Study Area and Study Site Delineation

The study area consisted of two large, microtidal (tidal range <0.5 m; Rozas 1995) river estuaries in coastal Mississippi (Figure 1a). The lower Pascagoula River estuary (PRE) is an approximately 15-km-long distributary that can be subdivided into eastern and western branches. The eastern branch has been highly altered and is bordered by intensely developed surfaces and hardened shorelines, while the shorelines of the western branch remain comparatively less modified and possess large expanses of intact natural habitats (Peterson et al. 2007; Partyka and Peterson 2008). The Biloxi Bay estuary (BB) is approximately 21.7 km in length and also consists of both highly impacted and unimpacted shorelines; however, the impacted shorelines are not as aggregated as those in the PRE. In both systems, altered shorelines include erosion control edges in the form of levees, rip-rap, and residential and commercial bulkheads (Peterson and Lowe 2009). Natural shorelines consist mostly of intertidal vegetation dominated by smooth cordgrass Spartina alterniflora and needlerush Juncus roemerianus, with occasional patches of the invasive common reed Phragmites australis (Peterson and Partyka 2006). Although both systems receive considerable freshwater input from upstream water-sheds, the Pascagoula River has considerably higher discharge rates than the Biloxi River (Lowe et al. 2012).

Previous work in these estuaries identified salt-marsh landscapes that ranged from natural to highly urbanized (Peterson et al. 2000; Partyka and Peterson 2008). These observations were combined with 2007 1-m orthorectified color infrared imagery in ArcGIS version 10.0 (Environmental Systems Research Institute) to identify within each estuary three potential sample sites that (1) contained small, first-order salt-marsh tidal creeks of similar lengths (all creeks ranged from 26.6 to 32.4 m long) and (2) were arrayed along a gradient of anthropogenic alteration from natural to highly altered local landscapes (Figure 1). Small, first-order tidal creeks draining large expanses of salt marsh with no evidence of shoreline alteration or development in the immediate vicinity (750–1,000 m) were considered intact natural (IN) salt-marsh landscapes (Figure 1b, 1e). Partially urbanized (PU) landscapes were identified as small, first-order tidal creeks draining marsh systems that were nestled within a moderately developed area, with modified shorelines disrupting the creeks' natural connection to the main water body (Figure 1c, 1f). Small, isolated salt-marsh patches that contained a small first-order creek and that were surrounded by both altered shorelines and developed surfaces were identified as completely urbanized (CU) landscapes (Figure 1d, 1g). Prior to sampling, each tidal creek and its surrounding landscape were examined to ensure the correct assignment to one of the three landscape types.

FIGURE 1.

(a) Map of the study area, including the 2005 land cover data for the Biloxi Bay estuary (BB) and Pascagoula River estuary (PRE), Mississippi (examples of landscape types are shown: triangles = intact natural [IN]; circles = partially urbanized [PU]; squares = completely urbanized [CU]). Inset panels depict examples of each landscape type (represented by symbols in panel a): (b) IN landscape in BB; (c) PU landscape in BB; (d) CU landscape in BB; (e) IN landscape in PRE; (f) PU landscape in PRE; and (g) CU landscape in PRE. Small and large circles in each panel represent the corresponding 250- and 750-m radial buffers used for landscape analyses. For the purpose of this work, the original classes for developed land (e.g., developed open space and high-, medium-, and low-intensity developed class) and estuarine wetlands (i.e., estuarine forested wetland, estuarine scrub or shrub wetland, and estuarine emergent wetland) were reclassified as “developed” and “salt marsh,” respectively.

Land Cover Data and Landscape Metrics

Land cover data for the study area in 2005 (after Hurricane Katrina; Figure 1a) were obtained from the National Oceanic and Atmospheric Administration's Coastal Change Analysis Program (C-CAP;  www.csc.noaa.gov/crs/lca/ccap.html). The C-CAP system classifies 30-m² (0.9-ha) pixels into 21 land cover classes at an overall accuracy of 85% (Dobson et al. 1995). For the purpose of this work, the original classes for developed land (e.g., developed open space and high-, medium-, and low-intensity developed class; cells containing 21–100% concrete, asphalt, or other constructed materials) and estuarine wetlands (i.e., estuarine forested wetland, estuarine scrub or shrub wetland, and estuarine emergent wetland) were re-classified as “developed” and “salt marsh,” respectively. The remaining classes were not modified.

For each sample site, ArcGIS Model Builder was used to extract a series of circular buffers at different spatial scales (radius = 250 or 750 m) centered on the mouth of each tidal creek (Figure 1e–g). These scales were considered spatially relevant for both less-mobile, resident species (e.g., Able et al. 2012) and more-mobile, transient species (e.g., Weinstein et al. 1984; Wolcott and Hines 1990; Saucerman and Deegan 1999). Within each GIS-rendered spatial extent, the extracted land cover data were used to calculate 10 spatial metrics (Table 1) at the class level and the landscape level by using FRAGSTATS version 4.0 (McGarigal et al. 2002). Primary emphasis was placed on the composition and configuration of the developed (DV) and salt-marsh (SM) classes in relation to the water (W) class. The percentages of the landscape occupied by the DV class (PLAND_DV) and SM class (PLAND_SM) were calculated for each spatial scale. Total edge (TE) and total edge contrast index (TECI) were used to estimate the relative amount of functional and nonfunctional class edges. For example, the amount of hardened shoreline (TECI_DV[W]) was calculated as W cell edges contrasted against DV cell edges, the amount of natural shoreline (TECI_SM[W]) was calculated as W edge cells contrasted against SM class cells, and the amount of salt-marsh edge that was bordered by developed surfaces (TECI_DV[SM]) was calculated as the amount of SM cell edge contrasted against DV cell edge (see Table 2). For the SM class, the complexity and aggregation of cells were calculated using the area-weighted mean shape index (SHAPE), the contiguity index (CONTIG), and the clumpiness index (CLUMPY). Salt marsh isolation was quantified with the connectivity index (CONNECT), which was used to describe creek connectivity within each spatial scale (proportion of small, first-order creek mouths in each buffer that were located within 250 m of each other; estimated from 2007 1-m orthorectified color infrared imagery in ArcGIS). Three spatial metrics were used to quantify the degree of salt marsh fragmentation (Jaeger 2000). The landscape division index (DIVI) was the probability (D) that two randomly chosen pixels in the landscape are not situated in the same salt-marsh patch. The splitting index (SPLIT) was defined as the number of salt-marsh patches (S) that resulted from dividing the landscape by the observed mean salt-marsh patch size while holding D constant. Effective mesh size (MESH) was the mean patch area obtained when the landscape was divided into S patches.

TABLE 1.

Spatial metrics calculated for each spatial extent (250 and 750 m) in the Biloxi Bay and Pascagoula River estuaries. Composition metrics (PLAND, TE, and TECI) were calculated for water (W), developed (DV), and salt-marsh (SM) classes. Configuration metrics (SHAPE-MESH) were calculated for the SM class only.

TABLE 2.

Derived spatial metrics for intact natural (IN), partially urbanized (PU), and completely urbanized (CU) sites in the Biloxi Bay estuary (BB) and Pascagoula River estuary (PRE) at 250- and 750-m spatial extents. Asterisks denote variables that were used for multivariate analyses. Landscape metrics and their units are defined in Table 1.

Faunal Collections

Weekly from May 3 to June 4, 2010, nekton and macroinfauna were collected and environmental variables were measured in each of the six tidal creeks (2 estuaries × 3 landscape types). Modified fyke nets with two 0.91 -m-diameter steel hoops positioned 1 m apart and with a single throat located on the first hoop (Memphis Net and Twine) were used to collect nekton in each creek. Fyke nets consisted of two wings (3 m long, 1.8 m high) and a mouth (3 m wide, 1.8 m high). Each net (including the wings and mouth) was constructed of 5-mm stretched nylon mesh, and the bottom of the net's leading edge was constructed with double-weighted lead line. Nekton were collected by placing the fyke net across the wet cross-sectional area of the tidal creek mouth at slack high tide (depth = 35.0–59.0 cm) and extending each wing onto the salt-marsh platform at an approximate 45° angle. Poles (10 cm in diameter, 4.0 m long) driven into the marsh platform were attached to the net at the float and lead lines on each side of the net mouth and at the end of each wing. Estuaries in the northern Gulf of Mexico are microtidal, and salt-marsh tidal creeks rarely drain completely except during extreme meteorological events (Rozas 1995). Therefore, once the tide had ebbed and all water had drained from the marsh surface (∼6 h after high tide), a 4.9-m minnow seine (3.2-mm stretched mesh) was pulled through about 75% of the total creek length (coinciding with the low-water mark) and into the mouth of the fyke net. The lead line was lifted out of the water, and nektonic organisms, including those in the wings, were funneled into the net mouth. Due to time constraints, a maximum of two creeks in the same estuary could be sampled on a given day. All nekton were removed from the cod end of the fyke net, placed on ice in the field, and returned to the laboratory, where they were frozen until they could be identified and enumerated. Nekton abundance in each fyke net was considered the CPUE.

Concomitant with nekton collections, environmental data (i.e., depth; temperature, °C; salinity, ‰; and dissolved oxygen [DO], mg/L; all measured with a hand-held YSI 85 meter) and macroinfauna were collected weekly at the mouth, middle, and head of each tidal creek (2 estuaries × 3 creeks × 4 weeks × 3 locations within a creek = 72 samples). Each macroinfaunal sample was taken from mid-channel by using a pole-mounted Ekman grab (0.024 m²); the sample was washed through a 500µm sieve in the field to remove excess mud, preserved in 7% buffered formalin containing rose bengal stain, and returned to the laboratory. Macroinfauna were sorted from each sample by using one of two methods. Samples with a high volume of detrital material were fluidized with 3.8–7.6 L (1–2 gal) of water and were quartered into approximately equal-volume samples with a Motodo plankton splitter; macroinfauna were then isolated from two of the four samples. Thirty-eight samples were split, and the mean difference in abundance between the two splits within a creek ranged from 3.1 to 4.0 total individuals (range of SD = 1.25–3.87; range of CV = 22–35%). The remaining 34 samples contained a low volume of detrital material, so macroinfauna were obtained from these samples in their entirety. All macroinfaunal samples were examined in random order in groups of eight samples, from which one sample was randomly selected for quality control. If the number of missed animals in a quality control sample was greater than 10% of the total animals that were observed during the first sorting event, then all eight samples were re-examined. Based on this criterion, one group of samples was re-examined and the percentage of animals that were missed ranged from 0.0% to 3.8%, with the initial quality control sample having missed 4 (11%) of 36 individuals. The remaining quality control samples ranged from 0% to 3% of animals missed. All macroinfaunal animals were identified to the lowest possible taxonomic level. Most individuals were identifiable to the species level. However, in taxonomic groups for which it was not possible to identify every individual to the species level, the lowest confirmed taxonomic level was used for classification purposes. To facilitate comparisons with other studies, macroinfaunal densities were scaled to 1 m² for all analyses.

Statistical Analyses

Univariate analyses.—Taxonomic richness and Simpson's evenness index (1—λ Clarke and Gorley 2006) were calculated for both nekton and macroinfaunal assemblages and were compared between estuaries (BB and PRE) and among landscapes (IN, PU, and CU) by using two-way ANOVA. An initial threeway ANOVA indicated that diversity measures for macroinfauna did not differ among locations within each creek (P > 0.05); as a result, the pooled samples for each week were treated as replicates.

Water temperature, salinity, DO, and depth were averaged across weeks and compared between estuaries and among landscapes and locations within the tidal creek (mouth, middle, and head) by using three-way ANOVA. For all univariate ANOVAs, relative F-values and associated effect size (partial η;²) values were used to assess the importance of significant interactions between main effects (Green and Salkind 2008). If the effect size of the interaction term was small (partial η;² ≤ 0.3; Field 2005) relative to the main effect or if there was no interaction, Tukey's honestly significant difference (HSD) post hoc test was used to examine significant differences among treatments for each variable. All variables used in univariate analyses were log₁₀ transformed and met the assumptions of normality (Kolmogorov—Smirnov test) and homogeneity (Levene's test). All univariate analyses were performed at an α level of 0.05 in SPSS version 20 (IBM).

Multivariate analyses.—Initial analysis of both nekton and macroinfaunal data indicated that collection week was not significant in any model and had negative variance component estimates (Fletcher and Underwood 2002). Therefore, samples were pooled across weeks for all multivariate analyses. Furthermore, macroinfaunal assemblages did not differ among locations within creeks (permutational multivariate ANOVA [PERMANOVA]: pseudo-P > 0.05) and were summed across all three locations for a given week to facilitate multivariate correlations with physical-chemical data by maintaining resemblance matrices of equal size. For both spatial scales, stationary landscape metrics were coupled with the dynamic environmental variables averaged weekly within each creek into a set of physical-chemical variables and were used to construct a resemblance matrix based on normalized Euclidean distance measures.

Rare taxa (those comprising less than 0.2% of total abundance for each assemblage) were removed, and a resemblance matrix of Bray-Curtis similarity values for each sample was created from fourth-root-transformed CPUE data (for nekton) or density (for macroinfauna) to downweight the importance of numerically dominant taxa (Clarke and Gorley 2006). Levels of similarity among samples (physical-chemical, nekton, and macroinfauna) were statistically compared between estuaries and among landscapes by using a full-factorial PERMANOVA (permutations = 999; Anderson et al. 2008). Due to issues associated with pseudoreplication, PERMANOVA is prone to type I errors (Atkinson et al. 2011). Therefore, conservative pseudo-F ratios, which were computed using the interaction error term as the denominator, were used in lieu of conventional pseudo-F ratios to assess the level of significance. Estimated variance components were used to assess the importance of significant main effects and interaction terms. Pairwise a posteriori comparisons using the multivariate analog of the t-test (pseudo-t) were made for each level of significantly different main effects and interaction terms. Patterns based on group average cluster analysis (CLUSTER) and similarity profiles (SIMPROF) were projected onto two-dimensional multidimensional scaling (MDS) ordination plots to examine the relationships among samples and to identify well-differentiated groupings. Rank dissimilarities (SIMPER) for nekton and macroinfaunal assemblages were used to identify characteristic taxa that were driving differences among (1) significant factors identified by PERMANOVA tests and (2) significant clusters identified by the CLUSTER and SIMPROF analyses.

The statistical agreement between physical-chemical and assemblage resemblance matrices was assessed with a nonparametric form of the Mantel test (RELATE; permutations = 999). Multivariate correlation (BEST; permutations = 999) was used to quantitatively examine the agreement between faunal assemblages and physical-chemical variables. The BEST procedure conducted rank correlations (coefficient p) to determine the scale of pattern matching between the physical-chemical resemblance matrix and each of the resemblance matrices for the nekton and macroinfaunal assemblages. This approach searches all possible combinations of physical-chemical variables (BIOENV function) to identify the subset of physical-chemical variables that give the best correlative explanation of the assemblage structure. The best subsets of physical-chemical variables were further investigated by using Pearson's product-moment correlations to relate individual species’ abundances to the landscape and environmental factors. All multivariate analyses were performed using PRIMER version 6.0 (Clark and Gorley 2006). Pearson's product-moment correlations were performed in SPSS.

Physical-Chemical Analyses

Environmental characteristics varied spatially throughout the study area and within the tidal creeks. Mean water depth at high tide ranged from 17 to 45 cm and differed only among locations within tidal creeks (ANOVA: P = 0.003), with the creek head being significantly shallower than the creek mouth (Tukey's HSD test: P = 0.002). Water temperature (range = 27.1–30.4°C) differed between estuaries (ANOVA: P = 0.001) and among landscape types (ANOVA: P = 0.04). On average, PRE was approximately 1.0°C warmer than BB (Tukey's HSD test: P = 0.03), and PU landscapes were about 1.5°C cooler than IN and CU landscapes (Tukey's HSD test: P = 0.03). Although DO concentrations (2.5–6.6 mg/L) fell within a suitable range for most estuarine nekton species (Wannamaker and Rice 2000), DO differed between estuaries (ANOVA: P = 0.003) and there was a significant estuary × landscape interaction (ANOVA: P = 0.017). However, both factors accounted for a similar amount of model variation (estuary: partial η;² = 0.152; estuary × landscape: partial η;² = 0.141) and precluded post hoc comparison of the main effect. Overall, DO concentrations were lower in BB (mean ± SE = 3.4 ± 0.7 mg/L) than in PRE (4.2 ± 0.5 mg/L), and this difference was further exacerbated by the lowest DO concentrations observed in BB-PU landscapes (2.7 ± 0.4 mg/L). Similarly, salinity differed among landscapes (ANOVA: P < 0.001; partial η;² = 0.474), and there was a significant estuary × landscape interaction (ANOVA: P < 0.001; partial η;² = 0.455). Both IN and CU landscapes were more saline than PU landscapes (Tukey's HSD test: P < 0.001), and the interaction was driven by higher salinities observed at the PRE-CU site (mean ± SE = 6.4 ± 1.0‰) relative to the BB-CU site (2.2 ± 1.0‰) and at the BB-IN site (6.7 ± 1.7‰) relative to the PRE-IN site (2.6 ± 0.9‰). However, observed mean salinities at all sites (1.9–8.4‰) fell within the oligohaline range for estuarine organisms (Bulger et al. 1993).

Regardless of estuary, the composition and configuration of the three coastal landscape types in this study were clearly different at both the 250- and 750-m scales (Table 2). In the IN landscape, SM was the dominant class (PLAND_SM). As a result, shoreline consisted almost exclusively of natural salt-marsh edge (TECLSM[W] = 89–100%). Salt-marsh cells within the IN landscapes tended to be aggregated (CLUMPY ≥ 0.8) and simply shaped (SHAPE = 1.2–2.0). Furthermore, tidal creeks were more connected at both the 250- and 750-m spatial scales (CONNECT = 63.7–74.4%) and were unfragmented (DIVI, MESH, and SPLIT). In both BB and PRE, PU landscapes were dominated by the SM class at the 250-m spatial scale (PLAND_SM = 64.1% and 55.9%, respectively). However, at the 750-m scale, PU landscapes were a mix of DV (PLAND_DV = 18.8% for BB and 50.3% for PRE) and SM (PLAND_SM = 24.5% for BB and 42.6% for PRE) classes. Overall, PU landscapes had more salt-marsh edge (i.e., TE) than either the IN or CU landscapes due to the large, convoluted creeks that are a dominant feature of the landscape and resulted in greater shape complexity (SHAPE = 1.9–2.1). However, the amount of natural shoreline (TECI_SM[W]) decreased inversely with the amounts of developed surface (PLAND_DV) and hardened shoreline (TECI_DV[W]), resulting in salt-marsh landscapes that were more urbanized (DIVI, MESH, and SPLIT) at the 750-m spatial scale. On the other hand, CU landscapes were dominated by the DV class (PLAND_DV = 30.0–64.9%), and hardened shorelines (TECI_DV[W]) constituted 42.3–52.8% of the shoreline in this landscape type. Salt-marsh patches in CU landscapes tended to be small (PLAND_SM = 3.5–17.3%), simply shaped (SHAPE = 1.1–1.3), moderately aggregated (CLUMPY = 0.5–0.6), and highly urbanized (DIVI, MESH, and SPLIT).

The conventional PERMANOVA indicated that physical-chemical variables differed between estuaries and among landscape types and that there was a significant interaction for both spatial scales (Table 3). However, variance components attributed most of the model variation to the landscape level, and the conservative model suggested that physical-chemical variables differed only among landscape types. In pairwise comparisons, all three landscape types were dissimilar at both the 250- and 750-m spatial scales. Further, due to the stationary nature of the landscape variables, all of the residual variance (i.e., within replicate) was attributable to the variation in environmental variables discussed previously. These results are corroborated by the MDS plots, which showed significant separation among the landscape types: four significant groupings were observed at the 250-m scale, and three significant groupings were observed at the 750-m scale (Figure 2).

TABLE 3.

Results of permutational multivariate ANOVA on normalized Euclidean distance matrices based on physical-chemical variables for 250- and 750-m spatial extents (landscape types: IN = intact natural; PU = partially urbanized; CU = completely urbanized) in the Biloxi Bay estuary (BB) and Pascagoula River estuary (PRE). Pairwise comparisons are the results of pseudo-t-tests (MSE = mean square error; ^* P ≤ 0.05, ^** P ≤ 0.01, ^*** P ≤ 0.001).

Nekton Assemblage Analyses

In total, 26,379 individual fish representing 36 species were collected (Table 4). Six species comprised approximately 94% of the total catch: Gulf Menhaden, Bay Anchovy, White Mullet, Gulf Killifish, Spot, and Sand Seatrout. Decapod crustaceans were represented by 35,714 individuals from six species (Table 5). Grass shrimp Palaemonetes spp. (73.3%), brown shrimp Farfantepenaeus aztecus (21.4%), and blue crab Callinectes sapidus (3.3%) dominated the total decapod crustacean catch. Nekton species richness differed only among the landscape types (ANOVA: P < 0.001) and was greater in PU landscapes (Tukey's HSD test; richness [mean ± SE] =18.1 ± 0.7) than in the IN (15.6 ± 1.2) or CU (15.3 ± 1.4) landscapes; PU landscapes, however, contained more freshwater species (e.g., Bluegill, Redear Sunfish, and Largemouth Bass) due to the lower salinity. Simpson's evenness index (1 — λ) differed only among landscapes (ANOVA: P < 0.01), and the nekton assemblage in CU landscapes (Tukey's HSD; evenness index [mean ± SE] = 0.68 ± 0.063) was more evenly distributed than that in either the IN landscapes (0.57 ± 0.023) or the PU landscapes (0.59 ± 0.031) due to the presence of highly abundant species (e.g., Gulf Menhaden and grass shrimp) in the latter two landscape types.

Once the rare species were removed from the data, 21 nekton species were retained for multivariate analyses (Tables 4, 5). Nekton assemblage composition differed between estuaries and among landscapes, and there was a significant estuary × landscape interaction (PERMANOVA; Table 6a). However, the conventional pseudo-F-test was compromised by a lack of independence among sampling units (i.e., weeks); the conservative pseudo-F-test showed that nekton assemblage composition differed among landscapes but not between estuaries. Despite attributing most of the model variation to the landscape level and residual error term, the interaction still accounted for a large portion of the variation, suggesting that the magnitude of the difference in nekton assemblages among landscapes was not similar across estuaries. Indeed, the PRE-PU and BB-PU landscapes differed markedly in the composition of their nekton assemblages. The MDS plots showed a similar differentiation among landscapes, with two significant groupings at 65% similarity (CLUSTER): group 1 contained all of the IN samples, the PRE-PU samples, and a single BB-CU sample; and group 2 contained the remaining PU and CU samples (Figure 3). Nekton assemblages in the IN and CU landscapes were most dissimilar (SIMPER; mean dissimilarity = 71.86%), followed by IN versus PU (mean dissimilarity = 58.39%) and PU versus CU (mean dissimilarity = 56.30%). Furthermore, the CPUEs of a few species (e.g., grass shrimp, Gulf Menhaden, brown shrimp, Spot, and blue crab) contributed much of the dissimilarity among landscape types (Figure 4) and between the two significant clusters (Figure 5).

FIGURE 2.

Multidimensional scaling (MDS) plots of the physical-chemical data for the (a) 250-m spatial extent and (b) 750-m spatial extent (landscape types: IN = intact natural; PU = partially urbanized; CU = completely urbanized) in the Biloxi Bay estuary (BB) and Pascagoula River estuary (PRE). Dashed contours identify significant clusters (based on Euclidean distance) from agglomerative hierarchical clustering and similarity profiles.

TABLE 4.

Mean (±SE) CPUE (individuals/sample) of fish species collected from intact natural (IN), partially urbanized (PU), and completely urbanized (CU) landscapes in the Biloxi Bay and Pascagoula River estuaries. Asterisks indicate species that were used in multivariate analyses (i.e., species comprising ≥ 0.2% of total abundance).

TABLE 5.

Mean (±SE) CPUE (individuals/sample) of decapod crustaceans collected from intact natural (IN), partially urbanized (PU), and completely urbanized (CU) landscapes in the Biloxi Bay and Pascagoula River estuaries. Asterisks indicate species that were used in multivariate analyses (i.e., species comprising ≥ 0.2% of total abundance).

Relationships between Nekton Assemblage and Physical-Chemical Patterns

Nekton assemblage patterns were significantly correlated with the physical-chemical patterns at the 250-m (BEST: global R = 0.59, P = 0.01) and 750-m (BEST: global R = 0.68, P = 0.01) spatial scales. For both spatial scales, the relative amounts of both natural salt-marsh edge (i.e., TECI_SM[W]) and developed shoreline (TECI_DV[W]) and the amount of salt-marsh habitat (PLAND_SM) were commonly correlated with the nekton assemblage patterns (Table 7). The three-variable model that included TECI_SM(W), PLAND_SM, and tidal creek connectivity (CONNECT) had the highest correlation with nekton patterns at the 250-m spatial scale (BEST: ρ = 0.571), but CONNECT alone was similarly correlated (BEST: ρ = 0.569). At the 750-m spatial scale, salt marsh fragmentation (SPLIT) was an important correlate of nekton patterns. For most nekton species, CPUE increased significantly with TECI_SM(W), PLAND_SM, and CONNECT and significantly decreased with increasing SPLIT (e.g., Gulf Menhaden, Bay Anchovy, Gulf Killifish, grass shrimp, and brown shrimp; Table 8). Conversely, the Sheepshead Minnow and Sailfin Molly were negatively correlated with CONNECT and positively correlated with SPLIT. Several species showed no correlation with any of these spatial metrics (e.g., Saltmarsh Topminnow, Spot, Southern Flounder, and blue crab).

TABLE 6.

Results of permutational multivariate ANOVA on fourth-root-transformed Bray—Curtis similarity matrices for nekton and macroinfaunal assemblages (landscape types: IN = intact natural; PU = partially urbanized; CU = completely urbanized) in the Biloxi Bay estuary (BB) and Pascagoula River estuary (PRE). Pairwise comparisons are the results of pseudo-t-tests (MSE = mean square error; ^* P ≤ 0.05, ^** P ≤ 0.01, ^*** P ≤ 0.001).

Macroinfaunal Assemblage Analyses

In total, 4,480 individual macroinfauna representing 25 taxa were collected in 72 Eckman samples (Table 9). Mean macroinfaunal densities (scaled to m²) ranged from 0.0 to 17,001.4 individuals/m². During the sampling period, the macroinfaunal assemblage was dominated by seven taxa: Chironomidae (midges; 29.87%), Capitellidae (polychaetes, 20.38%; includes Capitella capitata, Mediomastus californiensis, and Heteromastus filiformis), Tubificidae (oligochaetes; 17.66%), scuds Gammarus spp. (7.12%), the polychaete Amphicteis floridus (7.01%), Nereididae (polychaetes, 6.78%; includes Neanthes succinea, Laeonereis culveri, and Stenonineris martini), and the polychaete Streblospio benedicti (6.41%; Table 9). Taxonomic richness did not differ between estuaries (richness [mean ± SE] = 6.50 ± 0.78 for PRE and 5.91 ± 1.01 for BB; ANOVA: P = 0.63) or among landscapes (richness [mean ± SE] = 7.38 ± 1.27 for IN, 6.13 ± 0.90 for PU, and 5.63 ± 0.92 for CU; ANOVA: P = 0.25), and there was no significant estuary × landscape interaction (ANOVA: P = 0.15). Simpson's evenness index (1 — λ) did not differ between estuaries (evenness index [mean ± SE] = 0.55 ± 0.066 for PRE and 0.58 ± 0.042 for BB; ANOVA: P = 0.17) but was significantly different among landscapes (ANOVA: P = 0.008; partial η;² = 0.42), and there was a significant interaction (ANOVA: P = 0.02; partial η;² = 0.36) that accounted for a similar proportion of model variance. Although macroinfaunal assemblages in both PRE and BB were more evenly distributed in the IN (evenness index [mean ± SE] = 0.64 ± 0.047) and PU (0.57 ± 0.089) landscapes than in CU landscapes (0.42 ± 0.060), taxa were more evenly distributed in BB-PU (0.71 ± 0.039) than in PRE-PU (0.42 ± 0.079).

FIGURE 3.

Multidimensional scaling (MDS) plot of the nekton assemblages for each combination of estuary (Biloxi Bay estuary [BB]; Pascagoula River estuary [PRE]) and landscape type (IN = intact natural; PU = partially urbanized; CU = completely urbanized). Dashed contours identify significant clusters (based on Bray—Curtis similarity) from agglomerative hierarchical clustering and similarity profiles.

TABLE 7.

Multivariate correlation coefficients (p) between physical-chemical variables and the nekton or macroinfaunal resemblance matrices. Displayed are the top-four models from the multivariate correlation analysis (i.e., BEST) output (TEMP = temperature; SAL = salinity; other variables are defined in Table 1).

After the removal of rare macroinfaunal taxa, 13 taxa were retained for multivariate analyses (Table 10). The conventional PERMANOVA indicated significant differences in macroinfaunal assemblages at all levels, including a significant estuary × landscape interaction (Table 6b); however, the estimate from the conservative pseudo-F-test indicated that macroinfaunal assemblage structure did not differ between estuaries or among landscapes. Both the residuals and interaction term accounted for a large proportion of the model variation, suggesting that (1) macroinfaunal assemblages differed markedly among samples within sites and (2) differences in macroinfaunal assemblages were not consistent either across estuaries or across landscape types. The MDS ordination of the macroinfaunal resemblance data corroborated the PERMANOVA results (Figure 6), and six significant clusters were identified at 40% similarity.

FIGURE 4.

Mean (±SD) CPUE (individuals/sample) of the nekton species contributing to 90% of the cumulative variation among landscape types (IN = intact natural; PU = partially urbanized; CU = completely urbanized) in the Biloxi Bay and Pascagoula River estuaries. Mean dissimilarity between landscapes is shown in the upper left corner of each plot; mean (±SD) dissimilarity attributed to each species is indicated by the black circles. Note the difference in CPUE scale for the bottom panel (GSHP = grass shrimp; BSHP = brown shrimp; GMEN = Gulf Menhaden; SPOT = Spot; BLCB = blue crab; WMUL = White Mullet; SHMN = Sheepshead Minnow; PINF = Pinfish).

Relationships between Macroinfaunal Assemblage and Physical-Chemical Patterns

Despite the absence of a clear pattern, the macroinfaunal assemblage patterns were significantly correlated with the physical-chemical data at both the 250-m (BEST: global R = 0.32, P = 0.01) and 750-m (BEST: global R = 0.28, P = 0.01) spatial scales. For the 250-m spatial scale, three variables (TECI_DV[SM], SPLIT, and salinity) were commonly correlated (BEST: ρ = 0.395) with macroinfaunal patterns (Table 7b). The variables TECI_DV(W), PLAND_SM, SPLIT, temperature, and salinity were weakly correlated (BEST: ρ = 0.282) with the macroinfaunal assemblage at the 750-m scale. However, at this spatial scale, only combinations of five or six variables were correlated with macroinfaunal patterns, suggesting that a parsimonious solution could not be found. The density of S. benedicti was positively correlated with PLAND_SM and negatively correlated with TECI_DV(SM) and SPLIT (Pearson's r; Table 10). Densities of tubificid oligochaetes and capitellid polychaetes were positively correlated with TECI_DV(SM). Furthermore, the densities of a number of taxa were positively (amphipods Apocorophium spp., the amphipod Edotea triloba, and capitellid polychaetes) or negatively (Chironomidae, tubificid oligochaetes, and A. floridus) correlated with salinity. The densities of chironomids, tubificid oligochaetes, S. benedicti, and A. floridus were negatively correlated with SPLIT.

FIGURE 5.

Mean (±SD) CPUE (individuals/sample) of the nekton species contributing to 90% of the cumulative variation among significant groupings identified by agglomerative hierarchical clustering (see Figure 3). Mean dissimilarity between groups is shown in the upper left corner of each plot; mean (±SD) dissimilarity attributed to each species is indicated by the black circles (GSHP = grass shrimp; GMEN = Gulf Menhaden; SPOT = Spot; BSHP = brown shrimp; BLCB = blue crab; WMUL = White Mullet; MOLL = Sailfin Molly).