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. 2023 Jul 19;16:240. doi: 10.1186/s13071-023-05850-w

Morphological and DNA-based description of Trichophoromyia peixotoi n. sp. (Diptera: Psychodidae), a new sand fly species from the Brazilian Amazon

Bruno Leite Rodrigues 1,, Israel de Souza Pinto 2, Eunice Aparecida Bianchi Galati 1,3
PMCID: PMC10354958  PMID: 37468935

Abstract

Background

Phlebotomine sand flies of the genus Trichophoromyia Barretto, 1962 are of great relevance to public health as vectors of Leishmania protozoans. A new phlebotomine species named Trichophoromyia peixotoi n. sp. is here described based on both male morphology and COI DNA barcodes.

Methods

The sand fly specimens were collected in the Parque Nacional da Amazônia (PNA), situated in the municipality of Itaituba, state of Pará, Brazil. Morphological description was done based on 10 male specimens. Five specimens were DNA barcoded for the COI gene.

Results

The morphological and molecular analyses allowed the delimitation of this new species from others of Trichophoromyia. Trichophoromyia peixotoi n. sp. is closely related to other species with aedeagal ducts > 4 times the length of the sperm pump, from which it may be distinguished by the gonocoxite bristles and paramere shape.

Conclusions

The description of T. peixotoi n. sp. brings the number of species of Trichophoromyia to 45, including 24 for Brazil. The integrative taxonomy effort through the analysis of COI barcodes proved to be effective in the species delimitation of some Trichophoromyia spp.

Graphical Abstract

graphic file with name 13071_2023_5850_Figa_HTML.jpg

Keywords: Phlebotominae, Integrative taxonomy, DNA barcoding, COI

Background

Phlebotomine sand flies are important vectors of several pathogens of relevance for public health, including viruses, bacteria, and Leishmania protozoans [1]. The Phlebotominae subfamily comprises about 1060 species distributed worldwide [2], which are sorted into several tribes, subtribes, and genera according to Galati [3, 4]. One of the Neotropical subtribes—Psychodopygina Galati, 2003—is subdivided into seven genera, most of them with vector species of cutaneous leishmaniasis agents, including Trichophoromyia Barretto, 1962 [5].

The genus Trichophoromyia has been gaining evidence for the control of leishmaniasis, as some of its species have been incriminated as biological vectors and others are suspected vectors [6]. Currently, there are 44 nominal species described, 23 of them occurring in Brazil [2, 7]. Most of its species occur in the Amazon biome, including forest fragments or anthropized environments [7]. These sand flies are usually of medium size and brown or dark brown in colour; both sexes have Newstead’s sensilla on the second palpal segment, while males present terminalia equivalent to or longer than the length of the thorax, and females with spermathecae presenting 25 or more rings, the apical one frequently three or more times longer than the preapical [8].

Most of the taxonomic information on this genus is based on the adult male morphology, as only one species has its immature forms described [9], and few females can be truly distinguished [8]. Therefore, the Trichophoromyia taxonomy has many gaps and seems to be tricky. Thus, the use of integrative taxonomy can help by providing new lines of evidence for the delimitation, description of new species, and classification proposals [10]. The sequencing and analysis of molecular markers is one of these additional approaches, and can help to improve the taxonomy and systematics of sand flies [11, 12]. For Neotropical sand flies, DNA barcoding fragments of the cytochrome c oxidase subunit I (COI) gene [13] supported the description of females of Psathyromyia pradobarrientosi (Le Pont, Matias, Martinez & Dujardin, 2004) [14], but it had not been used until then to describe new sand fly taxa in the Americas. Recently, COI barcodes have been proposed as diagnoses for descriptions of new species, which might somewhat speed up the laborious process of describing new taxa [15]. However, this type of approach has proven insufficient and unstable for describing new species [16, 17], although it can be used as an additional line of evidence to support the description of new taxa.

A new sand fly species—Trichophoromyia peixotoi n. sp.—collected in the Parque Nacional da Amazônia (PNA), located in the Brazilian Amazon, is herein described using morphology and COI DNA sequences.

Methods

Sample collection

Sand flies were collected between 7 July and 11 November 2022 in the PNA, situated in the municipality of Itaituba, state of Pará, Brazil, bordering the state of Amazonas, with a hot and humid equatorial climate. Its predominant vegetation is the dense ombrophilous forest, typical of the Amazon biome, with numerous trees that can reach 40 m in height. In the boundaries of the eastern region of the PNA—where the sand fly collections were carried out—there is a significant increase in phytophysiognomic characteristics of anthropic action, such as pasture and secondary vegetation with palm trees [18]. Sand fly collections were performed under authorization for activities with scientific purpose of the Brazilian Sistema de Autorização e Informação em Biodiversidade (SISBIO) for the capture of zoological material (no. 81991-2).

For sample collection, Centers for Disease Control and Prevention (CDC)-type light traps were installed in two different vertical strata, 1 m above the ground, and in the canopy of trees, about 15 m in height. The traps were installed within the forest, close to the Trans-Amazonian Highway (BR 230), and operated overnight from 7 pm to 7 am of the next day. The three collection sites were set near the Tracoá and Uruá bases of the PNA: Trilha da Capelinha 01 (4°37′21.8″S; 56°23′22.3″W), Trilha da Capelinha 02 (4°36′41.5″S; 56°23′25.3″W), and Trilha de Monitoramento 03 (4°28′22.0″S; 56°17′12.1″W). The collections of sites 01 and 02 were done at the ground level, while those of site 03 were from the canopy.

Morphology

The description of this new species is based on 10 male specimens. Seven of them had the legs dissected and stored in microtubes for later DNA extraction, while the rest of the body was used for morphological description. Sand flies were clarified according to Forattini [19], and then slide-mounted in Enecê resin [20] or Canada balsam.

The terminology of morphological characters follows Galati et al. [21]. The structures were measured using the Zen version 4.7 program, with images taken with an Axiocam 105 color (Carl Zeiss MicroImaging GmbH, Jena, Germany) coupled to an optical microscope. All drawings were made in pencil using an Olympus camera lucida attached to a microscope.

All measurements are given in micrometers for the holotype, and the mean or range of countable characters, the standard deviation, and the number of analysed specimens for each structure are included in brackets.

Amplification and data analysis of COI DNA barcoding

Total DNA was extracted from legs. For this, plastic pistils were used to macerate the legs in a 1.5 ml microtube with Digsol Buffer (ethylenediaminetetraacetic acid [EDTA] 20 mM, Tris–HCl 50 mM, NaCl 117 mM; sodium dodecyl sulfate [SDS] 1%), and 2 μl of proteinase K at 20 mg/ml. After incubation (55 °C overnight), ammonium acetate (4 M) was added to each tube, vortexed, and then centrifuged for 15 min at 14,000 rpm and 10 °C. The supernatants were washed using absolute and 70°GL alcohol. After drying, 20 μl of TE buffer was added to dissolve the pellet, which was kept at −20 °C until use.

For DNA amplification, the PCR Master Mix (Invitrogen, Thermo Scientific™) was used, following the manufacturer’s instructions, and the primers LCO1490 (5′-GGTCAACAAATCATAAAGATATTGG-3′) and HCO2198 (5′-TAAACTTCAGGGTGACCAAAAAATCA-3′) [22] under the following conditions: an initial denaturation of 95 °C for 2 min; followed by 35 cycles of 95 °C for 1 min, 54 °C for 1 min and 72 °C for 1 min 30 s; and a final extension of 72 °C for 10 min. Samples were checked by electrophoresis using 1% agarose gels stained with GelRed (Biotium, Inc.), and all positive reactions that gave bands of the expected molecular size were sent to ACTGene Análises Moleculares (Brazil) for purification and direct sequencing of the PCR products in both directions (forward and reverse).

Initially, SeqTrace version 0.9.0 (http://seqtrace.googlecode.com/, [23]) was used to manually check the electropherograms, remove primer sequences, and assemble consensus sequences, which were submitted to the National Center for Biotechnology Information (NCBI) GenBank [24], and have been assigned accession numbers OQ843038–OQ843042.

By way of comparison, we constructed a dataset with other publicly available Trichophoromyia species. The sequence alignment was done using MUSCLE [25] implemented in MEGA v7 software [26]. Pairwise genetic distances for both maximum intraspecific and minimum interspecific (nearest-neighbour, NN) were generated in the BOLD Systems environment (available at https://boldsystems.org/) using the Barcode Gap Analysis tool and the Kimura 2-parameter (K2P) model. In order to check the clustering pattern of Trichophoromyia sequences, the consensus alignment was used to generate a maximum likelihood (ML) phylogenetic tree in the IQ-TREE software [27]. For this, we used the automatic model selection, and 10,000 ultrafast bootstrap pseudoreplicates in the IQ-TREE web server (http://iqtree.cibiv.univie.ac.at/ [28]). A sequence of Lutzomyia longipalpis (Lutz & Neiva, 1912) (KP112583.1) was included as an outgroup to root the ML tree. Tree visualization and editing were done in the iTOL v5 web server (https://itol.embl.de [29]).

The DNA barcode sequences were also identified at the molecular operational taxonomic unit (MOTU) level, which are groups of specimens based on their molecular similarity at a given molecular marker [30]. For this, we employed the automatic barcode gap discovery (ABGD) and refined single linkage (RESL) methods [31, 32]. The ABGD analysis (available at https://bioinfo.mnhn.fr/abi/public/abgd/abgdweb.html) was run using the K2P model, and the parameters Pmin = 0.005, Pmax = 0.1, and X = 1.5. For ABGD, the recursive partitions generated with the prior intraspecific divergence of 0.013 were considered. RESL analysis was run inside the BOLD environment using the ‘cluster sequences’ tool and default parameter.

Results

Family Psychodidae Newman, 1834

Subfamily Phlebotominae Rondani & Berté, in Rondani 1840

Genus Trichophoromyia Barretto, 1962

Trichophoromyia peixotoi n. sp. Rodrigues, Pinto & Galati (Figs. 1, 2, 3, 4, and 5)

Fig. 1.

Fig. 1

Trichophoromyia peixotoi n. sp. holotype: A Head, dorsal view (scale bar: 100 μm). B Flagellomeres FX–FXIV (scale bar: 50 μm)

Fig. 2.

Fig. 2

Wing of Trichophoromyia peixotoi n. sp. holotype (scale bar: 500 μm)

Fig. 3.

Fig. 3

Lateral view of male terminalia of the holotype (A) and the paratype M2 (E-16395) (B) of Trichophoromyia peixotoi n. sp. (scale bar: 200 μm)

Fig. 4.

Fig. 4

Trichophoromyia peixotoi n. sp. holotype (A and C), and paratype M2 (E-16395) (B and D): A, B Male terminalia, lateral view (scale bar: 100 μm). C, D Paramere, lateral view (scale bar: 20 μm)

Fig. 5.

Fig. 5

Trichophoromyia peixotoi n. sp. holotype. Genital filaments, with a focus on the apex of aedeagal duct (scale bar: 200 μm)

Diagnosis: The male of this new species can be distinguished from the others of the genus Trichophoromyia by characters of the terminalia, including the paramere with a triangular median lobe in the dorsal margin, and a rectangular paramere apex covered with fine bristles, in addition to the presence in the gonocoxite of a median cluster with about 12 thick and long setae.

Holotype description (male)

Insect predominantly brown in colour, with the pleurae pale. Pronotum, mesonotum, and metanotum dark brown. Katepisternum and katepimeron brown. Paratergite, upper anepisternum light brown. Medium-sized sand fly, total body length (from the head to the apex of the gonostylus) 2883 (3028.6; 88.71; n = 9).

Head (Fig. 1): length 373 (364.5; 9.9; n = 10), width 333 (331.1; 9; n = 9). Clypeus length 104 (100.2; 3.8; n = 10). Eye length 212 (206.7; 10.3; n = 10), width 101 (103.3; 4.9; n = 9). Interocular distance 132 (129.3; 4.3; n = 9). Interocular and interantennal sutures unconnected. Flagellomere lengths: FI 242 (222.7; 11; n = 9) FII 127 (121.2; 6.5; n = 9), FIII 124 (122.2; 4.6; n = 9), FXIII 69 (66.3; 2.9; n = 9), FXIV 58 (56.6; 4; n = 9). Labroepipharynx 221 (212; 8; n = 9). Preapical papilla present in FI and FII, but absent in FIII. Presence of apical, median, and basal papillae in FXII–FXIV. Simple setae present in FV–FXIV. Ascoidal formula FI–FXI 2, FXII–FXIV 0; ascoids long with rudimentary posterior spur, and the anterior projection reaching the basis of the subsequent flagellomere; internal/external ascoids implanted at nearly the same level; for FI, the external is slightly more basal than the internal. Labial sutures united. Palpal formula: 1.4.2.3.5. Newstead’s sensilla present in second palpal segment, and scattered in the third palpal segment. Length of the palpal segments: PI 33 (34.9; 3.1; n = 10), PII 85 (88.7; 3; n = 10), PIII 136 (129.4; 4.2; n = 9), PIV 58 (55.7; 3.3; n = 9), PV 159 (155.8; 8.7; n = 9).

Cervix: Ventro-cervical sensilla absent.

Thorax: length 525 (538.8; 21.2; n = 10), mesonotum length 501 (498.9; 18.8; n = 10). Pleurae with four proepimeral setae (3–4; n = 10) and 10 upper anepisternal setae (9–15; n = 10). Cervical sclerite with two sensilla. Wing (Fig. 2), length 2062 (2058.3; 58.5; n = 10), width 561 (573.9; 35.4; n = 10). Length of vein sections: R5 1261 (1289; 44.7; n = 10), R2 466 (539.4; 51.3; n = 10), R2+3 292 (268.9; 19.5; n = 10), R2+3+4 244 (238.6; 16.6; n = 10), delta 298 (365.2; 42.8; n = 10), pi 181 (150.1; 24.8; n = 10). Leg length: anterior, median, and posterior, respectively: coxa 330 (334.6; 11.6; n = 10), 319 (331.2; 6.3; n = 10), 332 (343.3; 10.9; n = 10). The remaining leg segments—femur, tibia, and tarsomeres—are not available for the holotype as they were processed for DNA extraction; however, we provide these measurements for some of the paratypes: femur (811; 32.1; n = 3), (784.3; 15.6; n = 3), (879.3; 25.5; n = 3); tibia (1053.7; 60.3; n = 3), (1318.3; 22.2; n = 3), (1502.3; 27.7; n = 3); tarsomere I (643; 16.8; n = 3), (775.3; 22.7; n = 3), (844.3; 22; n = 3); tarsomeres II+III+IV+V (692; 13; n = 3), (756; 28.6; n = 3), (824; 20; n = 3). Metatarsomere III (two verticils with spines, one median and one apical).

Abdomen: length 1394 (1494.7; 80; n = 10). Absence of tergal papillae from second to seventh tergites. Terminalia (Figs. 3 and 4): gonocoxite length 365 (382.4; 19.1; n = 10), width 124 (132.2; 17.7; n = 10); presence of a median cluster with about 12 (10–14; n = 10) thick and long setae, and more dispersed and thin bristles in the median-apical region of the gonocoxite, the most apical being thicker than the median portion. Gonostyle 226 (233; 9.8; n = 10) long, with four spines, having the following disposition: one apical 72 (85.3; 7; n = 10), the upper external preapical 55 (62.8; 8.6; n = 10), the lower external implanted after the medium region, so that it is closer to the upper than the internal one, which is implanted at the basal third of the gonostyle. Preapical spiniform setae absent. Paramere simple; dorsal margin length 189 (187.3; 7.8; n = 10) forming a triangular median lobe covered with fine bristles; apex of paramere rectangular, covered with fine bristles; ventral margin length of paramere 258 (246.4; 10.2; n = 10) with a small cluster of about 12 short setae. Parameral sheath triangular, dorsal margin length 89 (89.6; 5.6; n = 10), ventral 52 (55; 5.1; n = 10), and basal 72 (76.3; 5.3; n = 10). Epandrial lobe length 468 (464.6; 11.5; n = 10), width 29 (32; 1.9; n = 10). Cercus length 212 (219.2; 13.9; n = 10). Sperm pump (Fig. 5) length 172 (171.2; 3.7; n = 10); ejaculatory apodeme length 131 (137.1; 5.7; n = 10); sperm sac length 56 (52.2; 2.4; n = 10), width (26; 26.6; n = 10); pavillion width 40 (35.6; 5.5; n = 10); aedeagal duct 1020 (1034.2; 66; n = 9); ratio of aedeagal duct/sperm pump 5.9 (6; 0.3; n = 9); apex of the aedeagal duct tapered (Figs. 4D and 5).

DNA barcoding

The sequencing and analysis of the COI DNA barcoding region resulted in fragments ranging from 584 to 658 base pairs. Of the 10 analysed specimens (one holotype and nine paratypes), COI sequences of five paratypes were obtained. The visual inspection of the alignment indicates the absence of stop codons in the middle of sequences, pseudogenes, and/or nuclear copies of mitochondrial origin (NUMT).

In total, the five new COI sequences of T. peixotoi n. sp. were analysed with 16 publicly available barcode sequences of T. auraensis (Mangabeira [33]), T. octavioi (Vargas [34]), T. reburra (Fairchild & Hertig [35]), and T. viannamartinsi (Sherlock & Guitton [36]), totalling an alignment of 21 COI sequences and five species (Table 1). The maximum intraspecific K2P distance ranged from 0 to 1.39%, and the minimum distance to the nearest neighbour ranged from 1.92 to 13.3% (Table 1). In general, the interspecific distance was low, but T. reburra reached the highest value (13.3%), in discordance with the relationships of the other four species (Table 1).

Table 1.

DNA barcoded sand flies of the genus Trichophoromyia. Number of analysed sequences, maximum intraspecific genetic divergence, and the minimum distance to the nearest neighbour (interspecific) are given in percentage values

Species n Maximum intraspecific K2P distance (mean) Distance to the nearest neighbour
Trichophoromyia auraensis (Mangabeira) 5 0 (0) 1.92
Trichophoromyia octavioi (Vargas) 3 0.86 (0.57) 1.92
Trichophoromyia peixotoi n. sp. Rodrigues, Pinto & Galati 5 1.39 (0.79) 1.92
Trichophoromyia reburra (Fairchild & Hertig) 3 0.17 (0.11) 13.3
Trichophoromyia viannamartinsi (Sherlock & Guitton) 5 0.69 (0.31) 3.89

The phylogenetic inference recovered five well-supported clades that are in agreement with the analysed nominal species. In the same sense, the species delimitation algorithms sorted the COI sequences in MOTUs that agree with morphological identification (Fig. 6). Also, the ML analysis revealed a single well-supported clade containing the species T. auraensis, T. octavioi, T. peixotoi n. sp., and T. viannamartinsi, which seem to be more related to each other than to T. reburra (Fig. 6).

Fig. 6.

Fig. 6

Phylogenetic gene tree based on COI DNA barcodes of Trichophoromyia spp. Numbers near nodes indicate bootstrap values above 50. Lateral grey bars indicate the MOTU species delimitation partitions made by the algorithms ABGD and RESL

Type material

The male holotype and paratypes were collected in the PNA using CDC-type light traps operated overnight (Pinto et al. Col.). Holotype and three paratypes male were collected on 12 November 2022 near the Uruá base of the PNA. Four paratypes were collected on 7 July 2022, also near the Uruá base, and two were collected on 10 September 2022 near the Tracoá base of the PNA. These two latter specimens were collected in the tree canopy and were slide-mounted using Enecê resin, while the others were above the ground level and mounted using Canada balsam.

The five sand flies processed for molecular analysis correspond to the paratypes which were collected on 10 September 2022 (GenBank accession numbers OQ843041–OQ843042) and 12 November 2022 (OQ843038–OQ843040).

The holotype and paratypes are deposited in the Coleção de Referência da Faculdade de Saúde Pública (FSP–USP) at the Universidade de São Paulo, São Paulo, Brazil under museum numbers E-16393–E-16402.

ZooBank registration

To comply with the regulations set out in Article 8.5 of the amended 2012 version of the International Code of Zoological Nomenclature [49], details of the new species have been submitted to ZooBank. The Life Science Identifier (LSID) of the article is urn:lsid:zoobank.org:pub:43B5EC2C-239A-4D15-9969-A4C28726C575. The LSID for the new species name Trichophoromyia peixotoi is urn:lsid:zoobank.org:act:EF1DD733-4958–4669-BEE8-E35B92788B21.

Etymology

The name Trichophoromyia peixotoi is a tribute to Professor Alexandre Afranio Peixoto, for his great contribution to the knowledge of sand flies, especially in studies on population genetics.

Discussion

Trichophoromyia, a genus of the Psychodopygina subtribe comprising 44 nominal species, is morphologically characterized by the absence of ventro-cervical sensilla and papilla in the third flagellomere, and the presence of Newstead’s sensilla on the second palpal segment; male terminalia equivalent to or longer than the length of the thorax, and short gonostyle apical spine; females having cibarium with more than four pairs of posterior teeth, the anterior teeth distributed in several lines, and a wide sclerotized area; and lacinia with the external teeth implanted in two longitudinal lines and spermathecae with more than 20 rings [8]. The distinction between the species of Trichophoromyia has basically been based on the characteristics of the genitalia, especially of males. For females, the great similarity between the spermathecae has been an obstacle to the distinction of species, so that only 50% of them have females described. Among these, T. reburra differs from all others of the genus because it presents hyaline concretions on the spermathecal ducts, and T. cellulana (Young [37]), T. omagua (Martins, Llanos & Silva [38]), Trichophoromyia sp. 1 de Araracuara (Morales & Minter [39]), and T. ubiquitalis (Mangabeira [33]) are clearly distinguishable from all others by the apical ring of spermathecae which is three or less times as long as the preapical ring, while in the others this ring is six or more times longer [8]. In the present study, together with T. peixotoi n. sp. that clearly belongs to Trichophoromyia by morphology, we also collected males of T. ubiquitalis, and another undescribed Trichophoromyia sp. that is being published by another research group. In addition, we collected only female specimens having spermathecae with an apical ring six or more times as long as the preapical. Thus, it was not possible to make a reliable association of sexes by morphological characters, and the female of T. peixotoi n. sp. remains unknown.

This new species presents a dorsal lobe covered with thin bristles situated closer to the apex than to the base of the paramere, and the paramere apex facing towards the gonocoxite and gonostyle. These characteristics of the paramere of T. peixotoi n. sp. present similarities to those of a group of species constituted by T. adelsonsouzai Santos, Silva, Barata, Andrade & Galati [40], T. brachipyga (Mangabeira [33]), T. dunhami (Causey & Damasceno [41]), T. eurypyga (Martins, Falcão & Silva [42]), T. gibba (Young & Arias [43]), and T. viannamartinsi. However, all these aforementioned species present the cluster of thick bristles of gonocoxite in smaller numbers than T. peixotoi n. sp. (10–14), T. gibba (4–7), T. viannamartinsi (2), and T. brachipyga (4–6). In addition, T. peixotoi n. sp. also presents clear differences in the shape of the dorsal lobe and apex of the paramere: the dorsal lobe has a more triangular and the apex a more rectangular aspect regarding these closely related species. Moreover, these species have a gonostyle with a short and thicker apical spine, while in T. peixotoi n. sp. it is longer and thinner.

Beyond morphology, we accessed the information regarding one mitochondrial molecular marker, the COI gene fragment of DNA barcoding. Here, we did not use the COI barcode sequences for diagnostic purposes, mainly because most of the described species of the genus Trichophoromyia do not have available sequences, with less than 10% of its species processed for the COI gene [12], which makes the diagnostic potential of barcodes limited, although molecular analysis of T. peixotoi n. sp. supported the description of this new taxon.

Phylogenetic analysis of the COI gene recovered the analysed species into single clades each, also in accordance with species delimitation algorithms. Thus, all sequences of T. peixotoi n. sp. and the other analysed nominal species have molecular differences that allow the identification between them, including the morphologically similar species T. viannamartinsi. This scenario is promising for entomological monitoring, as it would allow the identification of isomorphic females by molecular methods [4446]. Unfortunately, it was not possible to sequence females of the species collected in the type locality of T. peixotoi n. sp., but future studies will be able to associate males and females to elucidate possible morphological differences between females.

Despite the limited number of analysed taxa, T. peixotoi n. sp. seems to be closely related to T. auraensis, T. octavioi, and T. viannamartinsi, retrieving a well-supported monophyletic clade. All these species belong to the Trichophoromyia group with long aedeagal ducts, which are > 4 times the length of the sperm pump, differing from another group with shorter ducts (≤ 3 times the length of the sperm pump) [8]. The latter comprises T. reburra, T. meirai (Causey & Damasceno [47]), T. ubiquitalis, T. omagua, and T. uniniensis Ladeia-Andrade, Fé, Sanguinette & Andrade Filho [48]. In our molecular analysis, T. reburra had a large genetic divergence compared to the other species of the genus, reaching values of interspecific K2P distances greater than 13%, while the interspecific divergence of the other four Trichophoromyia species was always less than 4%. This evidence leads us to suppose that the aedeagal ducts/sperm pump ratio may be a relevant character to sort Trichophoromyia species into at least two subgenera, but studies comprising a greater number of taxa and different molecular markers are needed to reinforce this idea.

Conclusions

The description of T. peixotoi n. sp. brings the number of species in this genus to 45, with 24 of them occurring in Brazil. We added new COI barcode sequences to DNA repositories, which are useful for Trichophoromyia species delimitation, and can be used for further species identification by integrative approaches.

Acknowledgements

We thank Diomar Coutinho de Barros, Kennedy Alves de Oliveira, and Marcos Miranda de Almeida for the help in the fieldwork. We also thank the Instituto Chico Mendes de Conservação da Biodiversidade (ICMBio) for providing the collection permissions (number 81991-1).

Abbreviations

COI

Cytochrome c oxidase subunit I

MOTU

Molecular operational taxonomic unit

ABGD

Automatic barcode gap discovery

RESL

Refined single linkage

ML

Maximum likelihood

Author contributions

BLR, ISP and EABG participated in the morphological analysis of the specimens and taxonomic discussion. ISP collected the material in the field. BLR did the drawings and measurements of the new species. BLR did the DNA barcoding analysis. BLR drafted the manuscript. All the authors read and approved this manuscript.

Funding

This study was financed in part by the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior—Brasil (CAPES)—Finance Code 001.

Availability of data and materials

All sequences obtained from the study were deposited in the GenBank database under the accession numbers OQ843038–OQ843042.

Declarations

Ethics approval and consent to participate

The entomological collections were performed under authorization for activities with scientific purpose of the Brazilian Sistema de Autorização e Informação em Biodiversidade (SISBIO) for the capture of zoological material (no. 81991-2).

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

Footnotes

Publisher's Note

Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.

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Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Data Availability Statement

All sequences obtained from the study were deposited in the GenBank database under the accession numbers OQ843038–OQ843042.


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