Howard Hughes Medical Institute, Departments of Physiology and Biochemistry, 533 Parnassus Avenue, Room U226, Box 0725, University of California, San Francisco, San Francisco, CA 94143-0725, USA
*Author for correspondence (e-mail: ynjan{at}itsa.ucsf.edu)
Accepted 2 April 2002
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SUMMARY |
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Key words: Dendrite development, Peripheral nervous system, Tiling, Dendritic arborization neurons, Drosophila
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INTRODUCTION |
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Interactions with nearby neurons can provide cues to stop dendritic growth or to change the trajectory of growth (Perry and Linden, 1982; Scott and Luo, 2001
; Jan and Jan, 2001
). The phenomenon of tiling appears to offer a particularly dramatic example of such interactions. Tiling, which has been studied most extensively in alpha ganglion cells of the mammalian retina (Wässle et al., 1981
), refers to the complete but non-redundant innervation of a receptive area by dendrites of functionally uniform groups of neurons. Studies of the alpha ganglion cells identified two functionally distinct subpopulations, ON-center and OFF-center, with cell bodies arranged in independent mosaics across the retina (reviewed in Wässle and Boycott, 1991
). Dendrites from each subpopulation fill in the space between the cell bodies completely but in doing so overlap minimally with other like dendrites. Consequently, each physiological type of cell covers every region of visual space with high economy (Wässle et al., 1981
). With additional techniques for labeling different subsets of ganglion cells, it has become apparent that several other types [there are up to 15 (Masland, 2001
)] are also organized as tiled systems (Wässle and Boycott, 1991
). Thus, in the mammalian retina, tiling is a dominant theme in the organization of complex dendritic fields within 2D planes. Such an arrangement ensures complete and yet non-redundant representation of the sensory or presynaptic input for each physiological function being processed.
The rules of tiling suggest that subtype-specific cues can direct like dendrites to avoid each other and thereby establish non-overlapping territories. Consistent with this notion, depletion of a patch of retinal ganglion cells causes surrounding neurons to grow dendrites preferentially toward the voided area (Perry and Linden, 1982; Hitchcock, 1989
). Lesion experiments have also demonstrated that growth occurs in a cell-class-specific manner (Weber et al., 1998
), suggesting that a like-repels-like mechanism normally operates between dendrites. Such a scenario is further supported by the occurrence of cell-type-specific dendritic contacts between alpha cells, which could provide an opportunity for signaling via cell surface molecules or gap junctions (Lohmann and Wong, 2001
). Despite strong experimental evidence for selective dendritic recognition and exclusion in the retina, the molecular mechanisms controlling territory avoidance by like dendrites are not known.
The peripheral nervous system (PNS) of insects is well suited for examining the molecular basis of dendritic morphogenesis and tiling. The PNS comprises defined cell types with characteristic dendritic projections (Zawarzin, 1912), including the type I neurons with ciliated monopolar dendrites and the type II neurons with multiple dendritic (md) projections (Fig. 1A). The md neurons of Drosophila have been further classified into three subtypes according to their substrate and morphology (Fig. 1A) (Bodmer and Jan, 1987
); (1) the tracheal dendrite (md-td) neurons, (2) neurons with bipolar dendrites (md-bd) and (3) the dendritic arborization (md-da) neurons, which spread dendrites along the epidermis. Two lines of evidence suggest that dendritic tiling occurs among the md-da neurons. First, in Drosophila larvae, dendrites of the dorsal cluster neurons normally avoid projecting across the dorsal midline but will invade this territory if cells on the other side of the midline are ablated (Gao et al., 2000
). Second, anatomical and physiological studies of individual larval da neurons in the moth Manduca sexta have shown that dendrites from morphologically similar, but non-homologous, neurons within a hemisegment innervate non-overlapping territories (Grueber et al., 2001
). Together, these data indicate that the Drosphila PNS may be a fruitful system in which to explore the molecular basis of dendritic tiling.
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MATERIALS AND METHODS |
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MARCM labeling and immunocytochemistry
To identify and characterize the peripheral dendrites of each da neuron we used the MARCM system (Lee and Luo, 1999). For producing clones, females were provided with a freshly yeasted grape agar plate and allowed to lay eggs for 2 hours. Developing eggs were kept at 23-25°C and given a 37°C heat shock 3-5 hours after the end of the laying period. Two distinct heat shock regimes were used. For random labeling of small numbers of peripheral neurons for arbor reconstruction we subjected embryos to a single 1 hour heat shock. To examine the spatial relationships of arbors of neighboring neurons, we gave a 30 minute heat shock, followed by a 30 minute recovery period and a second 45 minute heat shock. The first method usually resulted in three to five labeled peripheral neurons per animal. The second method resulted in up to six labeled da neurons per hemisegment.
We identified GFP-labeled clones by examining living third instar larvae under a fluorescence microscope fitted with a 4x lens. Selected larvae were immersed in phosphate buffered saline (PBS; pH 7.4) and opened along the dorsal or ventral midline depending on the location of the labeled neuron. Filleted and pinned larvae were fixed with 3.7% formaldehyde for 1 hour at room temperature, rinsed several times in PBS with 0.3% Triton X-100 (PBS-TX) and blocked in 5% normal donkey serum (NDS; Jackson Laboratories, West Grove, PA). Primary antibodies were used at a concentration of 1:100 for rat anti-mCD8 (Caltag, Burlingame, CA) and 1:200 for mouse mAb 22C10 (Zipursky et al., 1984) and incubated overnight at 4°C. Secondary antibodies were Cy2 or Cy3-conjugated donkey anti-rat (diluted 1:200; Jackson Laboratories) and goat anti-mouse (diluted 1:500), respectively. After overnight incubation in secondary antibodies, the tissue was rinsed for several hours in PBS-TX, mounted on poly-L-lysine coated coverslips, dehydrated using an ethanol series (5 minutes each in 30%, 50%, 75%, 90%, 100% and 100%), cleared in xylenes (2x10 minutes) and mounted in DPX (Fluka, Milwaukee, WI). As an alternative to antibody staining, we imaged GFP fluorescence in living third instar larvae by cutting their posterior termini and mounting them in 90% glycerol.
Image processing and cell reconstruction
Our maps of the da system of the mature third instar larva are based on data from over 300 marked neurons in segments A2-A6. Representative clones were selected for detailed cell reconstructions on the basis of the quality and completeness of staining and the integrity of arbors following mounting. For cell reconstructions, 1 µm Z-series stacks were acquired on a Bio-Rad MRC-600 confocal microscope (Bio-Rad, Hercules, CA) using a 40x objective (1.3 n.a.), projected into a 2D image using COMOS software and assembled as montages in Photoshop 5.0 (Adobe Systems, San Jose, CA). Black and gray levels were typically adjusted to equalize the various images. Tracings of the neurons were made in Photoshop by adding a transparent layer and tracing the arbors using a mouse.
Quantitative analysis
We used the Strahler method (Strahler, 1953; Uylings et al., 1975
) to order and analyze the branching patterns of the da neurons. Terminal branches were assigned an order of one. Where two first-order branches met, an order of two was assigned. Where two second-order branches met, an order of three was assigned and so on for the whole cell. If a lower order branch (i.e. one) met a higher order branch (i.e. two), the higher branch order was carried on without change. Once dendrites were ordered in such a manner, the assignments were reversed (Berry et al., 1975
) so that extensions from the cell body became the lowest order branches and the terminals became the highest order branches.
To quantify the dendritic field sizes of each neuron, Z-series files were acquired on a Leica (TCS SP2) confocal microscope using a 20x (0.7 n.a.) objective, projected into a 2D image and imported into Image Pro Plus (MediaCybernetics). Dendritic fields were delineated by a polygon connecting the distal-most dendritic tips or arcs. We used these same images to plot the dendritic terminals of each neuron manually in Photoshop using a mouse. Four plots of each cell were used to construct each of the four composite hemisegments. We standardized dendritic territory positions and orientations within a hemisegment by using the segment border and the lateral oenocytes as positional markers.
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RESULTS |
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The da neurons together spread extensive overlapping dendrites across the epidermis (Fig. 1B). Viewed together, the pattern of dendrites covering each hemisegment appeared to be stereotyped from animal to animal, suggesting that each cell probably had a defined morphology and dendritic territory. To examine the dendritic morphologies of individual neurons in more detail, we produced wild-type mCD8::GFP-labeled clones using the MARCM system (Lee and Luo, 1999). The dendrites of da neurons were robustly labeled by inducing MARCM clones during embryogenesis and imaging these clones in third instar larvae (n=303 clones; Fig. 1C). Each individual da neuron had a characteristic branching pattern and territory across the epidermis. We identified four classes of branching patterns and found that each cell had dendrites that were entirely and consistently of one or another of these types. We term these class I, II, III and IV neurons (and dendrites), in order of increasing arbor complexity (Fig. 1D; Table 1). We examine each class in more detail below.
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To begin to investigate the factors that control da neuron territory formation in Drosophila, we characterized patterns of overlap and non-overlap between pairs of identified neurons and related these results to the morphological classes of the neurons (according to the above classification scheme). By using a repeated heat shock MARCM protocol (see Materials and Methods), we induced simultaneous labeling of several neurons in each hemisegment. These clones revealed that, depending on their spatial proximity, neighboring neurons of different morphologies could show either extensive overlap or complete overlap of their dendritic fields (Fig. 6A,B). We found no evidence for stratification of morphologically different dendrites (the distance between dendrites in the Z-direction was typically less than 1 µm); thus overlapping dendrites essentially branched in a 2D space. Furthermore, primary branches of adjacent neurons often followed the same initial paths (Fig. 6B,B'). These regions of dendritic association typically concluded with one of the dendrites turning abruptly and the other continuing along its prior trajectory (Fig. 6B,B'), suggesting that one of the neurons received a stop signal to which the other did not respond.
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Lack of dendritic overlap among cells of the same morphological class
Whereas neurons in different classes often cluster together and project dendrites to overlapping regions of the epidermis, cells in the same class were more evenly spaced across the body wall and projected dendrites to distinct domains (Fig. 2A, Fig. 3A, Fig. 4A, Fig. 5A). To examine whether like dendrites partially overlapped or, on the contrary, were excluded from each others territories, we examined patterns of dendritic overlap between neurons of the same morphological type. Maps of the territories of class I and class II neurons (Fig. 2A, Fig. 3A) and a single dual label of adjacent ventral class II neurons (Fig. 7A,A') show that, within each class, dendrites are non-overlapping. However, these dendrites typically extended to regions of the body wall that were non-contiguous, and thus terminal dendrites of different cells were not usually found in close proximity.
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We identified a total of 21 cases in which two or three adjacent class IV neurons (vdaB, vada, or ddaC) were labeled. The arbors of vdaB and vada met approximately midway between their cell bodies (Fig. 7D,D'), whereas the dendrites of vada and ddaC met at the lateral margin near the oenocytes (Fig. 7E,E'). Dendrites of these adjacent pairs typically crossed once along their borders (Figs 7, 8), but along the rest of the border dendritic exclusion was the rule (Fig. 7D,E). These boundaries did not obviously correlate with physical boundaries such as muscle insertion sites. The dendritic exclusion between these neurons also occurred at segment boundaries (between both homologous and non-homologous pairs of neurons; Fig. 7E,E') and at the dorsal and ventral midlines (data not shown).
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MARCM analysis of the roles of starry night and sequoia in tiling
Studies of the starry night (stan) gene suggest that it is required for dendritic exclusion between homologous neurons at the dorsal midline and may act in a cell-autonomous fashion (Gao et al., 2000). We examined whether stan is required for widespread tiling of the body wall by using the MARCM system to produce mCD8::GFP-labeled da neurons carrying the stanE59 allele (Fig. 9A). In each single-cell clone examined (n=23), most dendrites formed defined boundaries where they would normally encounter the dendrites of adjacent neurons (Fig. 9B,C). In two out of 11 class IV neurons, we observed one or two unbranched dendrites that showed an abnormally long projection (Fig. 9D,E). In one case observed in the dorsal cluster, the branch did not invade the territory of the contralateral hemisegment but, rather, projected aberrantly along the dorsal midline to the anterior adjacent segment. In the other case, the ventral cluster class IV neuron showed sinuous unbranched dorsal and ventral overextensions that terminated as tufts of dendrites beyond the cells territory proper (Fig. 9D,E). The remaining branches of these neurons appeared to terminate at their normal locations on the body wall (Fig. 9D,E).
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DISCUSSION |
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Our morphological characterization of Drosophila da neurons indicates that they are similar to the da neurons of the moth Manduca sexta, of which there are at least three distinct morphological classes (Grueber et al., 2001). In Manduca, the alpha, beta and gamma da neurons show morphological similarities to the class I/II, IV and III da neurons of Drosophila, respectively. Manduca alpha neurons appear to function as proprioceptors, whereas gamma neurons probably function as touch receptors (Grueber et al., 2001
). Whether the Drosophila da neurons are functionally similar to Manduca da neurons remains to be determined. At least two lines of evidence, however, suggest that the morphological classes that we have identified in Drosophila represent functionally distinct types of neurons. First, pickpocket (ppk), a degenerin/epithelial sodium channel subunit (Adams et al., 1998
; Darboux et al., 1998
), appears to be expressed only in the class IV neurons ddaC, vada and vdaB (W. G., B. Ye, L. Y. J., Y. N. J., unpublished). As ppk may have a physiological role in mechanotransduction (Adams et al., 1998
), its expression in class IV neurons could underlie a functional specialization of these cells. Second, Drosophila da neurons have dichotomous axonal projections, which probably reflect their functional distinctions (Merritt and Whitington, 1995
; Schrader and Merritt, 2000
). Most da neurons project into the ventral neuropil (Schrader and Merritt, 2000
), a characteristic of tactile projections (Murphey et al., 1989
). vpda and an unidentified neuron in the dorsal cluster, by contrast, have more dorsal projections (Merritt and Whitington, 1995
; Schrader and Merritt, 2000
), which is similar to proprioceptive neurons (Pflüger et al., 1988
; Murphey et al., 1989
). The ventral-projecting neurons appear to correspond to the class II, III and IV neurons, whereas the dorsal projections belong to at least a subset of the class I neurons.
Genetic specification of the da neurons
An important issue arising from our characterization of the Drosophila da system is how the morphological properties of each neuron relate to their genetic specification. Previous studies have shown that the Drosophila da system consists of genetically distinct subgroups of neurons (Dambly-Chaudiere and Ghysen, 1987; Blochlinger et al., 1990
; Jarman et al., 1993
; Merritt and Whitington, 1995
; Brewster and Bodmer, 1995
). Most da neurons require proneural genes in the achaete-scute complex (ASC) (Dambly-Chaudiere and Ghysen, 1987
) arise as components of external bristle lineages (Brewster and Bodmer, 1995
; Orgogozo et al., 2001
), and express the Cut protein (Blochlinger et al., 1990
). The only da neurons that do not share these characteristics are vpda and two dorsal neurons. vpda remains in ASC-mutant embryos but is lost in animals mutant for the proneural gene, atonal (Jarman et al., 1993
). One dorsal da neuron requires a third proneural gene, amos (Huang et al., 2000
; Brewster et al., 2001
). Finally, vpda and two dorsal da neurons fail to express Cut (Blochlinger et al., 1990
).
Reconciling these accumulated data with our cell-by-cell characterization of the da system, it appears that the class II, III and IV neurons are those that require ASC genes and express Cut. Class I neurons, on the other hand, do not express detectable levels of Cut (W. B. G., L. Y. J., Y. N. J., unpublished) and could correspond to the da neurons that require atonal and/or amos (although only one ASC-independent neuron has been described in the dorsal cluster). Consistent with these assignments, during our mosaic analysis we often observed class III and class IV neurons co-labeled with es neurons (see Fig. 4E and 5B, respectively), suggesting that these cells could have arisen from a common precursor. The class II neurons are likely also es related because all four neurons in the ventral cluster are lineally related to es organs (Orgogozo et al., 2001) and two class II neurons reside here (Fig. 3). Understanding how the genes required for early da specification are linked to the activation of distinct programs of dendritic morphogenesis is an important goal for future studies.
Morphologically alike da neurons tile the epidermis
Tiling is a principle of dendrite organization in which functionally similar neurons completely fill available receptive territories with little or no redundancy. We have identified two independent tilings of the Drosophila epidermis by da neurons bearing similar morphologies (Fig. 7). A similar type of tiling has recently been identified in Manduca (Grueber et al., 2001), suggesting that this is an evolutionarily conserved plan for organizing the da sensory system. In Drosophila, tiling occurs between class III da neurons and between class IV da neurons, which each partitions the body wall into a collection of non-overlapping territories (Fig. 7). Furthermore, class III and IV neurons each provide a nearly complete segmental coverage (Table 2). Dendrites with distinct morphologies, by contrast, can cross extensively (Figs 6, 8).
The tiling of the Drosophila epidermis by class III and IV neurons appears analogous to the tiling among physiologically alike vertebrate retinal ganglion cells. In this system, ON-center and OFF-center, four ON-OFF direction-selective classes and several other cell types, including amacrine cells, provide independent tilings of the retina (Wässle et al., 1981; Wässle and Boycott, 1991
; Amthor and Oyster, 1995
; MacNeil and Masland, 1998
). Such an arrangement ensures that each region of the visual field is viewed by each physiological type of ganglion cell. Additionally, as visual information is distributed to the appropriate centers of the brain, the location of its origin is unambiguous, thereby maintaining a coherent representation of sensory space. The same rules of organization applied to the insect da system would likewise be advantageous. Mechanical and thermal stimuli often necessitate rapid and finely directed behavioral responses, particularly when they could lead to damage to the cuticle (Frings, 1945
; Walters et al., 2001
). If future studies show that the da neurons comprising each tiling class are united by their physiology, as we suspect, then these modalities would have the capacity to provide accurate spatial resolution of stimuli landing anywhere on the body wall.
What mechanisms and molecules control dendritic tiling?
Although the cellular mechanisms that control dendritic tiling are not yet understood, several developmental scenarios can be envisioned. Individual dendrites could repel like dendrites where they meet. Alternatively, neurons could be endowed with a limited capacity for dendritic growth (depending, for example, on cell size) and form their territories without influence from neighboring neurons. Finally, in the case of the da neurons, interactions with the epidermis or surrounding tissue, such as muscle, could provide permissive or restrictive growth signals. These mechanisms are not mutually exclusive and could conceivably act in concert. In the da system, however, dendritic boundaries could not always be correlated with physical boundaries, such as muscle insertion sites, and terminal dendrites typically turned abruptly where they met like dendrites. Thus, our data do not provide strong support for the latter two mechanisms (limited growth capacity and physical boundaries) but do suggest that branch interactions could contribute to tiling. Experimental studies of the effects of adding neurons to, and removing neurons from, the da system will provide essential tests of the importance of these mechanisms. Additionally, because our data are taken from mature da neurons, a crucial question still to be addressed is how dendrites of like neurons behave during development as their territories are established. Dendrites could show exclusion throughout their development or, alternatively, refine their boundaries as a maturational step.
Regulation of tiling by dendritic branch interactions is a likely scenario in the vertebrate retina, where contact-mediated avoidance signals appear to operate in a cell-type-specific manner (Wässle et al., 1981; Amthor and Oyster, 1995
; Hitchcock, 1989
). Furthermore, morphological data from mammalian retinal neurons show that dendro-dendritic contacts are made between like neurons but not between unlike neurons (Lohmann and Wong, 2001
). Such contacts could provide an opportunity for these neurons to signal to each other by their activity or cell surface composition (Lohmann and Wong, 2001
). Similarly, we typically observed single apparent dendritic contacts between tiling class IV neurons. Whether these contacts are important for exclusion among the remaining branches remains to be determined.
The molecular mechanisms of dendritic tiling in the vertebrate retina have not been established. Mutant screens of the second chromosome in Drosophila (Gao et al., 1999) (D. Cox, W. G., G. Tavosanis, L.Y. J., Y. N. J., unpublished) might be informative in this regard, as several candidate loci have been identified that cause early overextension of dendrites. We have tested alleles of two of these genes, stan (Gao et al., 2000
) and seq (Brenman et al., 2001
), for possible roles in tiling. In seq22 and stan72 mutant embryos, dendrites show an overextension phenotype and exhibit abnormal crossing of the dorsal midline (Gao et al., 2000
; Brenman et al., 2001
). Our MARCM analysis using the seq22 and stanE59 alleles suggests that such overextension might not reflect a widespread defect in dendritic exclusion, because a majority of the dendrites terminate or turn where contact with an adjacent like neuron occurs or would be expected (compare Fig. 5A with Fig. 9B-E). Importantly, however, one or two sparsely branched processes were seen extending beyond the normal boundary of the cell in 18% of the class IV stan-mutant neurons (Fig. 9D,E).
If branch recognition and exclusion are required for tiling, which appears to be the case for the class IV neurons (this study), one interpretation of the stan phenotype is that the dendrite is overextending because it does not receive or transduce a repulsive signal that requires Stan function. Alternatively, because in wild-type neurons exclusion occurs among terminal dendritic branches (Fig. 7), a lack of exclusion in stan-mutant neurons could arise if the overextended processes are equivalent to primary trunks and thus lack the machinery for tiling. However, without information about the fields of surrounding like neurons, we cannot eliminate the possibility that exclusion is intact in stan-mutant neurons. By extending earlier, or more rapidly, than the rest of the dendritic field (Gao et al., 2000), these single processes could have successfully invaded an uninnervated region of the body wall. This latter scenario seems to provide a reasonable explanation for why we observed a dorsal branch from ddaC overextending along the dorsal midline (one of the last regions of the body wall to become innervated; Fig. 9D). Whether a similar invasion scenario could account for the overextended processes from vdaB (Fig. 9E) might ultimately depend on the timing and pattern of outgrowth of its class IV neighbors (i.e. how far can a dendrite of a stan vdaB neuron extend before encountering like dendrites?). Because our MARCM experiments suggest that stan acts cell autonomously in the dendritic arborization neurons, future studies might be conducted using cell-type specific markers of the class IV neurons in a stan (and seq) mutant background. Such markers would allow the visualization of all neurons together and, as a result, provide a better indication of the relationship between early dendritic overextension phenotypes and tiling.
Could similar mechanisms regulate isoneuronal and heteroneuronal dendritic exclusion?
In addition to the dendritic exclusion that occurs between like neurons, we frequently observed exclusion between dendrites that belong to the same neuron (Figs 2-5). Such self-avoidance has been identified in Manduca sensory neurons (Grueber and Truman, 1999
; Grueber et al., 2001
) and characterized experimentally in leech sensory axons (Yau, 1976
; Kramer and Kuwada, 1983
; Kramer and Stent, 1985
; Gan and Macagno, 1995
; Wang and Macagno, 1998
; Baker et al., 2000
); however the underlying mechanisms are not understood. In theory, self-avoidance and tiling might not require distinct signals or signaling pathways (among like neurons) because isoneuronal dendrites could be developmentally identical to like heteroneuronal dendrites. It will therefore be of special interest to compare the mechanisms of exclusion by isoneuronal and heteroneuronal branches during development. Ultimately, an understanding of the distinction between these two processes will require the elucidation of their molecular underpinnings.
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ACKNOWLEDGMENTS |
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