Bioblitz survey

A bioblitz survey was conducted from 16 to 18 May 2007 by a team of 12 taxonomic specialists and volunteers. Adult caddisflies were collected with UV light traps and sweep nets. Larvae and pupae were collected with kick nets and by hand. Species or morphospecies were sorted into separate vials to minimize the chance of cross contamination. As many specimens as possible were morphologically identified to species in a 2-d session after collection. When discrepancies between these morphological assignments and COI assignments were detected, specimens were re-examined by specialists.

Trichoptera samples from other regions

Barcode records from specimens of Trichoptera species known from the GSMNP, but obtained through the TBoL effort, most of which were collected from other localities in North America, were used to create a barcode library with coverage for as many species as possible. Samples from much of the eastern US and Canada were included in our analyses (Fig. 1), but samples from other regions, e.g., Ozarks, Gulf Coastal Plain, Atlantic Coastal Plain, Wichita Mountains, Great Plains, Cumberland Plateau, that might potentially have high divergence levels were unavailable to us or were represented by few specimens. Samples from these regions should be investigated further. Representative sequences for caddisfly species known from the GSMNP were selected from projects in the global TBoL campaign. Caddisfly species from the TBoL library were included based on the most recent park checklist (Parker et al. 2007), which was based on examination of >130,000 specimens and records. Representatives of each haplotype cluster showing >2% divergence from its nearest neighbors were selected to represent each taxon. Our goal was to reflect the COI sequence diversity present within each species across its distribution. If a particular COI haplotype cluster was represented by multiple individuals, a single representative from each state or province was included in the analysis. Whenever available, full-length sequences derived from male specimens were selected.

Figure 1

Distribution map for 1638 caddisfly samples analyzed in our study.

Species identification via DNA barcoding

A significant fraction of the caddisflies collected in the 2007 bioblitz consisted of immature individuals or females, most of which presented a challenge for species-level identification. In such cases, DNA barcodes were used for species identification. We used a strict consensus criterion for these identifications—each specimen was identified only if its sequence nested within a sequence cluster delimited by positively identified specimens of that species (Zhou et al. 2007).

DNA protocols

All specimens were stored in 95% ethanol or pinned. Standard DNA-barcoding protocols (Ivanova et al. 2006, deWaard et al. 2008) were conducted at the Canadian Centre for DNA Barcoding, University of Guelph. In most cases, a single leg was removed from each individual and used for DNA extraction. A nondestructive extraction protocol was followed for some microcaddisflies (e.g., Hydroptilidae). In this protocol, the entire specimen was emerged in lysis buffer and was retained after extraction. The full-length barcode region of the COI gene was amplified with 2 sets of routine primers: LepF1 (5′-ATTCAACCAATCATAAAGATATTGG-3′)/LepR1 (5′-TAAACTTCTGGATGTCCAAAAAATCA-3′) (Hebert et al. 2004), and LCO1490 (5′-GGTCAACAAATCATAAAGATATTGG-3′)/HCO2198 (5′-TAAACTTCAGGGTGACCAAAAAATCA-3′) (Folmer et al. 1994). PCR products were visualized, cycle sequenced, purified, and bidirectionally sequenced on ABI 3730XL sequencers (Applied Biosystems, Foster City, California).

Data depository and output

All relevant voucher information, DNA sequences, and trace files are publicly accessible in projects GSMNP caddisflies (SMCAD) and GSMNP caddisflies additional samples (SMTRI), in the Barcode of Life Data Systems (BOLD systems;  http://www.boldsystems.org). All COI sequences have also been deposited in GenBank (accession numbers are in Appendix 1; available online from:  http://dx.doi.org/10.1899/10-010.1.s1 (10.1899_10-010.1.s1.xls)), except for 13 Churchill samples that were published in earlier papers (Zhou et al. 2009, 2010).

Sequence analysis and tree construction

Neighbor-Joining (NJ) trees were built for both GSMNP samples and combined samples using a Kimura-2-Parameter (K2P) distance model, using tree-construction tools on BOLD. The Newick tree files were subsequently imported into the web-based visualization tool, interactive Tree of Life (iTOL;  http://itol.embl.de/; Letunic and Bork 2007). The terminal nodes in the tree of samples from the GSMNP were collapsed for each morphological species, and the total branch lengths to the closest and the farthest terminal were used as sides of the triangle (Fig. 2). The combined NJ tree was presented in circular format. All terminal clades with average distance to terminals <2% were collapsed, but the overall tree topology was not changed (Fig. 3). Eleven monophyletic clades were recognized and pruned from the combined tree and presented as 9 subtrees (Figs 4–12). A NJ tree with detailed sample identification code (BOLD Sample ID), distribution, and sex information also was built with the BOLD tree construction function with K2P distances (Appendix 2; available online from:  http://dx.doi.org/10.1899/10-010.1.s2 (10.1899_10-010.1.s2.pdf)). Intra- and interspecific distances were calculated in BOLD with the Nearest Neighbor Summary analytical tool and a K2P distance parameter for all sequences >350 base pairs (bp).

Figure 2

A and B.—Neighbor-Joining tree of 80 Trichoptera species collected in the Great Smoky Mountains National Park during the 2007 bioblitz. Tree nodes are collapsed for each morphological species, where the total branch lengths to the closest and the farthest terminal are used as sides of the triangle. Species possessing ≥2% maximum intraspecific divergence are highlighted by thickened branches. Numbers in brackets next to species names represent number of individuals analyzed for the corresponding species.

Figure 2

Continued.

Figure 3

Neighbor-Joining tree of combined Trichoptera data set including 212 species. All terminal clades with average distance <2% are collapsed, but the overall tree topology is not changed. Each collapsed clade may contain many individuals, as shown in the inset figure. Eleven monophyletic groups (numbered 1–11 in this figure) are presented in subsequent figures (Figs 4–12).

DNA-barcode reference library

The GSMNP checklist was updated to ensure correspondence with current Trichoptera nomenclature (Morse 2010). Records from Parker et al. (2007) (with updates made by the authors of the present paper) and new records from our study were included in the updated checklist (Table 1). A total of 234 species, including 2 undescribed species by Parker et al. (2007) and 3 that have only provisional identifications, are now known from GSMNP. This total includes 2 species (Homoplectra flinti Weaver and Hydroptila coweetensis Huryn) that were collected for the first time in GSMNP during our bioblitz. COI sequences were available from the TBoL global library for 209 of these species (89%). Eighty species were collected during the bioblitz. Only 3 of these species were not already in the TBoL global library. Our coverage was 212 species (91% of the fauna), of which 208 (89%) were represented by barcode sequences >500 bp. Figure 1 shows the distribution of the 1638 caddisfly specimens examined in our study.

Table 1

Trichoptera of Great Smoky Mountains National Park (GSMNP) and barcode distances. Divergence values were calculated for all sequences >350 base pairs, using the Nearest Neighbor Summary tool provided in the Barcode of Life Data System (BOLD). Global library  =  Trichoptera Barcode of Life database, bioblitz  =  short-term, high-intensity sampling event, N  =  number of sequences in the database, NN  =  nearest neighbor, ISD  =  intraspecific distance, ID  =  identifier, N/A  =  not applicable. AB  =  Alberta, AL  =  Alabama, AR  =  Arkansas, AZ  =  Arizona, CO  =  Colorado, FL  =  Florida, GA  =  Georgia, IA  =  Iowa, IL  =  Illinois, IN  =  Indiana, KY  =  Kentucky, LA  =  Louisiana, MA  =  Massachusetts, MB  =  Manitoba, MD  =  Maryland, ME  =  Maine, MI  =  Michigan, MN  =  Minnesota, MT  =  Montana, NB  =  New Brunswick, NC  =  North Carolina, NJ  =  New Jersey, NL  =  Newfoundland and Labrador, NS  =  Nova Scotia, NV  =  Nevada, NY  =  New York, OH  =  Ohio, OK  =  Oklahoma, ON  =  Ontario, OR  =  Oregon, PA  =  Pennsylvania, PE  =  Prince Edward Island, QC  =  Quebec City, SC  =  South Carolina, SD  =  South Dakota, SK  =  Saskatchewan, TN  =  Tennessee, TX  =  Texas, VA  =  Virginia, WI  =  Wisconsin, WV  =  West Virginia, WY  =  Wyoming, VT  =  Vermont, ME  =  Maine, WA  =  Washington.

Barcode divergences in GSMNP Trichoptera

COI sequences were obtained from 645 of the caddisflies collected in the bioblitz. All 80 species in this collection exhibited reciprocal monophyly in the NJ tree, and no species shared barcodes (Fig. 2). COI divergences within species were, on average, much lower than those between nearest neighbors (mean intraspecific distance  =  0.7%, maximum intraspecific distance  =  1.4%; Table 1). Eleven species showed maximum intraspecific divergence >2% (Fig. 2, highlighted by thickened branches), a threshold found useful in species discrimination in many insect groups (e.g., Hebert et al. 2003, 2004, Ball et al. 2005), whereas 3 species had mean intraspecific divergence >2%. Exceptionally large intraspecific variation was observed in 2 species—individuals of Dolophilodes distincta (Walker) showed as much as 14.0% divergence and those of Polycentropus cinereus Hagen reached 9.9% divergence. Levels of within-species divergence were not correlated with the number of individuals analyzed for a species. In contrast to these cases of deep intraspecific variation, 1 species pair, Agapetus walkeri (Betten and Mosely) and A. tomus Ross, showed only 3.1% divergence, a result suggesting their recent speciation.

Barcode divergences in combined samples

Barcode coverage for the GSMNP fauna was extended by including 993 records from specimens collected at other localities to produce a data set with 1638 sequences (97% were >500 bp in length), representing 212 species (Fig. 1). The expansion of geographic range did not lead to a large increase in COI divergence for all species. For example, the maximum intraspecific divergence for Hydropsyche sparna Ross remained as low as 1.5% among samples collected as far as 2600 km apart. However, maximum intraspecific sequence divergences increased in many taxa, a result that reflected geographic variation. Between-species differences decreased because of greater taxon coverage, especially the addition of species that were closely related to those already in the data set. The barcode gap decreased, but intraspecific divergences were still much lower than interspecific divergences. Mean intraspecific distance was 1.7% (range: 0–10.2%), mean maximum intraspecific distance was 3.1% (range: 0–10.6%), and average distance to the nearest neighbor was 10.1% (range: 0–23.4%). The rise in intraspecific variation reflected the fact that some species showed very high divergence across their distribution. Half of the species represented by multiple individuals showed maximum intraspecific divergence ≥2% (Figs 4–12, Table 1), whereas 34% had a mean intraspecific divergence ≥2%. However, most of the overall rise in intraspecific variation arose from a few species with deep maximum within-species divergence. For instance, ∼11% of the species showed ≥8% maximum within-species divergences (Table 1, highlighted in grey blocks with a solid line in Figs 4–7, 9–10, 12). The 8% value was not selected to imply a generic barcode gap for the caddisflies examined in our study nor to suggest that taxa with <8% divergences should not be investigated. This arbitrary divergence was used simply to point out where large intraspecific divergences were observed in the focal taxa. Most of these taxa have not been thoroughly investigated via integrated morphological and molecular evidence, some are almost certainly species complexes, and others include multiple lineages with clear morphological differences. Despite cases of large sequence variation within species, most species (91%) defined by morphology were represented by a monophyletic assemblage of haplotypes (Figs 4–12).

Figure 4

Neighbor-Joining tree for clade 1. This clade includes members of the family Philopotamidae. Terminal leafs are collapsed based on morphological species or distinct cytochrome c oxidase subunit I (COI) haplogroups. Number of individuals and distributions (see Table 1 for postal abbreviation for states or provinces) are provided in brackets next to corresponding species. Species possessing ≥2% maximum intraspecific divergence are highlighted by thickened braches. Maximum intraspecific divergence values are noted on the leading branches. Taxa included in a grey block with a solid line include species for which the barcode data resolved current species taxonomy, but for which intraspecific variation was ≥8%. In these highly divergent species, haplotypes obtained from the 2007 Great Smoky Mountains National Park (GSMNP) bioblitz are noted with *.

Figure 5

Neighbor-Joining tree for clade 2. This clade includes members of the family Polycentropodidae. Species groups included in dotted lines represent those for which barcode data failed to resolve monophyletic taxa. Species groups not included in a grey block are taxa for which the barcode data failed to resolve species identity. Species groups in a grey block were not monophyletic but could be identified from barcode sequences. Maximum divergence values ≥2% are noted for each taxon showing paraphyly included in the dotted lines. Other figure annotations follow those of Fig. 4.

Figure 6

Neighbor-Joining tree for clade 3. This clade includes members of the family Hydropsychidae. Annotations follow those of Figs 4 and 5.

Figure 7

Neighbor-Joining tree for clade 5. This clade includes members of the family Rhyacophilidae. Annotations follow those of Figs 4 and 5.

Figure 8

A and B.—Neighbor-Joining (NJ) tree for clades 4 and 6. Clade 4 is pruned from the NJ tree in Fig. 3 and reattached to clade 6. This tree includes members of families Hydroptilidae, Calamoceratidae (in part), Glossosomatidae, and Ptilocolepidae. Annotations follow those of Figs 4 and 5.

Figure 8

Continued.

Figure 9

Neighbor-Joining tree for clade 7. This clade includes members of the family Leptoceridae. Annotations follow those of Figs 4 and 5.

Figure 10

Neighbor-Joining tree for clade 8. This clade includes members of families Odontoceridae, Calamoceratidae (in part), Molannidae, Sericostomatidae, and Helicopsychidae. Annotations follow those of Figs 4 and 5.

Figure 11

Neighbor-Joining tree for clades 9 and 10. This clade includes members of families Lepidostomatidae, Phryganeidae, and Brachycentridae. Annotations follow those of Figs 4 and 5.

Figure 12

Neighbor-Joining tree for clade 11. This clade includes members of families Goeridae, Uenoidae, Apataniidae, and Limnephilidae. Annotations follow those of Figs 4 and 5.

The exceptions are highlighted with transparent (Category 1 in Appendix 3; available online from:  http://dx.doi.org/10.1899/10-010.1.s3 (10.1899_10-010.1.s3.doc)) or grey (Category 2 in Appendix 3) blocks with a dotted line, representing instances where the barcode data could not definitively identify species or where barcode data could identify species, but species were not monophyletic, respectively. In Category 1, 14 species belonging to 6 species complexes either shared barcodes or formed clusters with representatives from ≥1 taxon (Figs 5, 6, 9–11, highlighted by transparent blocks with a dotted line). These cases included 5 pairs of species—Polycentropus colei Ross/Polycentropus rickeri Yamamoto (Fig. 5), Ceraclea nepha (Ross)/Ceraclea tarsipunctata (Vorhies) (Fig. 9), Triaenodes tardus Milne/Triaenodes marginatus Sibley (Fig. 9), Psilotreta rossi Wallace/Psilotreta rufa (Hagen) (Fig. 10), and Lepidostoma pictile (Banks)/Lepidostoma modestum (Banks) (Fig. 11). In addition, they included 1 group of 4 species—Cheumatopsyche campyla Ross/Cheumatopsyche speciosa (Banks)/Cheumatopsyche pasella Ross/Cheumatopsyche ela Denning (Fig. 6). In Category 2, 6 species each had multiple haplotype groups deeply diverging from each other and a closely related species nested within its species boundary but not overlapping with any of its haplotype groups: Nyctiophylax affinis (Banks), Diplectrona modesta Banks, Hydropsyche rossi Flint, Voshell, and Parker, Ceraclea flava (Banks), Oecetis inconspicua (Walker), and Psilotreta labida Ross. The potential reasons for these unusual barcode clustering patterns are briefly addressed in the discussion. Taxonomic changes have not been proposed in our paper because comprehensive taxonomic revision is not available. However, provisional opinions on the relevant issues are provided in Appendix 3.

Complexities when using DNA barcoding

Our study has further validated the effectiveness of DNA barcoding for the identification of Trichoptera within the GSMNP, but it has revealed some complexities. These complexities fell into 3 categories: 1) barcode data could not be used to distinguish some closely related species; 2) barcode data could be used to identify species, but species were not monophyletic; 3) barcode sequences recovered monophyletic taxa, but the genetic distances were very high. A comprehensive taxonomic revision is beyond the scope of our paper, but provisional opinions and observations made during the course of our study are provided in Appendix 3. Here, we discuss the implications of the present results in relation to past concerns expressed regarding the effectiveness of DNA barcoding.

Taxonomy and barcodes

Critics of DNA barcoding have based their concerns largely on theoretical objections (e.g., Rubinoff et al. 2006), or on failure to gain perfect resolution in a particular taxonomic group (Whitworth et al. 2007, Wiemers and Fiedler 2007, Alexander et al. 2009). Theoretical objections ultimately must account for actual data. Our study provides yet another example of the effectiveness of DNA barcoding as a tool for species identification, so it further weakens theoretical objections. Case studies have revealed that barcoding is not a perfect technology, but neither is any other approach for species recognition. Nevertheless, some generalized conclusions of barcoding failure are often made based on case studies in which just a few species within a particular group have been examined (e.g., Whitworth et al. 2007) and on the presumption that existing taxonomic systems are static and lack the capacity to evolve or to embrace new evidence (e.g., Alexander et al. 2009). Our results suggest that it is a great oversimplification to conclude that all cases of incomplete correspondence between current taxonomic assignments and barcode clusters reflect a flaw in barcode methods. For example, the heterogeneity in COI divergence values found within and among many caddisfly “species” in our study could be interpreted as the absence of a barcoding gap or the lack of a limit on intraspecific sequence variation in caddisflies. However, a critical examination of species with such properties reveals the strong concordance of anomalous results with the need for a better taxonomic investigation in the relevant taxa. We do not claim that barcode-based identifications are superior to morphological assignments when conflicts arise. However, we do argue that every exceptional case (e.g., nonmonophyletic species or taxa showing >2% intraspecific divergence following a more conservative standard for the caddisflies) should be examined in detail to understand the biological origins and implications of the divergent pattern. From the taxonomic point of view, species hypotheses proposed by morphology have been and always will be subject to nomenclatural revision when new evidence or analytical methods become available. We anticipate that some current barcoding failures will actually prove to be successes when taxonomists use barcode data to conduct much needed revisions. In fact, some recent nomenclatural changes have been supported by the barcode analyses in our study, e.g., the reinstatement of Cheumatopsyche enigma Ross, Morse, and Gordon as a full species instead of a subspecies of C. harwoodi Denning and Gordon (Flint et al. 2004). On the other hand, some past synonymization may have to be revised, e.g., the treatment of Drusinus uniformis Betten as a subspecies of Pseudostenophylax sparsus (Banks) (Schmid 1991). These 2 taxa can be readily differentiated based on color patterns of the forewings and genitalic structures and by barcodes, as revealed in our study (Fig. 12). In fact, they have been treated as separate species in practice by many taxonomists despite Schmid's (1991) revision. Thus, DNA barcodes (i.e., standardized mitochondrial COI sequences) can be used for identification of caddisflies and to provide a deeper understanding of species boundaries and of biodiversity at large.

Conclusion

DNA barcoding is a robust tool for identifying the Trichoptera species that occur within the GSMNP. The barcode analyses have drawn attention to various interesting issues in caddisfly biodiversity, ranging from the need for a re-evaluation of taxa in a number of species groups to the necessity of an appropriate interpretation of barcode analyses and its implications for understanding species diversity. Last, both local bioblitz surveys and global DNA-barcoding projects have played critical roles in assembling a barcode library for a local site. The strategy for barcode library construction developed in our study should serve as a model for similar efforts in other geographic regions.