Abstract:10We investigate the mechanisms of planar cell polarity (PCP) in the larval epidermis of 11 Drosophila. Measurements of the amount of Dachsous across the segment find a peak 12 located near the rear of the anterior compartment. Localisation of Dachs and 13 orientation of ectopic denticles reveal the polarity of every cell in the segment. We 14 discuss how well these findings evidence a zigzag gradient model of Dachsous activity. 15 Several groups have proposed that Dachsous and Fat fix the direction of PCP … Show more
“…Namely, we demonstrated that the overall direction of microtubules follows the cell's long axis whereas the alignment of microtubules with each other is consistent with the cell eccentricity in agreement with the robustness of this alignment previously reported (Płochocka et al, 2021). A similar role for cell shape in organising microtubule polarity independently of Ft-Ds polarity has also been suggested in the Drosophila larval epidermis (Pietra et al, 2020).…”
In epithelial cells, planar polarisation of subapical microtubule networks is thought to be important for both breaking cellular symmetry and maintaining the resulting cellular polarity. Studies in the Drosophila pupal wing and other tissues have suggested two alternative mechanisms for specifying network polarity. On one hand mechanical strain and/or cell shape have been implicated as key determinants, on the other the Fat-Dachsous planar polarity pathway has been suggested to be the primary polarising cue. Using quantitative image analysis in the pupal wing, we reassess these models. We found that cell shape was a strong predictor of microtubule organisation in the developing wing epithelium. Conversely Fat-Dachsous polarity cues do not play any direct role in the organisation of the subapical microtubule network, despite being able to weakly recruit the microtubule minus-end capping protein Patronin to cell boundaries. We conclude that any effect of Fat-Dachsous on microtubule polarity is likely to be indirect, via their known ability to regulate cell shape.
“…Namely, we demonstrated that the overall direction of microtubules follows the cell's long axis whereas the alignment of microtubules with each other is consistent with the cell eccentricity in agreement with the robustness of this alignment previously reported (Płochocka et al, 2021). A similar role for cell shape in organising microtubule polarity independently of Ft-Ds polarity has also been suggested in the Drosophila larval epidermis (Pietra et al, 2020).…”
In epithelial cells, planar polarisation of subapical microtubule networks is thought to be important for both breaking cellular symmetry and maintaining the resulting cellular polarity. Studies in the Drosophila pupal wing and other tissues have suggested two alternative mechanisms for specifying network polarity. On one hand mechanical strain and/or cell shape have been implicated as key determinants, on the other the Fat-Dachsous planar polarity pathway has been suggested to be the primary polarising cue. Using quantitative image analysis in the pupal wing, we reassess these models. We found that cell shape was a strong predictor of microtubule organisation in the developing wing epithelium. Conversely Fat-Dachsous polarity cues do not play any direct role in the organisation of the subapical microtubule network, despite being able to weakly recruit the microtubule minus-end capping protein Patronin to cell boundaries. We conclude that any effect of Fat-Dachsous on microtubule polarity is likely to be indirect, via their known ability to regulate cell shape.
“…Within the A compartment, about two rows of the most anterior cells (figure 5 c ) and about two rows of the most posterior cells (figure 5 d ) show D located posteriorly; thus, their Ds/Ft polarity is that normally characteristic of the P cells. The third instar larva, having fewer but larger polyploid cells told a similar story: a set of cells in the A compartment, those confined to the extreme posterior row, had variable polarity with some showing the same polarity as in the P compartment (D accumulating posteriorly, [40]). Figure 5Asymmetric localization of Dachs vis-à-vis A/P boundary.…”
The slope of a supracellular molecular gradient has long been thought to orient and coordinate planar cell polarity (PCP). Here we demonstrate and measure that gradient. Dachsous (Ds) is a conserved and elemental molecule of PCP; Ds forms intercellular bridges with another cadherin molecule, Fat (Ft), an interaction modulated by the Golgi protein Four-jointed (Fj). Using genetic mosaics and tagged Ds, we measure Ds
in vivo
in membranes of individual cells over a whole metamere of the
Drosophila
abdomen. We find as follows. (i) A supracellular gradient rises from head to tail in the anterior compartment (A) and then falls in the posterior compartment (P). (ii) There is more Ds in the front than the rear membranes of all cells in the A compartment, except that compartment's most anterior and most posterior cells. There is more Ds in the rear than in the front membranes of all cells of the P compartment. (iii) The loss of Fj removes intracellular asymmetry anteriorly in the segment and reduces it elsewhere. Additional experiments show that Fj makes PCP more robust. Using Dachs (D) as a molecular indicator of polarity, we confirm that opposing gradients of PCP meet slightly out of register with compartment boundaries.
“…Ft–Ds may also regulate microtubule orientation and core protein polarity in the anterior compartment of the abdomen. Here, microtubule plus-end growth is weakly biased towards the posterior ends of cells [54], although predominantly growth is along the mediolateral axis of the abdomen, orthogonal to the axis of asymmetry [129]. Consistent with this slight plus-end bias, Dsh particles show a posterior bias in their transport, as expected from the axis of the polarity of the core proteins [54].…”
Section: Indirect Effects Of Ft and Ds On Core Protein Localizationmentioning
confidence: 94%
“…The core proteins localize asymmetrically to anterior–posterior cell edges, but loss of core protein activity has relatively little effect on denticle orientation [107,134–136]. However, in the embryo and larva, denticle polarity correlates with asymmetric localization of Ds and D [129,137,138], and loss or overexpression of Ft–Ds severely disrupts denticle belt polarity [107,136–139]. Fj is highly expressed in the tendon cells which are posterior to rows 1 and 4 in the larval epidermis, which may explain the pattern of denticle polarity [140].…”
Section: Polarization Of Cuticular Structures By Ft–ds Independently ...mentioning
confidence: 99%
“…One way in which Ft and Ds might influence the polarization of cuticular structures could be by regulating cell shape and alignment. In wild-type embryos, cells are elongated on the dorsoventral axis and microtubules are aligned on this long axis [129,138]. In the absence of Ft, cells fail to elongate on the dorsoventral axis, and microtubules are disorganized [138].…”
Section: Polarization Of Cuticular Structures By Ft–ds Independently ...mentioning
Planar polarity describes the coordinated polarization of cells within the plane of a tissue. This is controlled by two main pathways in
Drosophila
: the Frizzled-dependent core planar polarity pathway and the Fat–Dachsous pathway. Components of both of these pathways become asymmetrically localized within cells in response to long-range upstream cues, and form intercellular complexes that link polarity between neighbouring cells. This review examines if and when the two pathways are coupled, focusing on the
Drosophila
wing, eye and abdomen. There is strong evidence that the pathways are molecularly coupled in tissues that express a specific isoform of the core protein Prickle, namely Spiny-legs. However, in other contexts, the linkages between the pathways are indirect. We discuss how the two pathways act together and independently to mediate a diverse range of effects on polarization of cell structures and behaviours.
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