Abstract
SAS-6 proteins are thought to impart the ninefold symmetry of centrioles, but the mechanisms by which their assembly occurs within cells remain elusive. In this paper, we provide evidence that the N-terminal, coiled-coil, and C-terminal domains of HsSAS-6 are each required for procentriole formation in human cells. Moreover, the coiled coil is necessary and sufficient to mediate HsSAS-6 centrosomal targeting. High-resolution imaging reveals that GFP-tagged HsSAS-6 variants localize in a torus around the base of the parental centriole before S phase, perhaps indicative of an initial loading platform. Moreover, fluorescence recovery after photobleaching analysis demonstrates that HsSAS-6 is immobilized progressively at centrosomes during cell cycle progression. Using fluorescence correlation spectroscopy and threedimensional stochastic optical reconstruction microscopy, we uncover that HsSAS-6 is present in the cytoplasm primarily as a homodimer and that its oligomerization into a ninefold symmetrical ring occurs at centrioles. Together, our findings lead us to propose a mechanism whereby HsSAS-6 homodimers are targeted to centrosomes where the local environment and high concentration of HsSAS-6 promote oligomerization, thus initiating procentriole formation.
| Original language | English |
|---|---|
| Pages (from-to) | 697-712 |
| Number of pages | 16 |
| Journal | Journal of Cell Biology |
| Volume | 204 |
| Issue number | 5 |
| DOIs | |
| Publication status | Published - 1 Jan 2014 |
| Externally published | Yes |
Keywords
- ACF, autocorrelation function
- ANOVA, analysis of variance
- CPM, counts per molecule
- EdU, 5-ethynyl-2?-deoxyuridine
- FCS, fluorescence correlation spectroscopy
- FL, full length
- FP, fluorescent protein
- PCM, pericentriolar material
- PCNA, proliferating cell nuclear antigen
- Px, pixel
- STORM, stochastic optical reconstruction microscopy
- WCE, whole-cell extract
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