Terni B , Llobet A .

             homeostatic process
             axon terminus
             synaptic signaling

	Figure 1. The endolysosomal system is present in axon terminals of olfactory sensory neurons (OSNs) of Xenopus tropicalis tadpoles.(A) Image of the olfactory bulb of a X. tropicalis tadpole stained with LAMP-1, an endolysosomal marker. LAMP-1 was present in axons (arrows) of OSNs entering the olfactory bulb, as well as in olfactory glomeruli, which were revealed by the accumulation of the synaptic vesicle protein synaptophysin (dotted circles). Axon terminals of OSNs form the presynaptic element of olfactory glomeruli. DAPI was used to reveal the position of cell nuclei. The image shows three regions of the olfactory bulb: nerve layer, glomerular layer, and the rostral portion of the mitral cell layer. Part of the olfactory nerve is also visible. (B). Transmission electron microscopy images allowed the observation of olfactory glomeruli (dotted circle). Axon terminals appeared as electrodense processes contacting dendrites (d). (C) The presynaptic compartment of OSNs is long, tortuous, and contains a large pool of cytoplasmic vesicles that acts as a reservoir of active zones (green arrow). Mitochondria (m) and late endosomes (yellow arrow) are present in the cytosol. (D) Detail of the boxed region in (B) indicating the presence of a lysosome (arrow). (E) Some autophagophores were also present in OSN presynaptic terminals. (F) Visualization of the entire morphology of OSNs in a zHB9::GFP X. tropicalis tadpole anesthetized and embedded in agarose. It is possible to observe the entire morphology of a population of GFP positive OSNs that project to a single glomerulus. Cell bodies are located in the olfactory epithelium (O.E). Axons travel along the olfactory nerve and give rise to two symmetrical olfactory glomeruli (O.G.) in the olfactory bulbs.
	Figure 2. Tracking the mobility of endolysosomes in olfactory sensory neurons in vivo.(A) Puncta stained with lysotracker deep red (L.D.R, red) co-localized with the product of the hydrolysis of magic red cathepsin-B (M.R., blue). The arrows indicate the line profiles of two acidic organelles located in the periphery of the GFP labelled glomerulus (arrow, magenta) and in an axonal region (arrow, brown). (B) Schematic morphology of a Xenopus tropicalis tadpole olfactory sensory neuron. The anatomical regions are indicated. Cilia (c), cell body (c.b.), axonal region (a) which comprises the olfactory nerve (ON) tract and the nerve layer (NL) of the olfactory bulb, and axon terminals forming glomeruli (a.t.). (C) Maximum intensity projection (left) and single confocal section (right) of the olfactory bulb. The mobility of acidic organelles (red staining) was evaluated separately in axon terminals originating the GFP-positive glomerulus (dotted circle) and in the NL of the olfactory bulb. The SMSS and the diffusion coefficient were calculated for puncta that fulfilled the analysis criteria (see the Materials and Methods section for details). Mobility tracks are indicated for three glomerular acidic organelles (red, green, and blue traces) and one acidic organelle of the NL (magenta). (D) Maximum intensity projection (left) and single confocal section (right) of a region of an ON. Acidic organelles found in the ON moved by confined diffusion (orange trace) and directed motion (green trace). Notice the presence of a population of GFP labelled axons, a characteristic of the zHB9::GFP X. tropicalis line.
	Figure 3. Mobility of endolysosomes found in presynaptic and axonal compartments.(A, B, C) Plot of the slope of the moment scaling spectrum (SMSS) against the diffusion coefficient (D.C.) of acidic organelles located in three different layers of the olfactory system. SMSS values found between 0.4 and 0.6 are associated to free diffusion (F.D., dotted lines), whereas SMSS values <0.4 or >0.6 are indicative of confined diffusion (C.D.) or directed motion (D.M.), respectively. Almost all acidic organelles present in presynaptic terminals move by confined diffusion. Free diffusion and directed motion are present in axonal regions. (D) Mean SMSS and diffusion coefficient values for acidic organelles found in the glomerular layer (n = 82), nerve layer (n = 40) and the olfactory nerve (n = 118, seven tadpoles). Error bars indicate SEM.
	Figure 4. Microinjection of secreted protein acidic and rich in cysteine (SPARC) in the olfactory bulb disrupts olfactory-guided behaviour.(A) Xenopus tropicalis tadpoles are attracted by local delivery of a 1 mM mixture of five different amino acids (methionine, leucine, histidine, arginine, and lysine), which act as waterborne odorants. Changes in the Euclidean distance found between the animal and the nozzle (arrow) delivering the odorants set the bases for quantifying olfactory-guided behaviour. For analysis, all tadpoles are considered to be 0 mm away from the odour source just before exposure to odorants. Negative distance values show attraction, whereas positive values indicate repulsion. (B) Average response of control tadpoles to local delivery of the amino acid solution (n = 72). Solid line and shadowed area indicate mean Euclidean distance and SEM, respectively. (C) Quantification of the time spent in the vicinity of the odour source (see the Materials and Methods section for details). The attraction for waterborne odorants is transient and occurs from 15 to 30 s after amino acids start to flow into the well (*P < 0.05, Kruskal–Wallis t test followed by Dunn’s multiple comparisons test). Dots indicate mean ± SEM (n = 72). (D) Average olfactory-guided response of tadpoles 5 h after injection of 50 μM full-length recombinant SPARC in the olfactory bulb (n = 78). Solid line and shadowed area indicate mean ± SEM changes in the Euclidean distance separating the animal and the nozzle delivering the amino acids. (E) Tadpoles injected with full-length SPARC are not attracted by waterborne odorants. Dots indicate mean ± SEM (n = 78). (F) Average olfactory guided response of tadpoles 5 h after injection of 500 μM peptide p4.2 (n = 51) or 500 μM peptide p2.1 (n = 54) in the olfactory bulb. Both peptides contain 20 amino acids found in the illustrated regions of SPARC. Peptide 4.2 displays an analogous activity to the full-length protein. Peptide 2.1 is inactive and is used as a control of injection. Solid line and shadowed area show mean ± SEM changes in Euclidean distance. (G) Labelling of olfactory sensory neurons with lysotracker deep red did not alter olfactory-guided behaviour (n = 58). Solid line and shadowed area indicate mean ± SEM changes in Euclidean distance. The grey trace indicates the control response (from B) for comparison purposes.
	Figure 5. Presence of multiple organelles of the endolysosomal system in axon terminals of olfactory sensory neurons during synaptic remodelling.(A, B, C, D, E, F, G) Presynaptic terminals forming olfactory glomeruli were inspected for the presence of components of the endolysosomal system upon exposure to full-length secreted protein acidic and rich in cysteine (SPARC) or its active peptidic fragment p4.2. Lysosome (A, arrow), late endosomes (B, C, arrows), endolysosomes (D, E, arrows), and autophagic intermediates (F, G, arrows). (H) Retraction bulb (arrow) suggesting an ongoing elimination of synaptic contacts.
	Figure 6. Secreted protein acidic and rich in cysteine (SPARC) alters the structure of F-actin patches present in olfactory glomeruli.(A) F-actin patches (arrows) were present in olfactory glomeruli (up). Plot of Intensity profiles (dotted yellow line) used to estimate the width and maximum fluorescence of the structures identified (down). (B) SPARC disrupted the appearance of F-actin patches by increasing their area and reducing their fluorescence peak. (C, D) Average intensity profiles from F-actin patches obtained in control condition (C, n = 92) or in tadpoles injected with 50 μM SPARC (D, n = 137). Solid lines and error bars indicate mean ± SEM obtained from the individual traces shown. (E) Normalized average intensity profiles showing an increase in the width of F-actin patches in tadpoles injected with SPARC (red) compared with control animals (black). (F) Comparison of the area covered by F-actin patches in the olfactory glomeruli of control (black, n = 104) and SPARC injected tadpoles (red, n = 95). Box plots show the median (horizontal line), 25–75% quartiles (boxes), and ranges (whiskers) of the area of F-actin patches. The difference between the two groups was established by the t test.
	Figure 7. The diffusion coefficient of endolysosomes found in axon terminals is increased during synaptic remodelling.(A) Acute effect of 50 μM latrunculin-A on the mobility of acidic organelles present in presynaptic terminals. Plot of the slope of the moment scaling spectrum (SMSS) against the diffusion coefficient (DC) of particles labelled with lysotracker deep red. SMSS values found between 0.4 and 0.6 are associated to free diffusion (F.D., dotted lines), whereas SMSS values <0.4 and >0.6 are indicative of confined diffusion (C.D.) and directed motion (D.M.), respectively. (B) Relationship between the SMSS and the DC of acidic organelles found in axon terminals of olfactory sensory neurons in five different experimental conditions. Dots indicate mean ± SEM obtained in the indicated groups. Control (n = 75, 8 tadpoles), p2.1 (n = 67, 8 tadpoles), p4.2 (n = 143, 6 tadpoles), full-length secreted protein acidic and rich in cysteine (SPARC, n = 72, 10 tadpoles), and latrunculin-A (n = 209, 14 tadpoles). Each dot indicates mean ± SEM. Colored bars indicate the ranges of SMSS values associated to confined diffusion (C.D.) and free diffusion (F.D.). (C) Box plots show the median (horizontal line), 25–75% quartiles (boxes), and ranges (whiskers) of DCs found for presynaptic acidic organelles in the five experimental groups showed in [B]. Statistical differences were established using the Kruskal–Wallis test followed by Dunn’s multiple comparisons test. (D) Box plots show the median (horizontal line), 25–75% quartiles (boxes), and ranges (whiskers) of the average velocity of presynaptic acidic organelles found in the five experimental groups showed in [B]. Statistical differences were established using Kruskal–Wallis test followed by Dunn’s multiple comparisons test. The percentage of particles reaching velocities >1 μm·s−1 in each experimental group is indicated in the upper plot.
	Figure 8. The increase in the mobility of presynaptic endolysosomes is associated to changes in the viscosity of the cytosol.(A) The radius of presynaptic endolysosomes increased when full-length secreted protein acidic and rich in cysteine (SPARC) triggered the remodelling of synaptic connectivity. Control (n = 60, eight tadpoles) and SPARC-injected tadpoles (n = 72, ten tadpoles) (B, C). The diffusion coefficient decreased as a function of the radius of puncta labelled with lysotracker deep red. Fitting of individual values to the Stokes–Einstein equation revealed that the viscosity (η) of 0.15 Pa·s found in axon terminals decreased to 0.066 Pa·s after the glomerular layer was exposed to SPARC. Bins indicate mean ± SEM. and dots show individual values. (D) Normalized Gaussian fits show that latrunculin-A and SPARC increased the size of acidic organelles compared to control conditions. (E) Latrunculin-A reduced the viscosity of the presynaptic cytosol to 0.085 Pa·s. Bins indicate mean ± SEM and dots show individual values. (F) Microinjection of the inactive SPARC derived peptide, p2.1, did not alter the viscosity of the presynaptic compartment (η = 0.14 Pa·s). Fits obtained in (B, C, E) are included for comparison purposes. (G) Average olfactory guided response (n = 56) of tadpoles injected with 50 μM latrunculin-A to local delivery of a 1 mM mixture of 5 different amino acids (methionine, leucine, histidine, arginine, and lysine). Solid line and shadowed area indicate mean Euclidean distance and SEM, respectively. The control response of non-injected animals is displayed for comparison purposes. Arrows show the time of initiation of the movement towards the odour source. Notice the delay present in tadpoles injected with latrunculin-A (time between arrows).
	Figure 9. Axonal transport of endolysosomes is not affected by synaptic remodelling.(A) Histogram of net displacements of all acidic organelles found in the olfactory nerve (ON) of a control tadpole occurring in a time interval of 200 s (n = 152). Negative values indicate retrograde transport and positive values indicate anterograde transport. A Gaussian fit was used to obtain the mean value of particle displacements, which in this example was of −0.105 μm. This distance was considered a quantitative indicator of the balance between retrograde and anterograde transport of endolysosomes in the ON and was representative of a given tadpole. (B) No differences (one-way ANOVA analysis followed by Dunnett’s multiple comparisons test) were found among the mean, net representative displacements of acidic organelles present in the ONs in the indicated experimental conditions. Control (n = 7 tadpoles), p2.1 (n = 7 tadpoles), p4.2 (n = 7 tadpoles), full-length secreted protein acidic and rich in cysteine (SPARC, n = 9 tadpoles). (C) No differences (one-way ANOVA analysis followed by Dunnett’s multiple comparisons test) were found in the average velocity nor the maximum velocity of endolysosomes present in the ONs in the indicated experimental conditions. Control (n = 7 tadpoles), p2.1 (n = 7 tadpoles), p4.2 (n = 7 tadpoles), and SPARC (n = 9 tadpoles).

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