Habitat influences skeletal morphology and density in the snailfishes (family Liparidae)

We tested the hypothesis that deep-sea fishes have poorly mineralized bone relative to shallower-dwelling species using data from a single family that spans a large depth range. The family Liparidae (snailfishes, Cottiformes) has representatives across the entire habitable depth range for bony fishes (0 m–> 8000 m), making them an ideal model for studying depth-related trends in a confined phylogeny. We used micro-computed tomography (micro-CT) scanning to test three aspects of skeletal reduction in snailfishes (50 species) across a full range of habitat depths: 1) reduction of structural dimensions, 2) loss of skeletal elements, and 3) reduction in bone density. Using depth data from the literature, we found that with increasing depth, the length of the dentary, neurocranium, and suborbital bones decreases. The ventral suction disk decreases width with increasing maximum habitat depth and is lost entirely in some deeper-living taxa, though not all. Although visual declines in bone density in deeper-living taxa were evident across full skeletons, individual densities of the lower jaw, vertebra, suction disk, hypural plate, and otoliths did not significantly decline with any depth metric. However, pelagic and polar taxa tended to show lower density bones compared to other species in the family. We propose that skeletal reductions allow snailfishes to maintain neutral buoyancy at great depths in the water column, while supporting efficient feeding and locomotion strategies. These findings suggest that changes in skeletal structure are non-linear and are driven not only by hydrostatic pressure, but by other environmental factors and by evolutionary ancestry, calling the existing paradigm into question. Supplementary Information The online version contains supplementary material available at 10.1186/s12983-021-00399-9.


Background
The majority of the habitable biosphere on Earth is in the deep sea, characterized by high hydrostatic pressures, cold temperatures, and the absence of sunlight (reviewed by [92]). Deep-sea habitats vary-from cold-water corals to abyssal plains, hydrothermal vents to deep-sea trenches, mesopelagic open waters to submarine canyons-and each are accompanied by distinct conditions and associated fauna. Specific environmental conditions such as temperature, hydrostatic pressure, and nutrient availability have given rise to a wide array of adaptations in deep-sea organisms. As a result, deep-sea fishes are incredibly diverse (e.g. [45,90]), with specialized traits to survive, feed, reproduce, and hide in deep-sea habitats (e.g. [21,51,90,93]).
Hydrostatic pressures in the deep sea reach more than one-thousand times atmospheric pressure, up to 100 MPa, posing an evolutionary challenge for fishes to radiate into the deep oceans. Fishes have evolved mechanisms to cope with these high hydrostatic pressures on multiple scales, from the molecular to the organismal (e.g. [101,110]). Many deep-sea organisms, including fishes, use pressure adaptations such as increased levels of polyunsaturated fatty acids that maintain fluidity of cellular membranes under high pressures and low temperatures [3,15,98], specialized enzymes and proteins [39,42,97,102], and protein-stabilizing molecules called piezolytes that prevent water from being pushed into the active sites of enzymes and proteins (reviewed by [113]). One notable example is the protein-stabilizing osmolyte trimethylamine-N-oxide (TMAO) that accumulates in fish cells with increasing habitat depth. In hadal trenches, at around 8200 m, cells become isosmotic with seawater due to these high TMAO concentrations, resulting in a likely physiological constraint on maximum depth for fishes [111].
High hydrostatic pressures pose an additional challenge for fishes-to maintain neutral buoyancy. The bony skeleton of fishes provides support, protection, and attachment surfaces for muscles. However, a skeleton is dense and reduces buoyancy. Gas bladders for buoyancy become increasingly difficult to inflate with increasing habitat depth [89,96]. Some deep-sea species use a subdermal gelatinous tissue to maintain neutral buoyancy without a gas-filled bladder [28,40,112], while others have lipid-filled swim bladders (e.g. [43,71]) and even lipid-rich bones [59] to add positive buoyancy. Deep-sea anglerfishes, gulper eels and several other lineages have poorly mineralized bone, which is assumed to be an adaptation to maintain neutral buoyancy by reducing the weight of the body's densest tissues [12,14,19,45,57,93]. Decreased mineralization of the skeleton can be achieved by reducing the size and thickness of bones, or by reducing the amount of mineral (such as calcium, phosphate, or sulfate) in the bone [93].
The diversity of deep-dwelling fishes (e.g. [90]), makes it difficult to distinguish specific deep-sea adaptations from variations across phylogeny or from other factors. This study examines skeletal properties across a depth range from a single family, the snailfishes (Liparidae). Liparids are generally small (< 20 cm), tadpole-shaped fishes that lack scales. Most liparids have a ventral sucking disk, used to stick to rocks and other substrates in shallow environments (e.g. [7]). In some deep-water species, the disk may be used in carcinophyly, a parasitic reproductive strategy where the fish attaches to the carapace of a king crab [114] and deposits its eggs inside the carapace on the gills [35,106]. The Liparidae are a morphologically distinct and monophyletic family [69,82,99] with over 430 described species [32]. Snailfishes live in cold polar to temperate waters and have the largest bathymetric range of any fish family-from the intertidal to over 8000 m [10,34,61,72]. As such, the liparids represent an appropriate system to investigate adaptation into the deep sea within a constrained phylogeny. Deep-sea liparids have been described as having "less firm" bodies and weakened skeletons in comparison to their intertidal counterparts, so there is anecdotal evidence of skeletal variation [7]. Phylogenetic evidence suggests that liparids evolved from a shallow-living ancestor, following which, the majority of the family diversified from a deep-water clade with both demersal and pelagic lifestyles [82]. A trend of evolutionary reduction in certain morphological features (pelvic fins, pseudobranchial filaments, skin spinules, brain mass, visual system) in liparid species more specialized for deep-sea habitats has also been noted [55,58,64].
Here, we investigate changes in skeletal density and form with habitat across the family Liparidae through micro-computed tomography (micro-CT), covering the complete bathymetric range of bony fishes. We predict that bones with fewer functional demands at depth will be reduced, while other crucial bones will remain relatively large and dense, even at great depths. We test three hypotheses related to skeletal declines: 1) dimensions of specific bones become reduced with increasing habitat depth; 2) skeletal elements that are not adaptive in a deep-sea habitats are lost in deep-sea taxa; and 3) density of individual bone structures declines with increasing depth. We then qualitatively examine other habitat-related trends in skeletal density such as between pelagic and demersal taxa and polar and subpolar species.
To test the first hypothesis-that bone dimensions would be reduced with increasing depth-we measured three areas of the skeleton: the jaw, pectoral girdle, and neurocranium (specific bones are shown in Fig. 1). We expected the neurocranium would be most reduced, because selective pressure for protection of the brain may be diminished due to decreased predation risk at increased depths [46]. We predicted the bones of the pectoral girdle and jaws would remain at least as large in deep-water fishes as in nearshore relatives due to their key role in suctionfeeding and swimming. Snailfishes from both intertidal waters and hadal trenches have been observed using pectoral fin motion to navigate and obtain resources (e.g. [40,53,107]). Snailfishes are primarily suction feeders (e.g. [2]), relying on the bones of the jaw to rapidly protrude and contribute to negative pressures in the mouth to capture prey [48,62,109]. Compared to other co-occurring fishes, some Antarctic liparids have a lower mechanical advantage and bite force but a higher suction index [2]. Both intertidal and deep-sea species rely on this suction feeding strategy to catch small crustaceans-their main prey [16,41,56,73].
Skeletons in deep-water fishes could also be reduced through the complete loss of bone structures. We hypothesize that certain skeletal elements are lost with increasing depth, due to changing evolutionary drivers. While snailfishes at any habitat depth would require certain bones, for example, pharyngeal jaws, other skeletal elements could be less important to life in the deep sea. For example, the ventral suction disk might be less important in deep-sea habitats, where hydrodynamic forces due to wave action are not a factor in evolutionary success.
A decline in bone density with increasing depth in deep-sea fishes is likely complicated by interactions with bone function. Bone mineralization is related to stiffness and strength, which in turn can limit performance. We quantified density in five bones with different biological functions and consequent performance requirements: the lower jaw, the pelvic suction disk, a vertebra, the hypural plate, and the sagittal otoliths (Fig. 2). Density of the lower jaw was measured as an indication of the energy the fish has devoted to mineralizing feeding structures. We expected no effect of depth on jaw density as liparids rely on a diet of small crustaceans across a broad range of habitat depths [41] and deep-living snailfishes should have similar requirements in feeding morphology to their shallow-living counterparts. We measured the first left pelvic disk pterygiophore as a proxy for suction disk performance with increasing depth. Here, we expected to see a reduction in density as deep-sea habitats are not subject to wave action and high current flow. The hypural plate captures the undulatory locomotor performance, with the hypothesis that fishes in deeper environments would have limited need for long burst swimming due to decreased interaction distances between predator and prey with declining light levels [11,24]. We measured the density of the third vertebra, which we predicted to reflect the overall density of the specimen and give insights into both locomotion and buoyancy. Reduced vertebral density with increasing habitat depth could also signal the need to maintain neutral buoyancy under high pressures. The sagittal otoliths, calcium carbonate structures in the inner ear that function in hearing, were included because their density reflects a sensory need that should not change with increasing depth and so might remain unchanged with depth. We then explore patterns of bone density with other habitat parameters, including latitude and lifestyle.

Results
We scanned 50 species of snailfishes (Family Liparidae) in 13 genera across the complete habitat depth range for bony fishes (0-8000 m). Specimens from different genera varied in scan brightness and morphology across taxa (Fig. 3). These CT scans were used to explore three potential skeletal declines across varying habitats: dimensional reductions, loss of skeletal elements, and reductions in bone density.

Bone dimension reduction
Length and width of skeletal elements of the jaw, neurocranium, pectoral girdle, and suction disk were measured for 35 species from 12 genera (Supplementary Table 1). Correlations of phylogenetic independent contrasts showed that there was a decrease in some bone lengths with increasing depth, while other bone lengths did not differ significantly along a depth gradient ( Table 1). The relative length of the dentary (dorsal fork and ventral fork lengths) significantly decreased with increasing minimum depth (Fig. 4a, dorsal fork length: α = 0.05, df = 35, p = 0.0432; ventral fork length: α = 0.1, df = 35, p = 0.0707). Dentary lengths did not significantly decrease with collection or maximum depth (Table 1). The maxilla (length and width), premaxilla (lateral length and ascending process length), and anguloarticular (length) were not significantly related to habitat depth by any metric (Table 1). Neurocranium length decreased with maximum depth (α = 0.05, df = 34, p = 0.0007; Fig. 4b) and collection depth (α = 0.1, df = 35, p = 0.0760). The length of the suborbital bone significantly decreased with increasing habitat depth by all metrics (Fig. 4c; α = 0.05, minimum depth: df = 22, p = 0.0010: maximum depth: df = 21, p = 0.0002; collection depth: df = 22, p = 0.0002), while suborbital width was not related to depth (Table 1). Pectoral girdle length did not significantly correlate with any depth metric after phylogenetic correction (Table 1). Maximum disk width decreased with increasing maximum depth (α = 0.1, df = 21, p = 0.0572), but did not relate to minimum or collection depth (Table 1). AIC values for PGLS models suggested that minimum depth often provided the best fit metric (maxilla length and width, premaxilla ascending process length, lengths of both the dorsal and ventral forks of the dentary, and anguloarticular length), though for other bones maximum depth (premaxilla length, neurocranium length, and maximum disk width) and collection depth (suborbital length and pectoral girdle length) resulted in the lowest AIC values (Table 1). Standard-length corrected phylogenetic residuals correlated with habitat depth across most bones and depth metrics (ANOVA, p < 0.05 for maxilla width, the ascending process of the premaxilla, premaxilla length, dorsal fork length of the dentary, neurocranium length, and suborbital length for all depth metrics, Supplementary Table 2).

Loss of skeletal elements
Each snailfish scan was analyzed for the presence of major skeletal features. Although declining density made elements such as pectoral fin rays, pectoral radials, and caudal vertebrae more difficult to see in the micro-CT scans, the only major skeletal element that was absent in some taxa was the pelvic suction disk. The disk was absent in 15 of the 45 species analyzed ( Table 2). The genera that lacked disks were Acantholiparis, Elassodiscus, Lipariscus, Nectoliparis, Paraliparis, and Rhinoliparis. The disk in Elassodiscus is reduced to small nonfunctional lobes, a condition we considered as absent here. Examples of variation in disk size, shape and development are shown in Fig. 5. All members of the polyphyletic genus Careproctus have suction disks, yet the distinct but tiny disk of Careproctus ostentum was not visible in the scanned specimen. Due to this discrepancy, this species was not included in our ancestral state reconstructions.
We examined the presence or absence of a ventral suction disk in relation to phylogeny and habitat depth. With the phytools package [94] in the statistical programming platform R [91], we found marginal ancestral state estimates and used the phylANOVA function to test for an effect of depth in predicting structure loss. Maximum habitat depth was a significant predictor of disk absence, while collection depth and minimum depth were not (phylANOVA, nsim = 1000, depths logtransformed; collection depth F = 8.364424, p = 0.146; maximum depth F = 14.735598, p = 0.038; minimum depth: F = 5.950088, p = 0.217). We then simulated ancestral states of disk presence or absence using stochastic character mapping in the simmap function [4] based on the tree of Orr et al. [82]. Our ancestral state reconstruction for the presence of the ventral suction disk across evolutionary time is shown in Fig. 6. These data indicate that the ventral suction disk was likely an ancestral feature of the snailfishes that has been lost at least three times over their evolution.

Changes in bone density
We examined bone density for five skeletal elements of 38 species from 13 snailfish genera by relating scan brightness to the brightness of known hydroxyapatite standards called phantoms (Fig. 7). Scan brightness, a proxy for bone density, was noticeably lower in deeperliving members within genera, as shown for the genus Liparis (Fig. 8). Losses of bone density with increasing habitat depth were visually evident across genera throughout the neurocranium and vertebral column (Fig. 7). Liparis fucensis, maximum depth 338 m, had the highest bone densities we measured, while Liparis fabricii, maximum depth 520 m, had the lowest (Supplementary Table 3).
In our quantitative analysis, no bones decreased density (% hydroxyapatite) with continuous depth according to phylogenetically-independent modeling at an alpha threshold of 0.05. Density of the vertebra and lower jaw correlated positively with minimum habitat depth (vertebra: df = 38, p = 0.0000; lower jaw: df = 38, p = 0.0001). Otolith density showed some corresponding decrease with increasing minimum depth at an α threshold of 0.1 (df = 11, p = 0.0689), though not for maximum or collection depth. Minimum depth yielded the lowest AIC values for the hypural plate and otolith, indicating the best fit model of the three depth metrics tested (Table 3). For the vertebra and lower jaw, the maximum depth model fit best, while for the ventral suction disk, collection depth resulted in the lowest accompanying AIC values (Table  3). When depth was treated as a categorical variable by ocean zone, depth trends for most bones matched those found in Table 3, with the exception of the Individual bones varied in density across the specimens studied. Within each specimen, relative bone density of each structure remained consistent, with otoliths being the densest structures measured (two-way ANOVA vertebra:otolith F 1,9 = 13.71, p = 0.0049; lower jaw:otolith F 1,9 = 15.72, p = 0.00328; disk:otolith F 1,5 = 7.554, p = 0.0404; hypural plate:otolith F 1,4 = 5.641, p = 0.0764). The disk was generally denser than the other bones measured (disk:vertebra F 1,18 = 81.08, p < 0.0001; disk:lower jaw F 1,18 = 52.71, p < 0.0001; disk:hypural plate F 1,11 = 128.8, p < 0.0001), followed by the lower jaw (lower jaw:vertebra F 1,36 = 277.1, p < 0.0001; lower jaw:   Minimum and maximum depth are provided for reference. *The externally visible suction disk of Careproctus ostentum was not evident in the scan. Depth sources are shown in Table 4 hypural plate F 1,14 = 169.6, p < 0.0001), the vertebra (vertebra:hypural plate F 1,14 = 127.9, p < 0.0001), and finally the hypural plate. A few species deviated substantially from this trend. The vertebra and lower jaw of Liparis tessellatus were substantially denser than the hypural plate and disk. Liparis fabricii had a comparatively lowdensity vertebra relative to other bones. Nectoliparis pelagicus, the only exclusively pelagic species analyzed, had the lowest density otoliths, both overall and relative to its bony skeleton (Supplementary Table 1).
Density and dimension of skeletal structures were often correlated, as shown in phylomorphospace visualizations (Fig. 9). For example, in certain deep-living taxa, lower jaw ossification and reduced dentary length were present, while some low-density, shallow-living taxa showed little reduction in dentary length (Fig. 9a). Vertebral density and neurocranium length showed a similar trend, though the relationship was less pronounced (Fig.  9b). The polar taxa Liparis tunicatus and Liparis fabricii displayed lower-density bones than others in the genus,  as was also visually evident (Fig. 8). A generalized reduction in suction disk density with increasing habitat depth was accompanied by a decrease in disk width (Fig. 9c).
There were also visual differences in density among specimens in bones that were not quantitatively analyzed. The neurocranium especially appeared to exhibit a wide range in density, with deep-water species tending to be less dense compared to intertidal species (Fig. 7), although this trend seems non-linear. While the neurocranium was reduced in density with increasing habitat depth, a crescent of more visibly ossified bones remained-the jaw bones, branchiostegal rays, and pectoral girdle. In analyzing the micro-CT three-dimensional images, we noticed a shift toward more rod-like narrow bones in species found at greater depths. This was especially clear in the maxilla and opercular series. In some species, such as Paraliparis paucidens and Elassodiscus tremebundus, variations in density in the other jaw bones were apparent, with a plate-like region of low density bone surrounding a rod of higher density bone.
The relationship between bone density and depth was found to be complex and non-linear. Bone density also seemed to be related to other ecological parameters, such as lifestyle and latitude, which are provided for all taxa in Supplementary Table 3, as well as to phylogenetic relationships. There are only a few liparids that are exclusively pelagic, limiting statistical power in comparing bone density across habitats. Qualitatively, however, vertebra and jaw densities appeared to be lower in pelagic species than in demersal taxa. Nectoliparis pelagicus had the lowest density otoliths. Pelagic species lacked suction disks, so disk density could not be compared across lifestyles. When accounting for phylogeny, latitude was a significant predictor of vertebral density, with

Discussion
Using micro-CT scanning, we found evidence for declines in skeletal dimension and loss of pelvic suction disks with increasing habitat depth in the snailfishes. The anecdotal reports of reduced bones in deep-sea fishes were supported in part by the present analysis, but our results reveal complexity in this relationship not previously described and challenge the paradigm that deepsea fishes have decreasing bone density with increasing Fig. 7 Visualization of bone density with habitat depth across the snailfishes, shown in micro-CT scan images. Brightness settings are standardized throughout the figure, serving as a proxy for bone density. Decreasing density is apparent with increasing maximum habitat depth in the family. Species are grouped by genera in columns, with depth on the y-axis. Scale bars are 1 cm habitat depth. In the snailfishes, bone density appears to be related not only to depth, but to lifestyle and habitat. Our qualitative results suggest that pelagic and polar species have lower-density bones, providing an important direction for future study. There are three different routes to skeletal loss -loss of elements, reduction in element size, and reduction in mineralization of elements. We found different lineages that show each of these and some combinations. Together, our results indicate that multiple environmental drivers influence skeletal declines in snailfishes. These drivers include, but are not limited to, increasing hydrostatic pressure. Skeletal reductions in fishes affect multiple physiological functions, including buoyancy, feeding, and locomotion; the implications of which are discussed below.

Buoyancy
Increasing hydrostatic pressures have been hypothesized to drive bone reductions in deep-sea species. However, our results suggest that the influence of increasing hydrostatic pressure on reducing bone density is both indirect-as a means to maintaining neutral buoyancy or a response to other environmental conditions-rather than a direct effect on bone mineral formation and not the only environmental factor important for bone density. Maintaining neutral or near neutral buoyancies is increasingly difficult for fishes under high hydrostatic pressures of the deep sea, where gas-filled swim bladders are energetically costly to inflate [89,96]. Fishes have multiple strategies for achieving neutral buoyancy, including large lipid deposits [23,27], gelatinous tissues   [28,40], and low-density cranial fluids [49]. Skeletonwide reductions were visible when comparing shallowliving and deep-living taxa of the present study (Fig. 7). Our finding that pelagic taxa seem to have lower density bones than demersal taxa, independent of habitat depth, support the idea that maintaining buoyancy is a strong driver of skeletal reductions. Further, shallower-living polar taxa that lack swim bladders can still achieve neutral and near-neutral buoyancy with reduced skeletal density, such as the notothenioids [26]. We show here that polar liparids also follow this trend. Lower locomotory capabilities and metabolic rates in deep-sea species [24] would also drive increased evolutionary pressure to maintain neutral buoyancy for energetic efficiency. We observed a clear reduction in ossification and length of the neurocranium in deep-water species. The dorsal portion of the skull was frequently one of the least dense areas observed in deep-sea specimens. A recent study describing the genome of the Mariana snailfish, Pseudoliparis swirei, also noted that this species has an incompletely ossified neurocranium or "open skull," which the authors interpret as a necessary adaptation to survival at high pressure because a "closed skull" would pop under hadal pressures [108]. While our findings and experience with dissections agree with this observation of reduced skeletal density in the bones of the neurocranium, we interpret this result differently. Reduced ossification of the neurocranium is not an adaptation for pressure equalization with the surrounding environment, but rather a means to achieve neutral buoyancy and a result of reduced selective pressures for strong protective skulls in the hadal environment. The logical flaw in the "open skull" hypothesis is that no skull is a completely sealed chamber of bone. The brain sac, within the skull, serves to maintain intracranial pressure in terrestrial vertebrates. In some fishes, these brain sacs are wellossified (e.g. [44]), but all have openings in the bone for connections to the nervous system. With the contextual CT data from shallow-living liparids presented here, it is clear that snailfishes, like all vertebrates, do not have skulls that are completely sealed with bone, even in shallow-water environments. As another illustration, mackerel are commonly used as bait in hadal camera and trap deployments (e.g. [61]). Although these are shallow-living fishes, their skulls show no pressurerelated mechanical damage upon retrieval from 10,000 m. Rather than an adaptation to physiological stress of high pressure, the reduction in bone mineral density of the neurocranium may be possible as a result of the reduced predation pressure on organisms in the deep sea [46], particularly in the case of the hadal snailfishes, which are the top known predators of the hadal zone [41]. It is likely that the majority of the bone is replaced by large areas of cartilage, as in the Antarctic snailfish, Paraliparis devriesi [28].
Does hydrostatic pressure have a direct physical effect on bone mineral density? Otoliths are calcium carbonate structures formed passively, in contrast to bones (e.g. [9,18]), thus serving as a test of the direct pressure effect on bone mineral density. We found that the density of the sagittal otoliths did not decline with increasing collection depth, suggesting that the depth-related density Fig. 9 Phylomorphospace visualization of bone density with habitat depth (m), considering phylogeny. Connections between data points indicate phylogenetic relationships. Colors represent standard-length corrected dimensions of related bones (red: longest, blue: shortest). a Lower jaw density with minimum depth, color indicates body size-corrected dentary length. b Vertebra density with maximum depth, color indicates body size-corrected neurocranium length. c Disk density with maximum depth, color indicates body size-corrected maximum disk width declines seen in other structures are not a direct physical effect of pressure. Interestingly, hadal snailfishes live well below the calcium carbonate compensation depth, where calcium carbonate dissolves faster than it can be formed due to the effects of pressure (e.g. [5]). The Mariana snailfish, Pseudoliparis swirei, also showed fully mineralized otoliths (Supplementary Table 3), despite its great habitat depth of 6000-> 8000 m, suggesting differences in the internal environment rather than the surrounding seawater. Our findings that lifestyle and habitat strongly influence bone density also indicate that reductions in bone density are not driven by physical pressure effects on mineralization.

Feeding
Decreases in bone size were not restricted to the neurocranium as predicted, but rather seen variably in the dentary and suborbital bones. Reductions in bones used for feeding need to be considered within that ecological context. In fishes that have protrusible jaws, a long ascending process allows the premaxilla to slide forward and downward when the jaws are opened (e.g. [109]). This jaw protrusion greatly enhances the forces exerted on prey during suction feeding [48] and moves the opening of the mouth closer to the prey in a behavior termed "jaw ram" [62]. Thus, it is likely important to maintain a long ascending process due to its important role in enabling effective suction feeding, even at great depths. The lack of a decrease in ascending process length with depth could indicate that the ascending process is a more critical portion of the premaxilla bone structure to maintain for effective feeding under the evolutionary pressure for a reduced skeleton.
The maxilla also plays a crucial role in suction feeding by rotating forward to form the bounds of the rounded gape and by applying force to the premaxilla to direct anterior jaw protrusion [25,31]. The lack of correlation between maxilla length and width and increasing depth indicates the evolutionary importance of maintaining the proportional dimensions of the oral cavity for suction feeding at all depths. The observed prevalence of more rod-shaped bones and visible declines in bone mineral density across the surface of the bone in deep-water specimens might indicate a selective pressure to reduce cross-sectional area of the bone. Thus, the feeding functionality of the bone is maintained while also reducing total bone volume in response to deep-water environmental constraints.

Locomotion
Reductions in vertebral density with increasing minimum depth of occurrence (polar taxa excluded) may correspond to reduced locomotory capability. This may be in part due to an increase in swimming efficiency and a tendency toward elongation in deep-water species [70]. It is likely that energy savings and metabolism are main drivers that influence adaptation into deep-sea habitats (e.g. [70]). The decrease in metabolic rates with increasing habitat depth is thought not to be a result of only high pressures and low food availability, but rather a decrease in interaction distances between predator and prey with declining light levels [11,24]. In surface waters, where visual cues dominate predator-prey relationships, these interactions occur over a larger spatial scale. At depth, where mechano-and chemo-sensory signals dominate the sensory landscape, fishes are not under such selective pressures to cover large distances and maintain high metabolic rates. This visual interactions hypothesis seems to be reflected not only in metabolic rates of deep-sea demersal taxa (e.g. [22]), but also in watery muscles (e.g. [21,112]), and decreased bone density (Present Study). Declining light levels bring decreased selective pressure for robust skeletons and fast swimming, as reflected by the decline in third vertebra densities with increasing habitat depth when excluding polar taxa, although limited to an alpha threshold of 0.1. Hypural plate densities, which would also be indicative of locomotory capabilities, did not significantly decline with increasing habitat depth, although sample sizes for this bone were comparatively small. It is also possible that reductions in pectoral girdle length could be due to the variation in pectoral girdle shapes observed.
We found depth-related declines in the width of the suction disk and loss of the suction disk in some deeperliving taxa. A decrease in wave action and flow rate with increasing depth likely reduces the need for strong suction disks [1]. Predation risk also declines significantly with increasing depth [46], decreasing the need to hide on and among rocks with the help of the suction disk. However, not all deep-living species have lost the ventral suction disk. At least two deep-water snailfishes have been observed using the suction disk in situ, Careproctus ovigerus and C. melanurus [107], suggesting that despite lower predation risks and current speeds, the suction disk remains useful in some deep-sea groups. There is a strong phylogenetic component to disk reduction and loss (e.g. [82]), which could mask habitat effects in our phylogenetically corrected analysis of bone density. Our ancestral state reconstruction results agree with the predictions of Orr et al. [82], which suggest at least three independent losses of the pelvic suction disk across the evolution of the snailfishes.

Habitat differences
While habitat depth was found to be a significant predictor of skeletal form across several bones, depth is not the only factor that characterizes a species' environment.
Bone density appeared to be lower in both polar and pelagic taxa, independent of depth. Liparis fabricii and Liparis tessellatus (e.g. [10]), both Arctic species, showed dramatically low bone densities. Further, Liparis fabricii can be pelagic and in our qualitative analyses, we observed that pelagic taxa (e.g. Lipariscus nanus, Nectoliparis pelagicus) displayed low-density bones. The differences we observed between bone density in pelagic and demersal taxa were non-trivial. For example, the estimated mean of vertebra and lower jaw density in pelagic taxa were three times lower than the means of demersal species, although this comparison has limited statistical power due to the low number of extant pelagic liparids. Evolutionary history could also constrain bone density. For example, Lipariscus nanus, which lives in the ocean's upper 1000 m, is most closely related to the deeper-dwelling snailfishes of the genus Paraliparis. The low-density bone in L. nanus may reflect a radiation into shallower water from a deeper population in addition to the species' pelagic lifestyle. Low-density polar species and the observed depth-related declines in bone density, suggest that temperature could be an important evolutionary driver of bone density, in addition to hydrostatic pressure.

Depth metrics
Our results varied depending on the different depth metrics chosen: collection depth, minimum habitat depth, and maximum habitat depth. Liparid habitat depth ranges can be large (e.g. Figure 10), so it is likely that changes in bone density are gradual and can be masked by overlapping depth ranges when considering just minimum habitat or specimen collection depth. We know also that the habitat depth information presented here is incomplete. Some species are known from only one or two collections. Further, while extremely valuable, databases such as FishBase [33] do not always provide full habitat characterizations for each species or can present erroneous depth values. With missing values and the potential for confounding ranges due to nonclosing collection equipment, it is important to use such databases as a starting point, but follow with deeper research into the primary literature and museum archives to confirm ranges (e.g. [85]). Basing our analysis on the  Table 4). This phylogenetic tree was visualized using the Interactive Tree of Life (iTOL [60];). Taxa analyzed in this study are shown in bold, with depth ranges in black. Depth ranges for taxa not analyzed in this study appear in gray. Sequences were available for 117 of the 430 described snailfishes, covering all major genera in the family. The maximum depth for Nectoliparis pelagicus shown here is believed to be greatly overestimated due to open trawl collections [10] and was not used in statistical analyses in the present study most complete information possible and testing multiple habitat depths provided additional insights into depthrelated trends.

Should depth-related trends be linear?
We do not see significant declines between 0 and 100 m habitat depth (e.g. Figure 8), which is as expected given pressure effects on physiology are negligible at these depths (e.g. [101]). It is also likely that depth-related changes in deep-sea fish skeletons are not linear. Depth in and of itself is not an environmental factor of biological relevance. Indeed, the only environmental driver that changes linearly with depth is hydrostatic pressure (e.g. Supplementary Fig. 2). Our results suggest that other environmental drivers influence skeletal density and dimension, such as declining light levels and changing temperatures. If temperature, light, and nutrient availability drive skeletal evolution, we would expect to see the greatest changes in bones in the first 1000 m from the surface. Most of the species we analyzed live in the 0-1000 m range, so it was not possible to fully explore the nuances of depth-related declines in skeletons in bathyal and abyssal habitats. With additional sampling, particularly in deeper waters near and beyond 4000 where few liparids have been collected (e.g. [37], Fig. 10), this hypothesis could be tested. In addition to increasing depth resolution, future studies should directly test for the effects of varying environmental parameters such as temperature and light and nutrient availability on bone density in fishes.

Ontogeny and future directions
Ontogeny is also an important consideration in assessing both depth metrics and density results as a whole. Many deep-sea fishes show ontogenetic changes in distribution, moving to different habitat depths throughout their lives, for example downslope migration in Microstomus pacificus, Dover sole (e.g. [52]). Compositions of muscle tissue are known to change with these changes in habitat depth [21]. It is possible that bone density and relative dimension also changes with ontogeny. Little is known about snailfish ontogeny [38,63,100]. Limited sampling and life history information has precluded full analyses across sizes, ages, and sexes in the snailfishes. Future research should examine bone density across life history stages by focusing on specific genera to better resolve these trends. Our observations here also call for further investigation of bone density in polar taxa and detailed comparisons of skeletal morphology between fishes with pelagic and demersal lifestyles.

Conclusions
Snailfishes have at least two routes for bone reduction in response to deep-sea environmental conditions: reduction of bone size and loss of unused skeletal elements. Reduction in bone size in the neurocranium, suborbital, dentary, and disk width indicate a complex response to environmental conditions in the deep sea. Bone size was differentially reduced with increasing habitat depth in each functional system (jaw, pelvic suction disk, and neurocranium) to retain specific key functions in feeding and swimming. Bone density of the vertebrae and otolith decreased by ocean zone, while density of the hypural plate, lower jaw, and ventral suction disk did not. These declines could be associated with trends for increased paedomorphy across depth and phylogeny in the snailfishes [26,63]. Skeletal reduction may be less constrained in fishes because bones have little role in calcium regulation compared to terrestrial vertebrates.
Our visual results support the general idea that bone density decreases in deep-sea fishes, but there is complexity in this trend that contradicts the prevailing paradigm, presumably driven by both physiological and ecological drivers. We found that latitude also significantly predicted bone densities, more so than habitat depth, and qualitative trends in density were apparent with species' lifestyle (i.e. pelagic vs. demersal). Working within one family (Liparidae) allowed systematic testing of skeletal declines with depth, reducing the influence of phylogeny. We propose that these trends apply across other families under the influence of the same ecological drivers. Future studies should test skeletal reduction across other wide-spread demersal taxa covering broad bathymetric ranges, for example the rattails (Macrouridae), cusk eels (Ophidiidae), eelpouts (Zoarcidae), and cutthroat eels (Synaphobranchidae). The varied ecology and physiology of these other taxa may provide additional insight into the drivers and adaptations of skeletal reductions in deep-sea fishes.

Micro-CT Scanning of Snailfishes
To visualize skeletal morphology and compare relative bone densities of 50 species among 13 genera across the family Liparidae, we used micro-computed tomography (micro-CT), a non-destructive sampling technique (Fig. 10). Specimens spanning collection depths of 0-8000 m were loaned from the University of Washington Burke Museum Ichthyology Collection (UWFC), the University of Hawaiʻi (from J.C. Drazen, Careproctus longifilis, [107]), and the Smithsonian Institution's US National Museum of Natural History (USNM, Table 4). Prior to scanning, specimens were photographed and standard lengths, total lengths, and head lengths were measured in ImageJ (Schneider et al., 2012). Specimens were scanned in batches (1-12 individuals) in a Bruker SkyScan 1173 at 65 kV and 123 μA with a 1 mm aluminum filter to reduce beam hardening (e.g. [6]) at the Karel F. Liem Bioimaging Center, Friday Harbor Laboratories, University of Washington. Scan resolution (voxel size) ranged from 14.9 to 35.5 μm, depending on the size of the fish. Knowndensity standards of 25 and 75% hydroxyapatite called phantoms either 7.5 or 10.5 mm in diameter were included in each scan to relate relative brightness to density. The inclusion of the same phantoms of similar thickness to the fishes in each individual scan allowed for a reduction in beam hardening to minimize inconsistency in X-ray attenuation. Scans were reconstructed using NRecon (Bruker, 2005-11) under standard procedure for optimal x/y alignment, ring artifact reduction, beam hardening correction, and post-alignment. The reconstructed scans were further segmented in DataViewer (Bruker, 2004-11). All scan reconstructions from this study are freely available for download on MorphoSource (Duke University).

Quantification of skeletal morphology and density
To test the first hypothesis-that dimensions of select skeletal structures are reduced with increasing habitat in fishes-we measured linear dimensions of bone regions in Horos [17]. We chose 12 dimensions and four bone regions to capture functionally relevant structural variation among species and size. Jaw measurements were as follows: maxilla length, maxilla width, premaxilla length, length of the ascending process of the premaxilla, dentary length (dorsal process), dentary length (ventral process), and anguloarticular length. Skull measurements included neurocranium length and suborbital length and width. On the ventral side of the fish, we measured the maximum width of the pelvic suction disk. Lastly, we measured the length of the pectoral girdle, the linear distance from the dorsal end of the scapula to the ventral end of the coracoid. These bones are illustrated in Fig. 1.
To test the second hypothesis-that skeletal structures that are not selected for in deep-sea habitats would be lost with increasing depth-we examined scans for missing skeletal elements. Following identification of specific lost structures, ancestral state reconstruction using a maximum likelihood framework was used to estimate the number of independent losses of certain skeletal elements among liparids. With the phytools package [94] in the statistical programming platform R [91], we obtained marginal ancestral state estimates and the phylANOVA function to test for an effect of depth in predicting structure loss.
To test the third hypothesis-that bone density decreases in fishes with increasing habitat depth-we used the 3D processing software Amira [103] to measure mean pixel brightness of individual bones as a proxy for bone density. For data visualization in Amira, colormaps were standardized across scans using a standard curve to achieve a range representing 10-90% hydroxyapatite. To reduce uncertainty at the variable ends of the brightness spectrum, all pixel values beyond the edges of this range became minimum (black) or maximum (white) values. This standardized the color scale to allow scans to be compared visually, with darker regions corresponding to lower X-ray absorption, or density, and lighter regions corresponding to higher absorption or density (e.g. [95]). These brightnesses were compared to known-density phantoms and converted to percent hydroxyapatite. These results are a proxy for bone density, rather than a direct calculation of density, and are treated as relative and purely for purposes of comparing taxa here. We compared relative densities of the third vertebra, lower jaw, first left disk pterygiophore, hypural plate, and sagittal otoliths (Fig. 2). The third vertebra was chosen for consistent Standard lengths (SL) are shown in mm, depth in meters (m). References for species' depth ranges are listed (min depth; max depth). Some museum specimens from the UWFC extend the published depth ranges for these species; these are noted as sources. All are museum specimens except Careproctus longifilis, whose collection is described by [107]. Collection depth for Careproctus acanthodes represents the collection lot and is considered an estimate. UW 154989 (Lipariscus nanus) and UW 155729 (Nectoliparis pelagicus) are pelagic species that were collected with non-closing benthic trawls comparison between specimens. Vertebral density varied visually across the fish, with posterior-most caudal vertebrae appearing less bright than anterior vertebrae. The first and second vertebrae were sometimes fused, while the third was markedly distinct from the neurocranium. Brightness data were not available for all five bones in each specimen. Due to otolith extraction upon collection, phylogenetic loss of suction disks, and loss of specimen tails, some bones could not be measured. Degrees of freedom for each relationship are shown in Table 3 and reflect sample numbers available.

Preservation effects
Upon collection, liparids are preserved in a standard solution of 4% buffered formaldehyde, then eventually transferred to 70% ethanol or 50% isopropanol for analysis and long-term storage. If the formalin is unbuffered, the acidic solution can dissolve hard structures in the specimen. Unfortunately, complete records of preservation and the amount of time specimens spent in different preservatives were not available for all museum specimens analyzed here. To test for potential confounding effects of preservation on our bone density measurements, we analyzed the relationship between collection year and pixel brightness. There was no significant relationship between depth and collection year (one-way ANOVA; collection depth: F There was a correlation between collection year and dentary density, significant at the α = 0.05 threshold, although it is unclear what is causing this decline. Bones in the same specimen of similar rod-like shapes, such as the disk pterygiophore did not correlate in density with collection year. We conclude that preservation did not significantly influence our findings presented below.

Data analysis
Statistical analyses were conducted in R [91]. To control for the effects of covariation in closely related species [30], phylogenetic generalized least squares (PGLS) models were used to investigate the relationship between habitat depth on bone dimension and density using the comparative method packages ape [83], PHYLOGR [20], nlme [87], and phytools [94]. We corrected all morphological data to specimen standard length by computing residuals of phylogenetic generalized least squares models using the function "phly.resid" in the phytools package. We reconstructed phylogenetic relationships of liparid species in our study according to the genetic tree presented by Orr et al. [82]. Cytochrome c oxidase subunit I (COI) sequences were aligned using MUSCLE [29], and a maximum likelihood phylogeny was prepared using RAxML [104] via the CIPRES Science Gateway [68]. Full details on the sequences and phylogeny construction are presented in Orr et al. [82]. We then pruned the phylogeny to only include species in our study for analysis. The ancestral state reconstruction was created using the function simmap with 1000 simulations and the ARD model [4,94]. Deep-sea fishes, including snailfishes, can inhabit broad depth ranges throughout their lifetimes, on the order of thousands of meters (e.g. [10,52,88]; Fig. 10). As such, it can be difficult to capture the full habitat depth range of a fish with one metric. To test the effects of habitat depth on skeletal dimensions and bone density, we conducted our statistical analyses using collection depth of individual study specimens, as well as minimum and maximum depth for the species from the literature. Sources for each of these depth ranges are listed in Table 4. This combination of metrics has been an effective way to test depth-related biological parameters in fishes in previous studies (e.g. [22]). To test for broad categorical trends, we binned depths roughly by ocean zone (0 to 10 m, 10 to 200 m, 200 to 1000 m, 1000 to 3000 m, 3000 to 6000 m, and 6000 to 11,000 m), in addition to treating depth as a continuous variable. Intertidal collections from 0 m were corrected to 0.1 m for log transformations. To explore the effects of lifestyle on bone density, taxa were classified as either pelagic or demersal according to the literature (e.g. [10]). Comparisons between pelagic and demersal taxa are treated as qualitative throughout the study because there are very few extant pelagic liparids, limiting statistical power (Supplementary Table 3). We also investigated latitudinal density variation according to the latitude of the species holotype as found in Eschmeyer's Catalog of Fishes [32]. Statistical results from each of the three depth metrics and latitude are reported and discussed. For each PGLS model, a coefficient and p-value are reported with α significance levels set at 0.05 and 0.1. The α threshold of 0.1 increases the risk of Type I error. We report both significance thresholds to most thoroughly examine the dataset and discuss limitations of these conclusions throughout the manuscript. Akaike Information Criterion (AIC) values were used to compare PGLS models built with different depth metrics. We would like to sincerely thank the scientists, ships, crews, and supporting agencies that collected the specimens used in this study and the museums and collections staff that make them available. Thanks to Schmidt Ocean Institute and the captain and crew of the RV Falkor. We particularly thank the staff of the RACE Groundfish and Shellfish Assessment Programs of the U.S. NOAA Fisheries Alaska Fisheries Science Center, who collected most of the specimens used in this study. The scientific results and conclusions, as well as any views or opinions expressed herein, are those of the author(s) and do not necessarily reflect those of NOAA or the Department of Commerce. Without these many people spanning decades of work, this research would not have been possible. We thank Katherine Maslenikov and Luke Tornabene at the Burke Museum (University of Washington, USA) and Jeffrey Drazen (University of Hawaiʻi at Mānoa, USA) who provided specimens from collections for CT scanning. We are grateful to Matthew Kolmann (University of Michigan, USA) and Rikki Tsoi (University of Washington, USA) for scanning support. We thank our funding sources for research support, including the Seaver Institute, Whitman College Internship Grant, the Mary Gates Endowment Research Scholarship, and an anonymous donor for supporting conference travel for AD to present this work at the Society of Integrative and Comparative Biology. We thank the Karel F. Liem Bioimaging Center at Friday Harbor Labs, University of Washington, the State University of New York at Geneseo, and the National Science Foundation-supported Open Vertebrate (oVert) grant DEB-1701665.

Animal ethics
This study used museum specimens exclusively. Museum specimen numbers are provided in the manuscript and supplementary material.
Authors' contributions MEG, SF, AvH, ASD, and APS devised the study. ASD, AvH, APS, and MEG collected scan data. ASD and AvH analyzed CT scans. Data analysis was conducted by MEG and SF. ASD, AvH, and MEG made the figures. JO contributed phylogenetic data. All authors wrote, edited, and approved the final manuscript.
Funding CT Scanning at the Karel F. Liem Bioimaging Center was supported by the National Science Foundation (oVert Grant DEB-1701665, to APS). We thank the NSF Postdoctoral Research Fellowship in Biology (DBI-1523836), Cornell CORALS program, University of Washington's Honors Undergraduate Scholarship, and the Mary Gates Endowment Research Scholarship for support. Environmental data in Supplementary Fig. 2 was obtained via the Hawaii Ocean Time-series HOT-DOGS application University of Hawaiʻi at Mānoa. National Science Foundation Award #1756517. AD was supported by a Whitman College Internship Grant and student research funding from Whitman College. MEG was supported by the Seaver Institute, Friday Harbor Labs, University of Washington, and the State University of New York at Geneseo.

Availability of data and materials
All CT scans from the present study are available open access on MorphoSource. Length, density measurements, and scan renderings are presented in the manuscript and supplementary materials.

Declarations
Competing interests