Sampling

We conducted field studies within several regions of Eastern Russia in the period 2004–2012 (see Fig 1 for the location of the study areas). Sampling on the Russian Federation territory was permitted within the framework of the special grants of the Russian Foundation for Basic Research (RFBR, no. 12-04-00594), the Ministry of Science and Education of Russia (no. № P362), and the scientific program of the Ural Branch of Russian Academy of Sciences (no. 12-P-5-1014). Sampling on the protected sites of the Kunashir Island was permitted by the Directorate of the State Nature Protected Area “Kurilsky” (scientific agreement no. 5/11 of 17.08/2010 between the Institute of Ecological Problems of the North of the Ural Branch of Russian Academy of Sciences and the Kurilsky Nature Reserve).

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Fig 1. Map of location of the field study areas.

1—Kamchatka Peninsula (2012, I. Bolotov, Y. Bespalaya, I. Vikhrev, M. Gofarov), 2—Central Sakhalin (2012, same team), 3—southern Sakhalin (2011–2012, same team & Y. Kolosova, O. Aksenova), 4—Kunashir Island (2011, same team & Y. Kolosova, O. Aksenova), 5—Primorye (2012, same team), 6—Transbaikalia (2004–2011, O.K. Klishko). Data on the studied river sites are presented in S1–S4 Tables.

https://doi.org/10.1371/journal.pone.0122408.g001

For molecular analyses, the tissue samples were collected from 52 live bivalves in 15 localities (see S1 Table). Samples were immediately preserved in 96% ethanol. Dead shells were collected from each field site for morphological investigation; additional shells from some museum collections were studied (see S2–S4 Tables). A total of 554 shells from 44 localities were studied (426 from our collection and 128 museum specimens).

Morphological studies

The total length of the live specimens and dead shells were measured to the nearest 0.1 mm with dial calipers [8]. The comparative morphologies of the shells were analyzed using shape and structure of the pseudo-cardinal and lateral teeth in the valves, shell shape, umbo position and the patterns of distribution of mantle attachment scars on the inner shell surface. We calculated the plane projection squares of the inner surface of the right valve for the estimation of the density of mantle attachment scars. Ten specimens of each species were taken for analysis. The squares were calculated using SHAPE v.1.3 software [42]. The scars were counted by the GNU Image Manipulation Program (GIMP) v.2.8. A normality test of the obtained density values and a one-way ANOVA Welsh’s test (S5 Table) were calculated using STATISTICA v.10 software.

The soft tissue morphologies were analyzed and compared based on the shape and structure of the inhalant siphon, gills and labial palps. Shell and soft tissue photos were taken using a DSLR camera (Canon EOS 7D, Japan) with a 24–70 mm lens (Sigma AF 24–70 mm f/2.8 IF EX DG ASPHERICAL HSM, Japan), and photos of the shell structure details and inhalant siphons were taken using a stereomicroscope (Leica M2C, Germany) and a DSLR camera with a 100 mm macro lens (Canon Macro Lens EF 100 mm 1:2,8 L IS USM, Japan). Descriptions of the shell morphologies were based on an analysis of the collected specimens and museum samples using the original species descriptions [18], [38], [43], [44], [45], [46] and a few other works [23], [24], [47], [48].

We studied the type specimens for the following taxa: Unio (Alasmodonta) dahuricus Middendorff, 1850; Margaritana middendorffi Rosén, 1926 (including specimens of Unio (Alasmodonta) complanatus Middendorff, 1851); and M. sachalinensis Zhadin, 1938 (ZISP). The type series of several comparatory “taxa” were also investigated, including Dahurinaia sujfunensis Moskvicheva, 1973; D. kurilensis Zatravkin & Starobogatov, 1984; D. tiunovae Bogatov & Zatravkin, 1988; D. komarovi Bogatov et al., 2003; D. ussuriensis Bogatov et al., 2003; D. prozorovae Bogatov et al., 2003; D. transbaicalica Klishko, 2008; Kurilinaia kamchatica Bogatov et al., 2003; and K. zatravkini Bogatov et al., 2003 (ZISP). In general, the ZISP systematic catalog has a very complicated numeration because V. V. Bogatov has transferred many specimens from different samples, including true type series, to his newly described comparatory “taxa”.

Species range mapping

The mapping was based on the data of our field studies (see S2–S4 Tables). We determined the precise coordinates of investigated river sites using a geographical positioning system (GPS). Data on other localities were obtained from museum collections and reliable published studies (see S2–S4 Tables). In the cases where a particular map scale did not allow separated precision pointing of closely situated localities, we marked those localities one by one with points and joined them under the one number in the respective table. The arrangement of the localities was digitized and mapped using ESRI ArcGIS 10. The presumed error of determination of the locality coordinates is around ±1–2 km, because published records and collection labels are usually ascribed to an approximate location. The layers of digital maps were added from standard ESRI Data & Maps 10 dataset.

PCR amplification and DNA sequencing

The present study includes new molecular data for 53 Margaritiferidae specimens (S1 Table). Genomic DNA was extracted from the foot or mantle tissues using the Diatom DNA Prep 200 reagents kit (“Laboratoriya Isogen” LLC, Russia) following the manufacturer’s protocol. The standard forward primer LCO 1490 [49] was used to amplify the mitochondrial COI gene from every species. As reverse COI primers, HCO 2198 in a modified version (without the first 6 bases at the 5´ end) was applied to M. dahurica, and C1-N-2329 was used for two other Margaritiferidae species [49], [50]. The newly designed primers 18S-IF (5´-TTCCTTAGATCGTACAATCCTAC-3´) and 18S-IR (5´-TCCTATTCCATTATTCCATGC-3´) were used to amplify the nuclear 18S rRNA gene from every species. The PCR mix contained approximately 200 ng of total cellular DNA, 10 pmol of each primer, 200 μmol of each dNTP, 2.5 μl of PCR buffer (with 10×2 mmol MgCl₂), 0.8 units of Taq DNA polymerase (SibEnzyme Ltd., Novosibirsk, Russia), and H₂O, which was added up to a final volume of 25 μl. Thermocycling included one cycle at 95°C (4 min), followed by 30–35 cycles of 95°C (50 sec), 52°C (50 sec), and 72°C (50 sec) and a final extension at 72°C (5 min). Forward and reverse sequencing was performed on an automatic sequencer (ABI PRISM 3730, Applied Biosystems) using the ABI PRISM BigDye Terminator v. 3.1 reagent kit. The resulting sequences were checked using a sequence alignment editor (BioEdit version 7.2.5, [51], [52]). In addition, 25 sequences were obtained from NCBI’s GenBank, including two sequences of Unio pictorum as outgroup (S6 Table).

Sequence alignment and phylogenetic analyses

The alignment of the COI and 18S sequences was performed using the ClustalW algorithm implemented in MEGA6 [53]. For the phylogenetic analyses, each sequence of the aligned datasets was trimmed, leaving a 654-bp COI and a 681-bp 18S fragment. The sequence datasets were collapsed into haplotypes using an online FASTA sequence toolbox (FaBox 1.41, [54]). The analyses were performed using 24 COI and 8 18S unique haplotypes, including an outgroup. The GTR+I model of sequence evolution was used for the COI gene sequences, and the K2+I model was used for the 18S gene sequences based on the corrected Akaike Information Criterion for small sample sizes (AICc) in MEGA6 [53]. Phylogenetic relationships were reconstructed for each gene separately, based on Bayesian inference as implemented in the software package MrBayes version 3.2.2 [55]. Four Markov chains, one cold and three heated (temperature = 0.1), were run simultaneously for 1,000,000 generations. The trees were sampled every 100^th generation. After completing the Markov Chain Monte Carlo (MCMC) analysis, the first 2,500 trees (25%) were discarded as burn-in, and the majority-rule consensus tree was calculated from the remaining 7,500 trees. The convergence of the MCMC chains to a stationary distribution was checked visually based on the plotted posterior estimates using an MCMC trace analysis tool (Tracer version 1.6, [56]). The effective sample size (ESS) for each parameter that was sampled from the MCMC analysis was observed to be greater than 1000. The combined set of trees showed a smooth frequency plot. The resulting phylogenies were constructed using a tree figure drawing tool (FigTree software version 1.4.0 [57]).

Nomenclatural acts

The electronic edition of this article conforms to the requirements of the amended International Code of Zoological Nomenclature, and hence the new names contained herein are available under that Code from the electronic edition of this article. This published work and the nomenclatural acts it contains have been registered in ZooBank, the online registration system for the ICZN. The ZooBank LSIDs (Life Science Identifiers) can be resolved and the associated information viewed through any standard web browser by appending the LSID to the prefix “http://zoobank.org/”. The LSID for this publication is: urn:lsid:zoobank.org:pub: 46C93315-18E0-45DD-B121-1F225D6E200F. The electronic edition of this work was published in a journal with an ISSN, and has been archived and is available from the following digital repositories: PubMed Central and LOCKSS.

Deposition of examined material

RMBH—Russian Museum of the Biodiversity Hotspots of Institute of Ecological Problems of the North of the Ural Branch of Russian Academy of Science, Arkhangelsk, 163000, Russia.

INREC—Institute of Natural Resources, Ecology and Cryology of the Siberian Branch of Russian Academy of Sciences, Chita, 672000, Russia.

ZISP—Zoological Institute of the Russian Academy of Sciences, St. Petersburg, 199034, Russia.

SMF—Forschungsinstitut und Natur-Museum Senckenberg, Senckenberg-Anlage 25, 6000 Frankfurt-am-Main 1, Germany.

Phylogenetic analyses

The Bayesian analysis of the nuclear 18S rRNA gene revealed that the NW Pacific species M. middendorffi and M. laevis belong to a well-supported monophyletic clade (BPP 1.00) together with the North American species M. marrianae and M. falcata (Fig 2A). Among these species, M. middendorffi is a sister to M. marrianae (BPP 1.00). M. dahurica, M. auricularia and C. monodonta cluster together in an unresolved clade (BPP 0.79), but there is a sister relationship between the two latter species (BPP 0.99). M. dahurica and M. auricularia both have an intra-specific variation of the nuclear 18S rRNA gene with two close haplotypes in each species.

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Fig 2. Bayesian phylogeny of Margaritifera spp. haplotypes.

The scale bar indicates the branch length. Asterisks: Posterior probabilities ≥0.95; other significant support node values are mentioned in the figure. For detailed locality and specimen data for analyzed haplotypes, see the supplementary materials (S1 and S2 Tables). A—The 18S rDNA gene dataset. B—The COI gene dataset.

https://doi.org/10.1371/journal.pone.0122408.g002

The analysis of the mitochondrial COI gene showed that C. monodonta forms a separate clade, which is basal within Margaritiferidae. M. dahurica, M. margaritifera, M. middendorffi, M. laevis and M. falcata cluster together in a well-supported clade (BPP 1.00) (Fig 2B). Among these, our Bayesian inference strongly supports the sister relationships within two pairs of species, namely M. dahurica and M. margaritifera as the first pair (BPP 1.00), and M. middendorffi and M. laevis as the second pair (BPP 0.97). M. falcata shows a closer affinity to M. middendorffi and M. laevis (BPP 0.93). Lastly, the COI phylogeny confirms that M. auricularia and M. marocana are sister taxa (BPP 0.98).

Shell and soft body morphology

The structure of hinge teeth and the shape and relative dimensions of the shell have specific characteristics that are described in detail below in the Taxonomic account of each species. The density of mantle scars has no significant differences (Welch’s test: F = 2.45, df = 16, 38, P = 0.12; (S5 Table)) whereas muscle scar has a high variability among studied taxa.

A general plan of the whole soft body of Margaritifera species is shown in Fig 3. The soft body morphology has more similarity than does the shell morphology among the studied taxa. The mantle color generally is colored cream to cafe au lait with black or brown edges (Fig 3). The gills are cream or light brown. The anterior margin inner gills are slightly longer and wider (higher) than the outer gills (Fig 3). The inner and outer gills are the same size in the middle of the posterior portion. The foot is massive, cream and dark brown distally (Fig 3). The labial palps are half-round, cream to cafe au lait, and convex dorsally. The palps have a smooth external surface and a finely canaliculated inner side. Three apertures are visible in the posterior portion: the supra-anal aperture, the exhalant and the inhalant siphons. This margin of the mantle has dark brown color with a small fold of the exhalant and a large fold of the inhalant siphon (Fig 4). The exhalant and the inhalant siphons are divided by the epithelial fold. The papillae of the inhalant siphon decrease in height in the direction of the ventral margin and are represented by monodactylous outgrowths. The morphological differences between the structures of the inhalant siphon papillae within Margaritifera spp. are presented below in the description of the each species.

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Fig 3. General plan of soft tissue of three Far Eastern margaritiferid species.

A—Margaritifera dahurica (Middendorff, 1850). B—M. laevis (Haas, 1910). C—M. middendorffi (Rosén, 1926). Scale bar—1 cm.

https://doi.org/10.1371/journal.pone.0122408.g003

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Fig 4. Inhalant siphon morphology of three Far Eastern margaritiferid species.

A—Margaritifera dahurica (Middendorff, 1850). B—M. middendorffi (Rosén, 1926). C—M. laevis (Haas, 1910). Scale bar—2 mm.

https://doi.org/10.1371/journal.pone.0122408.g004

Taxonomic account

Family MARGARITIFERIDAE

Margaritifera Schumacher, 1816

Margaritifera dahurica (Middendorff, 1850)—Amurean freshwater pearl mussel

Unio (Alasmodonta) dahuricus Middendorff, 1850: [43]: 109, [44]: 275–276, pl. 26, Figs 3–5.

Unio (Margaritana) dahuricus Middendorff, 1850: [58]: 699–700.

Unio margaritiferus Simpson 1895, partim (ident. err., non Linnaeus, 1758): [59]: 328.

Margaritana dahurica (Middendorff, 1850): [23]: 109–112, Fig 35, [24]: 289, Fig 250.

Margaritifera margaritifera dahurica (Middendorff, 1850): [60]: 120, [61]: 11.

Dahurinaia sujfunensis Moskvicheva, 1973 (comparatory “taxa”): [62]: 1468, Fig 3,e-h.

Dahurinaia sujfunica Moskvicheva, 1973 (inadv. err. in the species description). [62]: 1468.

Dahurinaia tiunovae Bogatov & Zatravkin, 1988 (comparatory “taxa”): [63]: 156–158, Fig 1, a-b.

Margaritinopsis dahurica (Middendorff, 1850): [4]: 42.

Dahurinaia komarovi Bogatov et al., 2003 (comparatory “taxa”): [26]: 45–47, Figs 3a & 3d.

Dahurinaia ussuriensis Bogatov et al., 2003 (comparatory “taxa”): [26]: 47, Figs 3b & 3g.

Dahurinaia prozorovae Bogatov et al., 2003 (comparatory “taxa”): [26]: 48, Figs 3c & 3i.

Dahurinaia transbaicalica Klishko, 2008 (comparatory “taxa”): [28]: 292–296, Figs 1–4, 5a.

Dahurinaia (Kurilinaia) laevis Klishko, 2009 (ident. err., non Haas, 1910): [64]: 237–238, Figs 1–2.

Dahurinaia (Kurilinaia) zatravkini Klishko, 2009 (ident. err., non Bogatov et al., 2003): [64]: 238–239, Fig 3.

Margaritifera dahurica Inoue et al., 2013 (inadv. err.): [65]: Fig 3(a).

Figs 3A, 4A, 5, 6A, 7A, 8 & 9A.

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Fig 5. Shells of Margaritifera dahurica (Middendorff, 1850).

A—Lectotype (ZISP: no. 7a). B—specimen from Komarovka River, Razdolnaya River basin, Primorye. Photos by I.V. Vikhrev. Scale bar—2 cm.

https://doi.org/10.1371/journal.pone.0122408.g005

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Fig 6. Teeth morphology of three Far Eastern margaritiferid species.

A—Margaritifera dahurica (Middendorff, 1850). B—M. middendorffi (Rosén, 1926). C—M. laevis (Haas, 1910). Scale bar—1 cm.

https://doi.org/10.1371/journal.pone.0122408.g006

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Fig 7. Microphotographs of the mantle attachment scars on shells of four Eastern Asian margaritiferid species.

A—Margaritifera dahurica (Middendorff, 1850). B—M. middendorffi (Rosén, 1926). C—M. laevis (Haas, 1910).

https://doi.org/10.1371/journal.pone.0122408.g007

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Fig 8. Range map of Margaritifera dahurica (Middendorff, 1850).

Green circles are representing recent viable populations (observed since 2000), white circles—old records (until 2000). Question mark is indicated an uncertain record from the Langry River [69], [26]. Grey areas are indicated an approximate modern species range (it is shown only for the large river systems). Species locality numbers on the map correspond to numbers in S2 Table.

https://doi.org/10.1371/journal.pone.0122408.g008

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Fig 9. Typical habitats of the Eastern Asian margaritiferid species.

A—Margaritifera dahurica (Middendorff, 1850): the Ilystaya River, Primorsky Kray. B—M. middendorffi (Rosén, 1926): the Nachilova River, Kamchatka. C—M. middendorffi (Rosén, 1926) & M. laevis (Haas, 1910): the Golovnina River, Kunashir Island. Photos by Y.V. Bespalaya, Y.S. Kolosova & I.V. Vikhrev.

https://doi.org/10.1371/journal.pone.0122408.g009

Material examined.

See S1 and S2 Tables.

Margaritifera middendorffi (Rosén, 1926)—Middendorff’s freshwater pearl mussel

Unio (Alasmodonta) complanatus Middendorff, 1851 (ident. err., non Dillwyn, 1817): [44]: 273–274, pl. 27, Figs 1–6.

Unio margaritiferus Simpson 1895, partim (ident. err., non Linnaeus, 1758): [59]: 328.

Margaritana middendorffi Rosén, 1926: [46]: 269–270, [23]: 112–114, Fig 36, [24]: 289, Fig 251.

Margaritana margaritifera middendorffi Rosén 1926: [61]: 12.

Dahurinaia middendorffi (Rosén, 1926): [66]: 16.

Dauhrinaia middendorffii Buyanovsky, 1993 (inadv. err.): [67]: 29.

Margaritinopsis middendorffi (Rosén, 1926): [4: 42].

Kurilinaia kamchatica Bogatov et al., 2003 (comparatory “taxa”): [26]: 48, Figs 4A & 4C.

Kurilinaia zatravkini Bogatov et al., 2003, partim (comparatory “taxa”): [26]: 49–50, Figs 4B & 4F.

Margaritifera laevis Huff et al., 2004 (ident. err., non Haas, 1910): [38]: 381, GenBank acc. no. AY579124.

Figs 3C, 4B, 6B, 7B, 9B, 10 & 11.

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Fig 10. Shells of Margaritifera togakushiensis (Kondo and Kobayashi, 2005) and Margaritifera middendorffi (Rosén, 1926).

A—Holotype of M. togakushiensis [18]: 137, figs 5–8. B—Lectotype of M. middendorffi (ZISP: no. 6). Photo by I. V. Vikhrev. Scale bar—2 cm.

https://doi.org/10.1371/journal.pone.0122408.g010

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Fig 11. Range map of Margaritifera middendorffi (Rosén, 1926) and Margaritifera togakushiensis (Kondo and Kobayashi, 2005).

Circles—M. middendorffi locations, squares—M. togakushiensis locations. Green circles and squares are representing recent viable populations (observed since 2000), white circles—old records (until 2001), yellow squares—records without exact dates. Grey areas indicate approximate modern species ranges (showing only the large river systems). Species locality numbers on the map correspond to numbers in S3 Table.

https://doi.org/10.1371/journal.pone.0122408.g011

Material examined.

See S1 & S3 Tables.

Margaritifera laevis (Haas, 1910)—Japanese freshwater pearl mussel

Margaritana dahurica Kobelt, 1879 (ident. err., non Middendorff, 1850): [71]: 427–428, pl. 13, Figs 1–2.

Unio margaritifer Schrenck, 1867, partim (ident. err., non Linnaeus, 1758): [58]: 700–704.

Unio margaritiferus Simpson, 1895, partim (ident. err., non Linnaeus, 1758): [59]: 303.

Ptychorhynchus laevis Haas, 1910: [45]: 498.

Margaritana sachalinensis Zhadin, 1938: [23]: 114–115, Fig 37, [24]: 289–291, Fig 252.

Margaritifera margaritifera laevis (Haas, 1910): [60]: 120, [61]: 12.

Dahurinaia kurilensis Zatravkin & Starobogatov, 1984 (comparatory “taxa”): [72]: 1789–1790, Figs 11–14, [66]: 21.

Dahurinaia shigini Zatravkin & Bogatov, 1987: (comparatory “taxa”): [66]: 23–24, Fig 4B.

Margaritifera (Dahurinaia) kunahiriensis Habe, 1991 (inadv. err.): [73]: 3.

Dauhrinaia kurilensis Buyanovsky, 1993 (inadv. err.): [67]: 29.

Margaritana sacchariensis Bába, 2000 (inadv. err.): [74]: 133.

Margaritinopsis laevis (Haas, 1910): [4]: 42.

Kurilinaia kurilensis (Zatravkin & Starobogatov): [26]: 42, [27]: 25.

Kurilinaia laevis (Haas, 1910): [26]: 45.

Kurilinaia zatravkini Bogatov et al., 2003: partim (comparatory “taxa”): [26]: 49–50, Figs 4B & 4F.

Figs 3B, 4C, 6C, 7C, 9C, 12 & 13.

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Fig 12. Shells of Margaritifera laevis (Haas, 1910).

A—Sennaya River, Kunashir Island. B—Tym’ River, Sakhalin Island. Photos by I. V. Vikhrev. Scale bar—2 cm.

https://doi.org/10.1371/journal.pone.0122408.g012

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Fig 13. Range map of Margaritifera laevis (Haas, 1910).

Green circles are representing recent viable populations (observed since 2000), white circles—old records (until 2001), yellow circles—records without exact dates. Grey areas indicate the approximate modern species range (showing only the large river systems). Species locality numbers on the map correspond to numbers in S4 Table.

https://doi.org/10.1371/journal.pone.0122408.g013

How many species are distributed in the rivers of the Russian Far East? What are their detailed recent ranges?

Three Margaritifera species inhabit the rivers of the Russian Far East, as discerned from morphological and molecular data: M. dahurica (Middendorff, 1850), M. middendorffi (Rosén, 1926) and M. laevis (Haas, 1910). However, the rivers of Northeastern Russia, where large mainland regions remain unexplored, are still not completely studied; therefore the same species that were previously noted by Smith [4] or additional species, may inhabit the north of the Khabarovsky kray, the Magadan oblast, and the Koryakia and Chukotka districts. These areas are difficult to access and require future studies.

M. dahurica has the largest range among the Eastern Asian species in the genus (see Fig 8). This species is found in almost all of the major tributaries of Amur Basin, an area of approximately two million km², as well as in Razdolnaya Basin and in two separate small rivers. A similar distribution pattern was found in some freshwater fish species, among which approximately 16 were endemic to this area [81]. We found only a single old record of M. dahurica from Sungari River, the largest Chinese tributary of the Amur, and a few occurrences from Mongolia. However, this species is likely widely distributed in part of the Amur River system within the territory of those countries. Dashi-Dorgi [82] reported M. dahurica as one of the most common mussel species in the rivers of Eastern Mongolia. This species is not found in the rivers of the Kurile Islands and the most of Sakhalin Island. Bogatov [69] and Bogatov et al. [26] reported a few specimens from the Langry River, which is situated on the extreme northwest of the Sakhalin Island. It is possible that because this river empties into the Amur Estuary, this river might have belonged to the ancient system of the Paleo-Amur [81]. The range of some Amurean fish species also includes rivers in northwestern Sakhalin Island [83]. Nevertheless, the species identification is in need of revision.

M. middendorffi is also a widespread species that inhabits many rivers across the Northwestern Pacific, from Kunashir Island to the Kamchatka (see Fig 11). Previously, this taxon was considered a local endemic for Kamchatka [4], [23], [24], [25], [31]. It is interesting that M. middendorffi ranges across the Bussol Strait, lying between the Urup and Simushir Islands (Central Kurile), which is the most significant biogeographical boundary within the Kurile Archipelago [84]. M. middendorffi and M. togakushiensis seem to be conspecific because of similar morphological patterns, small shell size (<100 mm) and overlapped ranges. However, the complicated relationships between these poorly known Far Eastern Margaritifera taxa preclude final taxonomic solution, which must be carefully verified using sequences for specimens from the type locality of M. togakushiensis (type series or newly collected topotypes).

The number of M. middendorffi localities increases northward. For example, on Kunashir Island, only three populations were found, but this species successfully inhabits the cold subarctic rivers of the Kamchatka and Northern Kuriles. Using data from the literature, this species ranges only in the rivers of the Western Kamchatka, Okhotsk Sea Basin [4], [8], [25]. This phenomenon is explained by the fact that these rivers in the Pleistocene were tributaries of the Paleo-Penzhina River system [25]. Therefore, the report by Eyerdam [85] of an occurrence of Margaritifera shell in the downstream part of the river Kamchatka (Pacific drainage) was questioned [25]. However, we found a reliable sample of shells from the Paratunka River of Eastern Kamchatka, which flows into the Pacific Ocean (see S3 Table, loc. no. 8). These data indicate that the Margaritifera record from the Kamchatka River is most likely true and that this species has a wider range on the Kamchatka Peninsula, but a large part of the region is difficult to access and is still poorly investigated.

From our data, the range of M. laevis is significantly narrower than the distribution of the previous species (see Fig 13). This species has a more southerly distribution, and has not been found north of central Sakhalin. However, the host fish Oncorhynchus masu is much more widespread northward up to Kamchatka Peninsula. Most of the known localities of M. laevis are situated on the Honshu Island, and their number is linearly reduced to the north. A few fish species have a distribution resembling this, including the Sakhalin Taimen (Hucho perryi (Brevoort, 1856)) [83].

What are the phylogenetic relationships of the Margaritiferidae from the Russian Far East?

Based on the nuclear 18S rRNA gene, M. laevis and M. middendorffi cluster together with two North American species, M. falcata and M. marrianae. These results support the hypothesis of an ancient Beringian exchange between the freshwater mussel faunas of Northeastern Asia and North America [86]. These data also correspond to results of molecular studies of cyprinid fishes of Eurasia and North America, where the Far Eastern phoxinins have dispersed from North America to the Far East across the Beringia land bridge during the Late Cretaceous or Early Paleocene [87]. It is interesting, that recent populations of M. marrianae are isolated in a few tributaries of the Alabama and the Conecuh (Escambia) rivers [4], [88]. It is known that North American Margaritiferidae are not limited strictly to drainages of the Great Basin and Pacific Coast but also occur in parts of the upper Missouri drainage, where they are represented by one species M. falcata [86].

According to the COI gene sequences, we found a similar “Beringian” clade, formed of M. laevis, M. middendorffi and M. falcata. Unfortunately, the position of M. marrianae based on the COI phylogeny remains uncertain, because there are only three very short COI sequences for this species in NCBI’s Genbank, which are unsuitable for phylogenetic assessment. However, the minimal COI distances were found between M. laevis and two other species, M. marrianae (4.7%) and M. middendorffi (5.5%), which is in agreement with results, obtained from 18S sequences. M. dahurica is the sister species of M. margaritifera, which is distributed across Western Europe and in the river basins of the Atlantic coast of North America [4], [8], [10], [38], [65]. Similar patterns have been found for several freshwater fishes that have closely related representatives from Amur Basin and European rivers, with a huge gap in the Siberian Plain [89], [90], [91], [92], [93]. Most Eastern Asian species have very low intraspecific COI divergence, particularly M. dahurica and M. middendorffi. For each of these species, only two COI haplotypes were observed. For twelve examined M. margaritifera populations, a lack of differentiation was observed in the COI and 16S genes, and these populations may be considered as a metapopulation [9]. A survey of five populations of North American species Margaritifera hembeli (Conrad, 1838) showed extensive allozyme monomorphism [94]. These authors mentioned that low genetic diversity appears to be characteristic of Margaritiferidae, as an ANOVA indicated that mussels of the family Margaritiferidae (only M. auricularia, M. margaritifera and M. hembeli were tested) have a significantly lower heterozygosity level than do mussels of the family Unionidae. These authors assumed that, although bottlenecks are known to cause low genetic variability, Margaritiferidae might exhibit metapopulation structure with extinction/re-colonization dynamics leading to low genetic variability. Meanwhile, both COI and microsatellite loci have substantially high levels of genetic variation between C. monodonta populations that are, most likely, associated with the Pleistocene history of the Mississippi Basin [65]. However, the genetic diversity within each of the populations was low, indicating high gene flow after isolation during the last glacial period.

Is it possible to reliably identify the Far Eastern species using morphological patterns?

In this study, we analyzed the applicability of specific shell features that were indicated in previous studies for reliable species identification. Three pearl mussel species were identified using a complex of morphology patterns and molecular data. The development and expression of hinge teeth, the shape and the relative dimensions of the shell, the mantle attachment scars, and the muscle scar shape are the most used conchological key features [4], [10], [18], [23], [24], [34], [38], [47], [43], [44], [45], [46], [95], [96], [97], [98], [99].

The dimensions of the shell are the least reliable morphological traits in Unionoida, upon which to base a description [4], [32] due to high variability and the dependence on environmental gradients [4], [33], [34], [100], [101]. However, sometimes, the shell dimensions and shape are useful for distinguishing several Margaritiferidae species. For example, M. middendorffi has a small shell length (<100 mm) (Fig 10), and M. dahurica has the largest shell length (up to 196.5 mm) among the Far Eastern pearl mussels (Fig 5).

According to Kondo & Kobayashi [18], the adductor muscle scar shape is one of the key features for M. togakushiensis identification. However, according to our data, this feature has a high variability and cannot be used for species identification among studied taxa. In the review of recent Margaritiferidae by Smith [4], this feature was also not mentioned as a diagnostic. The adductor muscle scar shape was not used in the morphological descriptions of other unionoid species [10], [86], [95], [96], [97].

The structure and expression of pseudo-cardinal and lateral teeth have a low interspecific variability (Fig 6) and could be reliable characteristics for identification of Margaritiferidae species [4]. The specific characteristics of the structure of the hinge plate in the right valve of M. middendorffi, namely the arranged deep groove passing through a thickened fold, are typical only for this species and are present in adults, as well as juvenile individuals. Zhadin [23] indicated this key feature, but it was not mentioned within hinge descriptions in later studies of the species [86]. The reduced anterior pseudo-cardinal tooth of the left valve is the basic distinctive feature for M. dahurica that has been noted in numerous studies [4], [23], [24], [28], [43], [98]. The lateral teeth of M. laevis are present as thin rudimental lamellae in both of the valves [4], [18], [23], [24]. In all other species of the Far Eastern pearl mussels, lateral teeth are absent or are present as weakly pronounced rudimentary lamellae.

According to Smith [4], [99], the mantle attachment scars on the inner surface of the valves are formed by modified epithelial cells, and specific patterns of the distribution and density of the scars can be identified among taxa. Therefore, the presence of mantle-attachment scars in M. marocana was sufficient to separate M. marocana and M. auricularia [10]. However, our data do not confirm significance of this character for species identification within Margaritiferidae. Fig 7 shows that the mantle scar shape has a high intra-specific variability that overlaps with the differences between taxa. Based on visual assessments, it seems that M. middendorffi has weaker and less frequent scars than M. dahurica or M. laevis.

In addition to shell morphology, the soft body details were also analyzed. The structure of inhalant siphon papillae is often used for species identification [28], [34], [95], [96], [97]. The Far Eastern pearl mussels have differences in this organ. The length of papillae, their frequency, the characteristics of papillae outgrowth, and the position with respect to the mantle edge can be patterns for species identification. Our data confirm the previous description of the M. dahurica inhalant siphon [28], [34], whose papillae are large and have variable widths. The papillae in the siphon of M. dahurica are branched over the mantle edges, in contrast to the papillae of M. laevis and M. middendorffi. In addition, the papillae of M. laevis are more branched but in other respects, their structure is similar to that of the papillae of M. dahurica. Similarly to the mantle attachment scar pattern, the structure of the inhalant siphon of M. middendorffi is the most distinct; its papillae are less branched and thinner. The structure of the gills and labial palps have no specific features and, despite some differences, could not be used to identify Margaritifera spp.