixed embryos. Second, with mRNA injection, whole-embryo live-imaging with Selective Plane Illumination Microscopy (SPIM), and in silico cell tracking, I monitored these cleavages in 4-D, constructed the early cell lineages, and revealed the subtle asynchrony of the four quartets. Third, together with the spindle inclination angle measurement, I discovered the leading role of the D macromere during P. dumerilii spiral cleavage. I also confirmed that the dextral micromere orientation is neither affected by the eggshell nor the presence of all the neighbor macromeres, suggesting that this cellular property may be achieved by cell autonomous molecular mechanisms.
In order to quantify the candidate cytoskeletal dynamics during spiral cleavage, I optimized the construction of the injected mRNAs and the injection protocol to achieve the highest translational level of the fluorescent protein within a given developmental time. Beside mRNA injection, I also established a protein expression and injection protocol for P. dumerilii protein injection in order to visualize the target gene as early as possible. Both techniques didn’t dramatically influence embryogenesis and allow for quantification of the protein dynamics. With these strategies, I discovered and measured the chiral counter rotational flow of cortical actomyosin in each spiral cleavage and revealed that it’s present in the first two spiral cleavages, especially of the macromeres. The biophysical force generated by actomyosin contributes in the cell deformation and spindle inclination, resulting in proper dextral micromere positioning, during the first spiral cleavage, confirmed by the chemical treatment to the P. dumerilii embryos. The asymmetric actomyosin distribution, nuclei migration, and the change of the cell axes during cytokinesis in the macromeres also suggests that the macromeres may play critical roles to lead spiral cleavage.
This work is built on the knowledge of the spiral cleavage machinery and has extended it in multiple dimensions. The detailed phase-by-phase description of each cleavage increases the information of P. dumerilii embryogenesis. The established labeling and imaging techniques in this thesis are the important basis for investigation and comparisons of different spiralian development in the future. More broadly, the discovery of actomyosin dynamics shows conservation to the left-right symmetry breaking events of the animals which does not belong to Spiralia. These together bring insights to a global evolutionary speculation: a conserved mechanical force generation pathway, tuned by the upstream molecular signals, may be the key of the miscellaneous cleavage types, resulting in the astonishing variety of embryo patterning.
| Identifer | oai:union.ndltd.org:DRESDEN/oai:qucosa:de:qucosa:72836 |
| Date | 20 November 2020 |
| Creators | Hsieh, Yu-Wen |
| Contributors | Tomancak, Pavel, Technische Universität Dresden |
| Source Sets | Hochschulschriftenserver (HSSS) der SLUB Dresden |
| Language | English |
| Detected Language | English |
| Type | info:eu-repo/semantics/publishedVersion, doc-type:doctoralThesis, info:eu-repo/semantics/doctoralThesis, doc-type:Text |
| Rights | info:eu-repo/semantics/openAccess |
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