Biochemical reconstitution of branching microtubule nucleation

Alfaro-Aco, Raymundo; Thawani, Akanksha; Petry, Sabine

doi:10.1101/700047

Cited by 15 publications

(26 citation statements)

References 37 publications

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“…7, graph). Indeed, recent reconstitution experiments have shown that sites of condensation may serve as branch points for new MTs 21 .…”

Section: Discussionmentioning

confidence: 99%

“…See also Supplementary Fig. 5e first be deposited on MTs for augmin to be recruited 21,22 . Furthermore, TPX2 interacts with the tetrameric kinesin Eg5 30,43 , which was recently demonstrated to promote MT nucleation in vitro 44 .…”

Section: Discussionmentioning

confidence: 99%

“…Branching MT nucleation requires the universal MT nucleator module, consisting of the γ-Tubulin Ring Complex (γ-TuRC) 15,16 and its recently discovered co-factor XMAP215 [17][18][19] , as well as the protein complex augmin that directly recruits γ-TuRC along the length of a pre-existing MT 20 . Branching MT nucleation is initiated by the MT-associated protein TPX2 10 , which has been proposed to both recruit augmin to MTs 21,22 and activate γ-TuRC via TPX2's C-terminal domain 23,24 . In vitro, TPX2 can directly generate MTs from tubulin via its N-terminal domain 25,26 , but this domain is dispensable for MT nucleation in the cytosol 23,27 .…”

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confidence: 99%

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Phase separation of TPX2 enhances and spatially coordinates microtubule nucleation

2020

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Phase separation of substrates and effectors is proposed to enhance biological reaction rates and efficiency. Targeting protein for Xklp2 (TPX2) is an effector of branching microtubule nucleation in spindles and functions with the substrate tubulin by an unknown mechanism. Here we show that TPX2 phase separates into a co-condensate with tubulin, which mediates microtubule nucleation in vitro and in isolated cytosol. TPX2-tubulin co-condensation preferentially occurs on pre-existing microtubules, the site of branching microtubule nucleation, at the endogenous and physiologically relevant concentration of TPX2. Truncation and chimera versions of TPX2 suggest that TPX2-tubulin co-condensation enhances the efficiency of TPX2-mediated branching microtubule nucleation. Finally, the known inhibitor of TPX2, the importin-α/β heterodimer, regulates TPX2 condensation in vitro and, consequently, branching microtubule nucleation activity in isolated cytosol. Our study demonstrates how regulated phase separation can simultaneously enhance reaction efficiency and spatially coordinate microtubule nucleation, which may facilitate rapid and accurate spindle formation.

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“…7, graph). Indeed, recent reconstitution experiments have shown that sites of condensation may serve as branch points for new MTs 21 .…”

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 99%

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Phase separation of TPX2 enhances and spatially coordinates microtubule nucleation

2020

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“…Compared to interphase, mitotic microtubules are shorter and more dynamic; they are nucleated from γ-tubulin complexes either at centrosomes or along pre-existing MTs [1]. Away from centrosomes, MT nucleation requires Ran-dependent liberation of spindle assembly factors such as TPX2, HURP, or NuSAP, together with augmin complexes that are assembled along preexisting microtubules [1,2,3,4,5]. At kinetochores, microtubules interact with several microtubule-associated proteins (MAPs, including microtubule-dependent motors), and appear as cold-resistant MT bundles called kinetochore-fibers (k-fibers) [6].…”

Section: The Biological Contextmentioning

confidence: 99%

How Does SUMO Participate in Spindle Organization?

Abrieu

Liakopoulos

2019

Cells

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The ubiquitin-like protein SUMO is a regulator involved in most cellular mechanisms. Recent studies have discovered new modes of function for this protein. Of particular interest is the ability of SUMO to organize proteins in larger assemblies, as well as the role of SUMO-dependent ubiquitylation in their disassembly. These mechanisms have been largely described in the context of DNA repair, transcriptional regulation, or signaling, while much less is known on how SUMO facilitates organization of microtubule-dependent processes during mitosis. Remarkably however, SUMO has been known for a long time to modify kinetochore proteins, while more recently, extensive proteomic screens have identified a large number of microtubule- and spindle-associated proteins that are SUMOylated. The aim of this review is to focus on the possible role of SUMOylation in organization of the spindle and kinetochore complexes. We summarize mitotic and microtubule/spindle-associated proteins that have been identified as SUMO conjugates and present examples regarding their regulation by SUMO. Moreover, we discuss the possible contribution of SUMOylation in organization of larger protein assemblies on the spindle, as well as the role of SUMO-targeted ubiquitylation in control of kinetochore assembly and function. Finally, we propose future directions regarding the study of SUMOylation in regulation of spindle organization and examine the potential of SUMO and SUMO-mediated degradation as target for antimitotic-based therapies.

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“…The ringshaped g-tubulin complex (g-TuRC) serves as the structural template for the initial tubulin assembly, thereby accelerating the initial lag phase (Zheng et al, 1995). However, the g-2 TuRC alone is not an efficient MT nucleator, and efficient nucleation requires association with other proteins, such as CDK5RAP2, XMAP215/ch-TOG, TPX2, and augmin (Alfaro-Aco et al, 2020;Choi et al, 2010;Consolati et al, 2020;Flor-Parra et al, 2018;Tariq et al, 2020;Thawani et al, 2018). Some of these activators likely alter the conformation of g-TuRC to better fit the ends of MT protofilaments (Consolati et al, 2020;Liu et al, 2020;Wieczorek et al, 2020), whereas others cooperate with g-TuRC (Consolati et al, 2020;Flor-Parra et al, 2018;King et al, 2020;Thawani et al, 2018).…”

Section: Introductionmentioning

confidence: 99%

Microtubule-associated proteins promote microtubule generation in the absence of γ-tubulin in human colon cancer cells

Tsuchiya

Goshima

2021

Preprint

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γ-Tubulin complex acts as the predominant microtubule (MT) nucleator that initiates MT formation and is therefore an essential factor for cell proliferation. Nonetheless, cellular MTs are formed after experimental depletion of the γ-tubulin complex, suggesting that cells possess other factors that drive MT nucleation. Here, by combining gene knockout, auxin-inducible degron, RNA interference, MT depolymerisation/regrowth assay, and live microscopy, we identified four microtubule-associated proteins (MAPs), ch-TOG, CLASP1, CAMSAPs, and TPX2, which are involved in γ-tubulin-independent MT generation in human colon cancer cells. In the mitotic MT regrowth assay, nucleated MTs organised non-centriolar MT organising centres (ncMTOCs) in the absence of γ-tubulin. Depletion of CLASP1 or TPX2 substantially delayed ncMTOC formation, suggesting that they promote MT nucleation in the absence of γ-tubulin. In contrast, depletion of CAMSAPs or ch-TOG did not affect the timing of ncMTOC appearance. CLASP1 also accelerates γ-tubulin-independent MT regrowth during interphase. Thus, MT generation can be promoted by MAPs without the γ-tubulin template.

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Biochemical reconstitution of branching microtubule nucleation

Cited by 15 publications

References 37 publications

Phase separation of TPX2 enhances and spatially coordinates microtubule nucleation

Phase separation of TPX2 enhances and spatially coordinates microtubule nucleation

How Does SUMO Participate in Spindle Organization?

Microtubule-associated proteins promote microtubule generation in the absence of γ-tubulin in human colon cancer cells

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