Abstract
An ant-pathogenic neogregarine in Temnothorax affinis and T. parvulus (Hymenoptera: Formicidae) is described based on morphological and ultrastructural characteristics. The pathogen infects the hypodermis of the ants. The infection was mainly synchronous so that only gametocysts and oocysts could be observed simultaneously in the host body. Gametogamy resulted in the formation of two oocysts within a gametocyst. The lemon-shaped oocysts measured 11–13 μm in length and 8–10 μm in width. The surface of the oocysts is not smooth but contains many buds. A ring-shaped line containing rosary-arrayed buds line up in the equatorial plane of the oocyst. These specific characteristics were observed for the first time in neogregarine oocysts from ants. Polar plugs were recognizable clearly by light and electron microscopy. The oocyst wall was quite thick, measuring 775 to 1000 nm. Each oocyst contained eight sporozoites. The neogregarines in the two Temnothorax species show many similarities such as the size and shape of the oocysts, a relatively fragile gametocyst membrane, host affinity, and tissue preference. We identified these neogregarines as Mattesia cf. geminata, which is here recorded from natural ant populations in the Old World for the first time. All neogregarine pathogens infecting ants in nature so far have been recorded from the New World. We present the two ant species, Temnothorax affinis and T. parvulus, as new natural hosts for M. cf. geminata. Furthermore, the morphological and ultrastructural characteristics of the oocyst of M. cf. geminata are documented by scanning and transmission electron microscopy for the first time.
Similar content being viewed by others
Avoid common mistakes on your manuscript.
Introduction
Entomopathogens contribute to the natural regulation of insect populations, as they naturally infect many insect species and transmit between insect populations (Lange and Lord 2012; Baki et al. 2021). Gregarines are common protistan entomopathogens in insects. Among gregarines, only the neogregarines are frequent causes of insect morbidity and mortality by generally invading the fat body and thus consuming their host’s energy sources. Neogregarines have been isolated and identified from various insect orders including Coleoptera, Hymenoptera, Lepidoptera, and Siphonaptera (Buschinger and Kleespies 1999). Recently, studies on neogregarines have focused on the identification of new species (Yaman and Radek 2015, 2017), their presence in different insect groups, and their distribution in host populations (Yaman 2017).
Several neogregarines have been identified from different insect groups (Undeen and Vávra 1997), but studies on the neogregarine pathogens of ants (Formicidae) are still limited. Although there are current studies on faunistic or habitat types (Kiran and Karaman 2021; Stukalyuk et al. 2020, 2021), there is no further research on neogregarines from ants. Up to now, two members of the genus Mattesia and one undefined gregarine have been recorded from ants. The life cycle of Mattesia species in short is as follows (Perkins et al. 2000): oocysts are taken up orally; hatched sporozoites migrate to the fat body and develop into meronts; a first generation of micronuclear merozoites spreads the infection within the fat body; then macronuclear merozoites are formed and differentiate into gamonts; pairs of gamonts form gametocytes; after nuclear divisions including meiosis two zygotes emerge; each zygote transforms to a thick-walled oocysts with polar plugs and 4–8 internal sporozoites. Mattesia geminata from Solenopsis geminata is the only species from an ant identified at the species level (Jouvenaz and Anthony 1979). Later, it was also recorded from two Leptothorax species from the L. muscorum complex (Buschinger et al. 1995; Kleespies et al. 1997). This pathogen has also been experimentally transmitted to some other ant species from the genus Leptothorax (Buschinger and Kleespies 1999; Kleespies et al. 1997). One yet undescribed Mattesia species, which is morphologically clearly different from M. geminata, was recorded from Solenopsis invicta (Pereira et al. 2002). In addition to the two Mattesia species, one undefined gregarine pathogen was recorded from the Australian bull ant, Myrmecia pilosula (Crosland 1998). In the present study, we report M. geminata in populations of Temnothorax affinis and T. parvulus for the first time. Furthermore, we are the first to describe the morphological and ultrastructural characteristics of the oocyst of M. geminata by scanning and transmission electron microscopy.
Material and methods
Insect samples
The study was carried out on ant samples stored in 70% ethanol. Pupae and adults of Temnothorax affinis and T. parvulus, collected in 2012 and 2013 in Artvin and Gümüşhane, Turkey, respectively were provided by one (K.K.) of authors from his collections, originally collected from natural populations.
Pupae and adults of Temnothorax spp. were collected by hand from mixed forests in the northeast Black Sea region of Turkey. The insects were put into glass bottles to prevent possible contamination. They were brought to the laboratory and dissected as soon as possible. Detailed information about the collecting sites is given below:
Host species: Temnothorax affinis (Mayr 1855)
Site: Artvin-Şavşat-Kirazlı Village, 1662 m, N 41°15′06″, E 42°29′29″ and Kelkit-Babakonağı Village, 1800 m, N 40°03′24″, E 39°21′57″
Collection date: 12 August 2012 and 21 August 2013
Habitat: Mixed forest with spruce, elm, and maple (Acer pseudoplatanus), no slope, grasslands and spruce forests around
Microhabitat: Rotten beech branch
Examined samples: Twenty adults (worker) and three pupae
Host species: Temnothorax parvulus (Schenck 1852)
Site: Gümüşhane-Kelkit-Sadak Village, 1702 m, N 40°01′47″, E 39°38′05″
Collection date: 20 August 2013
Habitat: Oak forest (with very few Pinus sylvestris), 20° slope
Microhabitat: In soil
Examined samples: Twenty adults (worker) and two pupae
Light microscopy
Ant samples were examined for symptoms of infection under a stereo microscope. Then, each ant was dissected in insect Ringer solution and wet smears were examined for the presence of a neogregarine infection under a light microscope at a magnification of 200–1000 × (Yaman 2017). When an infection was found, the slides were air-dried and fixed in methanol for 2–5 min. The slides were then washed with distilled water and stained for approximately 10 h in freshly prepared 5% solution of Giemsa stain (stock solution, Carloerba, No. 6B712176C). Afterwards, the slides were washed in running tap water, air-dried, and re-examined under the microscope (Undeen and Vávra 1997). Detected gametocysts and oocysts were measured and photographed using Optika B-293PLi microscope with a digital camera and Optika Proview Digital Camera Software. The data of fresh oocysts are presented as mean values ± standard deviation. Parts of the infected specimens were used for preparing samples for scanning (SEM) and transmission (TEM) electron microscopy.
Electron microscopy
Samples for transmission electron microscopy were fixed in 2.5% glutaraldehyde in 0.1 M cacodylate buffer (pH 7.4) for 2 h, rinsed in cacodylate buffer, post-fixed in 1% OsO4 for 2 h, and rinsed in cacodylate buffer. After dehydration in an increasing ethanol series, parts of infected beetles were embedded in Spurr’s resin (Spurr 1969). Ultra-thin sections were mounted on Pioloform-coated copper grids which were stained with saturated uranyl acetate and Reynolds lead citrate (Reynolds 1963). They were then examined with a Philips EM 208 transmission electron microscope. For scanning electron microscopy, tissue samples stored in distilled water were crushed in a drop of water, slightly spread on a cover glass, and air dried. After sputtering with gold, the samples were observed in a FEI Quanta 200 scanning electron microscope.
Results
There were no obvious external signs of infection under the stereo microscope. Under the light microscope, neogregarine infections were found only in four pupae of the two Temnothorax species, T. affinis and T. parvulus, collected from two natural populations. The typical lemon-shaped oocysts and early gametocysts of the pathogen were observed in the hypodermis (Figs. 1, 2, 3, and 4). The stages were also found dispersed in the hemolymph (Fig. 1) but did not infect tissues other than hypodermis. The infection was synchronous so that only early gametocysts and oocysts could be observed at the same time, but not other, vegetative stages (Figs. 1, 4). This was true for infected pupae. We could not find any infection in twenty adult (worker) individuals for each ant species from two colonies.
The gametocyst wall appeared to be fragile and not resistant so that mature oocysts were rarely observed in pairs. The oocysts were lemon-shaped and had a quite uniform size. Fresh oocysts (n = 50) measured 12.26 ± 0.62 (11.04–13.29) in length and 9.04 ± 0.37 (8.20–9.87) μm in width in T. affinis and Giemsa-stained oocysts measured 11.29 ± 0.53 (10.5–12.36) in length and 7.53 ± 0.63 (6.35–8.57) μm in width in T. affinis and 11.27 ± 0.78 (10.21–12.3) in length and 7.49 ± 0.47 (6.5–8.32) μm in width in T. parvulus. Polar plugs were recognizable clearly by light microscopy (Fig. 1). Each oocyst contained eight sporozoites (Fig. 3). Detailed examination of the oocyst by scanning electron microscopy showed that clearly visible annular ridges surround the polar plugs (Figs. 5, 6, and 7).
The surface of the oocysts is not smooth but contains many buds (Figs. 5, 6, and 7). Additionally, a ring-shaped line containing rosary-arrayed buds line up in the equatorial plane of the oocyst (Figs. 5, 6). The structure of the oocyst was well seen in the transmission electron microscope (Figs. 8, 9, 10, 11, and 12).
The polar plug measured 1000 to 1100 nm in diameter, excluding the annular ridge. The oocyst wall with the surface buds was quite thick, measuring 775 to 1000 nm (Figs. 8, 9, 11, 12). The wall consisted of two layers, a very thin, more electron-dense outer layer and a thick, less electron-dense inner layer. The ring surrounding the polar plug was clearly visible in a longitudinal section of the oocyst (Fig. 10).
Discussion
Taxonomic identity
Light and electron microscopic observations revealed that the neogregarine pathogen detected in Temnothorax species has typical characteristics of the members of the genus Mattesia Naville, 1930 (family Lipotrophidae) as two oocysts within a gametocyst and eight sporozoites within each oocyst (Jouvenaz and Anthony 1979; Kleespies et al. 1997; Perkins et al. 2000; Undeen and Vávra 1997). Mattesia exclusively infects insects. To date, two Mattesia species, M. geminata and Mattesia sp., and one undefined gregarine infection have been observed in ants (Table 1) (Jouvenaz and Anthony 1979; Buschinger et al. 1995; Pereira et al. 2002). All infected ant hosts belong to the subfamily Myrmicinae (Formicidae: Hymenoptera). The typical infection site in all recorded Mattesia infections is the hypodermis (Fig. 8; Table 1). Large gametocysts with numerous oocysts (> 70) are typical for the undefined gregarine of the Australian bull ant Myrmecia pilosula, and thus this pathogen is clearly distinct from the genus Mattesia (Crosland 1998). Oocysts of the undescribed Mattesia species from Solenopsis invicta are larger than the ones of M. geminata and may thus belong to new species (Pereira et al. 2002). The oocyst size of the neogregarine found in our study closely resembles the oocyst size of M. geminata.
The host affinity is generally recognized as a valid taxonomic character for differentiating neogregarine species from insects (Jouvenaz and Anthony 1979; Kleespies et al. 1997; Levine 1988; Lord 2003). However, the host specificity of M. geminata in infection experiments using different ant species as hosts was ambiguous. While the authors were not able to transfer this pathogen from Solenopsis geminata to S. invicta, they succeeded in infecting some species belonging to other genera of the subfamily Myrmicinae, such as Leptothorax acervorum, L. muscorum, L. unifasciatus, L. recedens, and Harpagoxenus sublaevis (Buschinger and Kleespies 1999).
The neogregarine pathogen from Temnothorax species shows many matches with M. geminata (Jouvenaz and Anthony 1979) such as size and shape of oocysts, relatively fragile gametocyst membrane, host affinity, and tissue preference. The dimensions of the oocysts are a good criterion for comparing neogregarines from different insect hosts (Pereira et al. 2002). As seen in Table 1, the neogregarine in this study shows a considerable difference in oocyst size compared to Mattesia sp. from S. invicta. The oocyst of the pathogen presented here is much smaller, especially in length (12.26 ± 0.62 (11.04–13.29 μm)), than the oocyst of Mattesia sp. (18.7 × 10.8) from S. invicta (Pereira et al. 2002). However, it is relatively similar to the oocyst of M. geminata from Solenopsis geminata (11.3 × 7.9; Jouvenaz and Anthony 1979) and that from two Leptothorax species from the L. muscorum complex (13.8 × 9.3 μm; Buschinger et al. 1995). Except for insignificant variations in size between the described M. geminata oocysts, there are no morphological differences justifying the creation of a new species for the neogregarine from the Temnothorax species. Thus, we conclude that the reported pathogen in natural populations of two Temnothorax species is identical to M. geminata and thus, T. affinis and T. parvulus should be added to the list of hosts for this pathogen. However, we named the identified neogregarine pathogen as Mattesia cf. geminata. Confer (cf.) is used for the pathogen species as it cannot be supported with a comparison of 18S rRNA sequences of neogregarine pathogens from ants to confirm the pathogen clearly as M. geminata recorded from original host.
Ultrastructure
All descriptions of M. cf. geminata were based on light microscopic observations to date, but in the present study, we provided ultrastructural information in addition to detailed morphological analysis. In two recent studies, we presented fine structural features of oocysts from two species of different neogregarine genera, Mattesia weiseri from Dendroctonus micans (Coleoptera: Curculionidae) (Yaman and Radek 2015) and Ophryocystis anatoliensis from Chrysomela populi (Coleoptera: Chrysomelidae) (Yaman and Radek 2017). Both species have oocysts with a smooth surface and without annular ridges around the polar plugs. In contrast, unlike M. geminata, clearly visible annular ridges that surround the polar plugs further distinguish M. weiseri and O. anatolensis from M. cf. geminata.
Life cycle and pathogenicity of Mattesia species
In the original study, Jouvenaz and Anthony (1979) found M. geminata in the pupae of S. geminata, and not in adults from infected colonies. They showed that the reason for the absence of pathogens in adults was that the pupae died and could not mature as the disease appeared to be fatal. Later Buschinger et al. (1995) also found M. geminata in the pupae of Leptothorax ants. We also found M. cf. geminata only in the pupae of Temnothorax species and not in the adults from the infected colonies. Other neogregarine species do not seem to cause mortality of ant pupae. Crosland (1998) reported an undefined gregarine pathogen in adults of the Australian bull ant Myrmecia pilosula, and Pereira et al. (2002) found Mattesia sp. in adults of the red imported fire ant S. invicta in Florida. Buschinger and Kleespies (1999) proved experimentally that M. geminata can infect several other ant species from the subfamily Myrmicinae. According to these studies, there is a possibility that M. geminata can infect adult ants under natural conditions.
Neogregarines infect insects, and many species are pathogenic to their hosts. They are usually found in the fat body, hemolymph, hypodermis, gut, or Malpighian tubules. The most common site of infection is the fat body. However, neogregarines found in ants generally show a tissue specificity for the hypodermis. M. geminata seems to even have different tissue affinities in different ant hosts (Kleespies et al. 1997). In Leptothorax species, e.g., it first multiplies in the hemolymph before it enters the hypodermis and fat body (Kleespies et al. 1997), while in S. geminata it only infects the hypodermis and oenocytes (Jouvenaz and Anthony 1979). In Temnothorax. we found the neogregarine in fat body, hypodermis, and hemocoel at the same time. Neogregarine infections in ants may cause specific symptoms. The earliest pathogenic symptom of a M. geminata infection in S. geminata appears as an irregularity of the developing eyes of the pupa, followed by melanization of the cuticle, and then the entire pupa becomes solid black (Jouvenaz and Anthony 1979). M. geminata also causes an irregular eye pigmentation of the gray pupae of Leptothorax species (Buschinger et al. 1995). An undescribed Mattesia species in the red fire ant, S. invicta, causes a typical yellow-orange colored head and sometimes thorax and was therefore designated Mattesia “yellow-head disease” (YDS) (Pereira et al. 2002). According to Crosland (1998), a strong infection with the undefined gregarine in the Australian bull ant, Myrmecia pilosula, interferes with the normal darkening of cuticle in the pupal stage, leading to abnormal brown ants. In contrast to these symptoms in different ant species, we did not observe any symptoms in the infected pupae of the two investigated Temnothorax species.
The ant genus Temnothorax Mayr is one of the most species-rich genera in the subfamily Myrmicinae (Rasheed et al. 2020), and Leptothorax and Temnothorax are closely relative genera. Leptothorax has a distribution in North America, Western Asia, and the northern parts of Europe, while Temnothorax has a general holarctic distribution. Species of both genera live in very diverse habitats—from cold forests in the forest-tundra zone to the dry steppe or even semi-desert and can be found in the same habitat (Bolton 2003; Radchenko 2004). One of the interesting results of our study is that the locations (Artvin and Gümüşhane, Türkiye) of the Temnothorax species infected with M. cf. geminata are from the Old World. All neogregarine pathogens infecting ants in nature so far have been recorded from the New World (Table 1).
Data availability
All of the data generated and analyzed during this study are included in this published manuscript.
References
Baki D, Tosun HŞ, Erler F (2021) Indigenous entomopathogenic fungi as potential biological control agents of rose sawfly, Arge rosae L. (Hymenoptera: Argidae). Turk J Zool 45:517–525. https://doi.org/10.3906/zoo-2105-15
Bolton B (2003) Synopsis and classification of Formicidae. Mem Am Entomol Inst 71:1–370
Buschinger A, Kleespies RG (1999) Host range and host specificity of ant-pathogenic gregarine parasite, Mattesia geminata (Neogregarinida: Lipotrophidae). Entomol Gen 24:93–104
Buschinger A, Kleespies RG, Schumann RD (1995) A gregarine parasite of Leptothorax ants from North America. Ins Soc 42:219–222
Crosland MWJ (1998) Effect of a gregarine parasite on the color of Myrmecia pilosula (Hymenoptera: Formicidae). Ann Entomol Soc Am 81:481–484. https://doi.org/10.1093/aesa/81.3.481
Jouvenaz DP, Anthony DW (1979) Mattesia geminata sp. n. (Neogregarinida: Ophrocystidae) a parasite of the tropical fire ant, Solenopsis geminata (Fabricus). J Protozool 26:354–356
Kiran K, Karaman C (2021) Ant fauna (Hymenoptera: Formicidae) of central Anatolian region of Turkey. Turk J Zool 45:161–196. https://doi.org/10.3906/zoo-2008-6
Kleespies RG, Huger AM, Buschinger A, Nähring S, Schumann RD (1997) Studies on the life history of a neogregarine parasite found in Leptothorax ants from North America. Biocontrol Sci Technol 7:117–129
Lange CE, Lord JC (2012) Chapter 10 – protistan entomopathogens. In: Vega FE, Kaya KK (eds) Insect pathology, 2nd edn. Academic Press, pp 367–394. https://doi.org/10.1016/B978-0-12-384984-7.00010-5
Levine ND (1988) The protozoan phylum Apicomplexa, vol 1 and 2. CRC Press, Boca Raton, p 357
Lord JC (2003) Mattesia oryzaephili (Neogregarinorida: Lipotrophidae), a pathogen of stored-grain insects: virulence, host range and comparison with Mattesia dispora. Biocontrol Sci Technol 13:589–598. https://doi.org/10.1080/0958315031000151800
Pereira RM, Williams DV, Becnel JJ, Oi HD (2002) Yellow-head disease caused by a newly discovered Mattesia sp. in populations of the red imported fire ant. Solenopsis Invicta J Invertebr Pathol 81:45–48
Perkins FO, Barta JR, Clopton R, Peirce MA, Upton SJ (2000) Phylum Apicomplexa. In: Lee JJ, Leedale GF, Bradbury P (eds) An illustrated guide to the protozoa, 2nd edn. Society of Protozoologists, Lawrence USA, pp 190–369
Radchenko A (2004) A review of the ant genera Leptothorax Mayr and Temnothorax Mayr (Hymenoptera, Formicidae) of the Eastern Palaearctic. Acta Zool Acad Sci Hung 50:109–137
Rasheed MT, Bodlah I, Magomedovıch YZ, Fareen AGE, Bodlah MA, Prebus M, Wachkoo AA (2020) Preliminary contributions toward a revision of the ant genus Temnothorax Mayr Hymenoptera: Formicidae from Pakistan. Turk J Zool 44:375–381. https://doi.org/10.3906/zoo-2003-54
Reynolds ES (1963) The use of lead citrate at high pH as an electron-opaque stain in electron microscopy. J Cell Biol 17:208–212
Spurr AR (1969) A low-viscosity epoxy resin embedding medium for electron microscopy. Clin Microbiol Res 3:197–218
Stukalyuk S, Radchenko Y, Netsvetov M, Gilev A (2020) Effect of mound size on intranest thermoregulation in the red wood ants Formica rufa and F. polyctena (Hymenoptera, Formicidae). Turk J Zool 44:266–280. https://doi.org/10.3906/zoo-1912-26
Stukalyuk S, Gilev A, Antonov I, Netsvetov M (2021) Size of nest complexes, the size of anthills, and infrastructure development in 4 species of red wood ants (Formica rufa, F. polyctena, F. aquilonia, F. lugubris) (Hymenoptera; Formicidae). Turk J Zool 45:464–478. https://doi.org/10.3906/zoo-2105-39
Undeen AH, Vávra J (1997) Research methods for entomopathogenic protozoa. In: Lacey L (ed) Manual of techniques in insect pathology. Academic Press, London, pp 117–151
Valles SM, Pereira RM (2003) Use of ribosomal DNA sequence data to characterize and detect a neogregarine pathogen of Solenopsis invicta (Hymenoptera: Formicidae). J Invertebr Pathol 84:114–118. https://doi.org/10.1016/j.jip.2003.09.001
Yaman M (2017) Distribution and occurrence of the neogregarine pathogen, Ophryocystis anatoliensis (Apicomplexa) in populations of Chrysomela populi L. (Coleoptera: Chrysomelidae). Acta Protozool 56:283–288
Yaman M, Radek R (2015) Mattesia weiseri sp. nov., a new neogregarine (Apicomplexa: Lipotrophidae) pathogen of the great spruce bark beetle, Dendroctonus micans (Coleoptera: Curculionidae, Scolytinae). Parasitol Res 114:2951–2958
Yaman M, Radek R (2017) Ophryocystis anatoliensis sp. nov., a new neogregarine pathogen of the chrysomelid beetle Chrysomela populi. Eur J Protistol 59:26–33
Acknowledgements
Temnothorax samples in this study were provided by one (K.K.) of authors from his collections. The author wants to mention that he received TUBITAK support while collecting these samples for another faunistic study.
Author information
Authors and Affiliations
Contributions
Mustafa Yaman conducted experiments, identified the neogregarine pathogen, and wrote the manuscript. Kadri Kıran provided ant samples. Renate Radek conducted experiments and improved the manuscript.
Corresponding author
Ethics declarations
Ethical approval
This is not applicable to the present manuscript.
Consent to participate
This is not applicable to the present manuscript.
Consent for publication
All authors reviewed and approved the final version of the manuscript.
Conflict of interest
The authors declare no competing interests.
Additional information
Handling Editor: Julia Walochnik
Publisher's note
Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Rights and permissions
Springer Nature or its licensor (e.g. a society or other partner) holds exclusive rights to this article under a publishing agreement with the author(s) or other rightsholder(s); author self-archiving of the accepted manuscript version of this article is solely governed by the terms of such publishing agreement and applicable law.
About this article
Cite this article
Yaman, M., Kıran, K. & Radek, R. Mattesia cf. geminata, an ant-pathogenic neogregarine (Apicomplexa: Lipotrophidae) in two Temnothorax species (Hymenoptera: Formicidae). Parasitol Res 122, 1573–1579 (2023). https://doi.org/10.1007/s00436-023-07860-0
Received:
Accepted:
Published:
Issue Date:
DOI: https://doi.org/10.1007/s00436-023-07860-0