Phylogenetic Analysis and Karyotype Evolution in Two Species of Core Gruiformes: Aramides cajaneus and Psophia viridis
by
,
Ivanete de Oliveira Furo
1,2,3, 
Rafael Kretschmer
3,4
,
Patrícia C. M. O’Brien
3,
Jorge C. Pereira
3,
Malcolm A. Ferguson-Smith
3 and 
Edivaldo Herculano Corrêa de Oliveira
2,5,*
1
Post-Graduation Program in Genetics and Molecular Biology, Federal University of Pará, Belém, Pará 66075-110, Brazil
2
Laboratory of Tissue Culture and Cytogenetics, SAMAM, Evandro Chagas Institute, Ananindeua, Pará 67030-000, Brazil
3
Cambridge Resource Centre for Comparative Genomics, Cambridge CB3 0ES, UK
4
Pos-Graduation Program in Genetics and Molecular Biology, Federal University of Rio Grande do Sul, Porto Alegre, Rio Grande do Sul 91509-900, Brazil
5
Faculty of Natural Sciences, Institute of Exact and Natural Sciences, Federal University of Pará, Belém, Pará 66075-110, Brazil
*
Author to whom correspondence should be addressed.
Genes 2020, 11(3), 307; https://doi.org/10.3390/genes11030307
Submission received: 30 January 2020
/
Revised: 4 March 2020
/
Accepted: 10 March 2020
/
Published: 13 March 2020
(This article belongs to the Special Issue Mechanisms Driving Karyotype Evolution and Genomic Architecture)
Abstract
:Gruiformes is a group with phylogenetic issues. Recent studies based on mitochondrial and genomic DNA have proposed the existence of a core Gruiformes, consisting of five families: Heliornithidae, Aramidae, Gruidae, Psophiidae and Rallidae. Karyotype studies on these species are still scarce, either by conventional staining or molecular cytogenetics. Due to this, this study aimed to analyze the karyotype of two species (Aramides cajaneus and Psophia viridis) belonging to families Rallidae and Psopiidae, respectively, by comparative chromosome painting. The results show that some chromosome rearrangements in this group have different origins, such as the association of GGA5/GGA7 in A. cajaneus, as well as the fission of GGA4p and association GGA6/GGA7, which place P. viridis close to Fulica atra and Gallinula chloropus. In addition, we conclude that the common ancestor of the core Gruiformes maintained the original syntenic groups found in the putative avian ancestral karyotype.
1. Introduction
Despite major progress in the reconstruction of phylogeny of Aves in the last decade, the classification of species within the order Gruiformes still represents one of the least stable among this class [1,2]. Nowadays, the order Gruiformes contains five modern families: Heliornithidae, Aramidae, Gruidae, Psophiidae and Rallidae, this last one greatly exceeding other Gruiformes families in species richness (144 species), geographical range and taxonomic complexity [3,4]. In addition, some gaps on the evolutionary history and interrelationships among Gruiformes species also remain unsolved. For example, the taxonomy of the Rallidae family has been the subject of debate, mainly because this group has adapted to similar environments across their geographic distribution, and consequently, they have been subject to convergence evolution, making difficult the understanding of their evolutionary origins [3,4,5]. Members of the Rallidae family inhabit a range of ecological environments, including freshwater and saltwater marshes, mangroves, sparsely vegetated atolls, cool-temperate woodlands, tropical forests and grasslands [3]. Similarly, the relationship of Psophiidae, a family of birds restricted to the Amazon basin forests, with the other five families included in the core Gruiformes is still controversial [4].
Concerning cytotaxonomic data, the karyotypes of Gruiformes are characterized by the typical avian formula, with diploid numbers (2n) close to 2n = 80, consisting of approximately 10 pairs of macrochromosomes and 30 pairs of indistinguishable microchromosomes [6,7,8]. However, there are species outside this standard, such as Porzana albicollis (2n = 72) [7] and Fulica atra (2n = 92) [6].
The advances in comparative chromosome mapping with the use of chromosome painting has provided important information for inferences about phylogenetic relationships in some groups of birds, clarifying some problems left by the analyses of molecular biology [9,10,11,12,13,14]. Furthermore, despite the apparent karyotypical conservation among birds observed by conventional staining, comparative chromosome painting has revealed many rearrangements, such as fusions and fissions in several macrochromosomes; this information allowed the inference of a putative ancestral karyotype (PAK) of birds, which is actually highly similar to the chromosomal complement of Gallus gallus, with the exception of pair 4, which corresponds to two distinct pairs in the proposed ancestral karyotype [9,10,11,15,16].
Up to now, comparative chromosome painting has been performed in only two species of Gruiformes—the coot (Fulica atra—FAT) and common moorhen (Gallinula chloropus—GCH), both belonging to the Rallidae family. Fulica atra (2n = 92) and Gallinula chloropus (2n = 78) share the fissions of the ancestral chromosomes GGA5 and GGA4 [17]. Moreover, these species also share chromosome associations between GGA4/5 and GGA6/7 [17]. However, in order to understand the dynamics of the karyotype evolution in this group, it is necessary to analyze other species belonging to different families of Gruiformes.
Therefore, with the aim of broadening our understanding of the events occurring during the chromosomal evolution of Gruiformes, we carried out the comparative chromosome painting with chicken macrochromosome paints in two species of this order: Aramides cajaneus—ACA (Gray-necked Wood-Rail), a member of the Rallidae family and Psophia viridis—PVI (Green-winged Trumpeter), a member of the Psophiidae family. The goal of this study was to investigate (a) whether Aramides cajaneus shows a karyotype organization similar or different to Fulica atra and Gallinula chloropus and (b) whether Psophia viridis has similar or different rearrangements compared to Rallidade species. Based on the chromosome painting data for Aramides cajaneus and Psophia viridis, together with the data from the literature for other Gruiformes species, we discuss the possible process of karyotype evolution in Gruiformes.
2. Materials and Methods
2.1. Cell Cultures and Chromosome Preparations
Skin biopsies of Aramides cajaneus (one female) and Psophia viridis (one female) were collected at Museu Paraense Emilio Goeldi (Belém, PA, Brazil). The experiments were carried out according to the ethical protocols approved by an ethics committee (CEUA—Federal University of Pará) under no. 170/2013 and SISBIO 68443-1). Fibroblast cells were obtained from skin biopsies after dissociation with collagenase IV (0.0186 g in 4 mL of DMEM (Dulbecco’s Modified Eagle’s medium, Sigma-Aldrich, MO, USA), for 1 h at 37 °C, and maintained in DMEM medium (Sigma-Aldrich, MO, USA) supplemented with antibiotics (1%) and fetal bovine serum (15%) at 37 °C [18]. Chromosomal preparations were obtained after mitotic arrest by adding 100 µL colcemid (0.05 µg/mL) for 1 h, followed by suspension and incubation with 0.075 M KCl (10 min at 37 °C) and fixed in Carnoy’s fixative (3 methanol:1 acetic acid). Chromosome preparations were kept at −20 °C until the analyses.
2.2. Microscopic Analyses
At least 30 metaphases with conventional staining (Giemsa 5% in phosphate buffer, pH 6.8) were examined to determine the diploid number and chromosome morphology for each species. Images were captured using a 100× objective, microscopy DM1000 (Leica, CO, USA) and GenASIs software (ADS Biotec, Omaha, NE, USA) and the karyotype were ordered according to their arm ratios.
2.3. Chromosome Painting
Whole-chromosome probes of G. gallus (pairs 1–10) generated by flow-sorting (Cambridge Resource Centre for Comparative Genomics, Cambridge, UK) were labeled either with biotin or digoxygenin (Roche Diagnostics, Mannheim, Germany) by degenerate oligonucleotide-primed polymerase chain reaction (DOP-PCR) [19]. After denaturing in 70 °C for 10 min and preannealed for 30 min at 37 °C, the hybridization solution (1 µL labeled probe in 14 µL hybridization buffer) was added on slides with chromosome preparations previously desnatured at 70% formamide for 1 min and 20 s and dehydrated by serial ethanol dehydration (70%, 90% and 100%). Hybridization and detection by Avidin-Cy5 or anti-digoxygenin (Vector Laboratories, Burlingame, CA, USA), proceeded according to standard protocols [15]. Chromosomes were counterstained with 4′,6-diamidino-2-phenylindole (DAPI) (Sigma-Aldrich, St. Louis, MO, USA).
At least 10 metaphase spreads per individual were analyzed to confirm the hybridizations signals. FISH results were analyzed using a Zeiss Imager 2 microscope, 63× objective and images were captured using Axiovision v.4.8 software (Zeiss, Jena, Germany). Final edition of images was made using Adobe Photoshop CS6 software. For chromosomal evolution inferences, we used chromosome painting data from Fulica atra (FAT) and Gallinula chloropus (GCH) [17].
2.4. Phylogenetic Analysis
The inference of the phylogenetic tree was made based on cytogenetic information (chromosome painting) of four Gruiformes species, three belonging to the Rallidae Family (Fulica atra, Gallinula chloropus and Aramides cajaneus) and Psophiidae family (Psophia viridis), taking into consideration the presence or absence of chromosome features in these species.
3. Results
3.1. Karyotypes of Aramides cajaneus and Psophia viridis
The karyotype of Aramides cajaneus has 2n = 78. Pairs 1, 2 and 4 are submetacentric, while 5, 6 and 8 are metacentric. The remaining autosomal chromosomes are telocentric (Figure 1A). The Z and W sex chromosomes are metacentric. Psophia viridis has a karyotype comprised of 80 chromosomes. Pair 1 is submetacentric, while pairs 2 and 5 are acrocentric, and pair 4 is metacentric and easily distinguishable from other chromosomes. The remaining autosomal chromosomes are telocentric. Among the sex chromosomes, Z is submetacentric and the W chromosome is telocentric (Figure 1B).
3.2. Chromosome Painting
The chicken probes corresponding to pairs GGA1–10 showed the following correspondence in the karyotype of Aramides cajaneus (ACA): GGA1 (ACA1); GGA2 (ACA2); GGA3 (ACA3); GGA4 (ACA5 and ACA7); GGA5 (ACA4q); GGA6 (ACA6); GGA7 (ACA4p); GGA8 (ACA8); GGA9 (ACA9) and GGA10 (ACA10). In addition, an association between GGA5/GGA7 was identified in (ACA4) (Figure 2C,D); therefore, a total of 11 homology signals were found in the karyotype of A. cajaneus with GGA probes (Figure 2 and Figure 4A). However, in Psophia viridis, chicken painting probes showed a slightly different correspondence when compared to Aramides cajaneus. Hence, the homologies between chicken and Psophia viridis (PVI) are: GGA1 (PVI1); GGA2 (PVI2); GGA3 (PVI3); GGA4 (PVI5, PVI9 and ACA11); GGA5 (PVI6); GGA6 (PVI4q); GGA7 (PVI4p); GGA8 (PVI7); GGA9 (PVI8) and GGA10 (PVI9). Furthermore, a fission in GGA4 and an association between GGA6/GGA7 in (PVI4) were observe in this species, thereby, a total of 12 homology signals were observed between the chromosomes of P. viridis and GGA probes (Figure 3; Figure 4B).
3.3. Syntenic Blocks Shared among Gruiformes Species and Phylogentic Analyses
In order to proceed with the phylogenetic analysis, comparative chromosome painting data covering the homology of macrochromosome pairs of four species of Gruiformes—Aramides cajaneus and Psophia viridis from the present work, and Fulica atra and Gallinula chloropus previously described by [17]—were organized in a matrix (Table 1). The phylogenetic tree obtained is shown in Figure 5. F. atra and G. chloropus are more derived in relation to the A. cajaneus, and form a clade supported by three rearrangements—the fusion GGA4/GGA5 and GGA6/GGA7, and also the fission of GGA4p—chromosome features not observed in A. cajaneus. Concerning P. viridis, it would be closer to the clade formed by F. atra and G. chloropus, with which this species shares two rearrangements: the fission of GGA4p and the association GGA6/GGA7.
4. Discussion
The diploid chromosome numbers of both species analyzed are very similar, A. cajaneus 2n = 78 and P. viridis 2n = 80 (Figure 1). Additionally, both species are characterized by a typical avian karyotype, since the mode of the chromosome number in birds is 2n = 80, with a high number of microchromosomes [16,20].
In general, rearrangements found in Gruiformes involved chromosome pairs homologous to GGA4, GGA5, GGA6 and GGA7. The fission of ancestral syntenies GGA4p and GGA5 followed by fusion have been proposed as ancestral events in Gruiformes, since these rearrangements are present in F. atra and G. chloropus [17]. However, in P. viridis, only the fission in GGA4p has been observed, without the fusion between GGA4q/GGA5 (Figure 4A). Furthermore, A. cajaneus does not share these rearrangements (Figure 5).
The association GGA6/GGA7 has been found in two species of family Rallidae (F. atra and G. chloropus) [17] and family Psophiidae (P. viridis); however, it is absent in A. cajaneus (Table 1). The association between GGA6/GGA7 has been detected in five species belonging to different orders of birds: Galliformes—Numida meleagris [21], Strigiformes—Pulsatrix perspicillata [22], Trogoniformes—Trogon s. surrucura [23], Psittaciformes—Nymphicus hollandicus, Agapornis roseicollis, Melopsittacus undulates [24], Ara macao [25], Ara chloropterus, Anodorhynchus hyacinthinus [9], Psittacus erithacus [26], Pyrrhura frontalis, Amazona aestiva [11] and Columbiformes—Leptotila verreauxi [16]. Hence, GGA6/GGA7 association originated independently in five different orders.
The apparent multiple independent origins of associations between GGA6/GGA7 in avian species suggest that there are specific sites in these chromosomes that are susceptible to rearrangement processes (hotspots) [27,28,29]. This fact highlights the potential for the occurrence of rearrangements, such as chromosomal fusions, inversions and centromere shifts [30].
Phylogenetic Analysis
The results obtained from the experiments in this study, together with data previously published concerning two other Gruiformes (Table 1; Table 2), were plotted using the phylogenetic tree proposed by [4] and [5] to improve understanding of chromosomal evolution in this order (Figure 5).
In respect of family Rallidae, some phylogenetic relationships, such as F. atra and G. chloropus as sister-groups, are well supported [31,32]. According to [5], A. cajaneus was included in the ‘‘Aramides clade”, as a sister-group of “Fulica clade”. The chromosome data of these species corroborate this relationship, since F. atra and G. chloropus share the same chromosome rearrangements, such as associations GGA6/GGA7, GGA4/GGA5 and fissions of GGA4p and GGA5, not found in A. cajaneus (Figure 4B and Table 1 and Table 2). In this way A. cajaneus, which shares less chromosome syntenies with the other two species (F. atra and G. chloropus), would be more basal than the ‘Fulica clade’.
In our previous study with Eurypyga helias (Eurypygidae), formerly included in Gruiformes, but now regarded as belonging to a different order (Eurypygiformes) with only two families (Rynochetidae and Eurypygidae), we had proposed that the putative common ancestral karyotype of core Gruiformes would have a fission of GGA4p, since it had been found in the three species studied (P. viridis, F. atra and G. chloropus) (Table 1; Table 2) [10,17]. If this hypothesis was correct, A. cajaneus would have regained the ancestral character. Alternatively, the absence of this fission in A. cajaneus indicates that it does not represent a synapomorphy of the Gruiformes.
According to [29], there are regions of bird genomes that are prone to breakage, facilitating chromosomal rearrangements, and this could explain the fission of GGA4p in some species but not in A. cajaneus. As more bird genomes are sequenced, the reasons for the conservation of some syntenic groups, while others were disrupted and reorganized, will become clearer.
Despite the fact that the phylogenetic position of the Psophiidae family is not well resolved within the Core Gruiformes [4], our results show that P. viridis shares some rearrangements with F. atra and G. chloropus, such as fission of GGA4p and association of GGA6/GGA7 (Table 1; Table 2); these rearrangements place P. viridis close to F. atra and G. chloropus (Rallidae family) (Figure 5).
Accordingly, the last common ancestor from the Core Gruiformes would have a karyotype similar to the putative ancestral avian karyotype (PAK) [16], because some rearrangements that were found in this group are the result of independent events, such as the association between GGA5/GGA7 in A. cajaneus, despite the fact that some association and fission events were not found in all the species analyzed (Figure 5).
Thus, molecular cytogenetic analysis confirms earlier studies on the relationships between F. atra and G. chloropus. Furthermore, they support the fact that the chromosome rearrangements accumulated in P. viridis are similar to the Rallidae species, although A. cajaneus shows a karyotype organization different from F. atra and G. chloropus. Nevertheless, this study has improved our understanding of the process of karyotype evolution in the Core Gruiformes.
Author Contributions
Conceptualization, I.d.O.F. and E.H.C.d.O.; Data curation and formal analysis, I.d.O.F., R.K. and E.H.C.d.O.; Investigation, I.d.O.F. and R.K. Methodology, I.d.O.F., P.C.M.O. and J.C.P.; Project administration, E.H.C.d.O.; Funding acquisition, M.A.F.-S. and E.H.C.d.O.; Validation, I.d.O.F. and E.H.C.d.O.; Writing (original draft), I.d.O.F., R.K. and E.H.C.d.O.; Writing (review and editing), P.C.M.O. and M.A.F.-S. All authors have read and agree to the published version of the manuscript.
Funding
This research was partially funded by a grant to EHCO from CNPq (307382/2019-2) and to MAFS from the Wellcome Trust in support of the Cambridge Resource Centre for comparative genomics.
Acknowledgments
Authors would like to thank the Museu Paraense Emilio Goeldi (Belém, PA) for samples used in this study. We are very grateful to the staff of the Laboratório de Cultura de Tecidos e Citogenética, Instituto Evandro Chagas, and to the Wellcome Trust, CNPq (309699/2015-0), PROPESP-UFPA and CAPES for technical and financial support. We also are grateful to Mr. Alex Araújo for the artwork for Figure 5. Finally, we would like to thank the reviewers for their helpful comments.
Conflicts of Interest
The authors declare that they have no conflict of interest.
References
- Hackett, S.J.; Kimball, R.T.; Reddy, S.; Bowie, R.C.; Braun, E.L.; Braun, M.J.; Chojnowski, J.L.; Cox, W.A.; Han, K.L.; Harshman, J. A phylogenomic study of birds reveals their evolutionary history. Science 2008, 320, 1763–1768. [Google Scholar] [CrossRef]
- Prum, R.O.; Berv, J.S.; Dornburg, A.; Field, D.J.; Townsend, J.P.; Lemmon, E.M.; Lemmon, A.R. A comprehensive phylogeny of birds (Aves) using targeted next-generation DNA sequencing. Nature 2015, 526, 569–573. [Google Scholar] [CrossRef]
- Livezey, B.C. A phylogenetic analysis of the Gruiformes (Aves) based on morphological characters, with an emphasis on the rails (Rallidae). Philos. Trans. R. Soc. Lond. B Biol. Sci. 1998, 353, 2077–2151. [Google Scholar] [CrossRef]
- Fain, M.G.; Krajewski, C.; Houde, P. Phylogeny of ‘‘core Gruiformes’’ (Aves: Grues) and resolution of the Limpkin–Sungrebe problem. Mol. Phylogenet. Evol. 2007, 43, 515–529. [Google Scholar] [CrossRef]
- Garcia-R, J.C.; Gibb, G.C.; Trewick, S.A. Deep global evolutionary radiation in birds: Diversification and trait evolution in the cosmopolitan bird family Rallidae. Mol. Phylogenet. Evol. 2014, 81, 96–108. [Google Scholar] [CrossRef]
- Hammar, B. The karyotypes of thirty-one birds. Hereditas 1970, 65, 29–58. [Google Scholar] [CrossRef]
- Giannoni, M.L.; Giannoni, M.A. Cytogenetic analysis of the species Porzana albicollis (Saracura-sanã, or Sora). Rev. Bras. Genet. 1983, 4, 649–665. [Google Scholar]
- Gunski, R.J.; Kretschmer, R.; Souza, M.S.; Furo, I.O.; Barcellos, S.A.; Costa, A.L.; Cioffi, M.B.; de Oliveira, E.H.C.; Garnero, A.D.V. Evolution of Bird Sex Chromosomes Narrated by Repetitive Sequences: Unusual W Chromosome Enlargement in Gallinula melanops (Aves: Gruiformes: Rallidae). Cytogenet. Genome Res. 2019, 158, 152–159. [Google Scholar] [CrossRef]
- Furo, I.O.; Kretschmer, R.; O’Brien, P.C.M.; Ferguson-Smith, M.A.; de Oliveira, E.H.C. Chromosomal Diversity and Karyotype Evolution in South American macaws (Psittaciformes, Psittacidae). PLoS ONE 2015, 10, e0130157. [Google Scholar]
- Furo, I.O.; Monte, A.A.; dos Santos, M.S.; Tagliarini, M.M.; O’Brien, P.C.M.; Ferguson-Smith, M.A.; de Oliveira, E.H. Cytotaxonomy of Eurypyga helias (Gruiformes, Eurypygidae): First karyotypic description and phylogenetic proximity with Rynochetidae. PLoS ONE 2015, 10, e0143982. [Google Scholar] [CrossRef] [Green Version]
- Furo, I.D.O.; Kretschmer, R.; O’Brien, P.C.M.; Pereira, J.C.; Garnero, A.D.V.; Gunski, R.J.; Ferguson-Smith, M.A.; de Oliveira, E.H.C. Chromosome Painting in Neotropical Long- and Short-Tailed Parrots (Aves, Psittaciformes): Phylogeny and Proposal for a Putative Ancestral Karyotype for Tribe Arini. Genes 2018, 9, 491. [Google Scholar] [CrossRef] [Green Version]
- Rodrigues, B.S.; de Assis, M.F.L.; O’Brien, P.C.M.; Ferguson-Smith, M.A.; de Oliveira, E.H.C. Chromosomal studies on Coscoroba coscoroba (Aves: Anseriformes) reinforce the Coscoroba–Cereopsis clade. Biol. J. Linn. Soc. Lond. 2014, 111, 274–279. [Google Scholar] [CrossRef] [Green Version]
- Kretschmer, R.; de Oliveira, E.H.C.; dos Santos, M.S.; Furo, I.O.; O’Brien, P.C.M.; Ferguson-Smith, M.A.; Garnero, A.D.V.; Gunski, R.J. Chromosome mapping of the large elaenia (Elaenia spectabilis): Evidence for a cytogenetic signature for passeriform birds? Biol. J. Linn. Soc. Lond. 2015, 115, 391–398. [Google Scholar] [CrossRef] [Green Version]
- Nie, W.; O’Brien, P.C.M.; Ng, B.L.; Fu, B.; Volobouev, V.; Carter, N.P.; Ferguson-Smith, M.A.; Yang, F. Avian comparative genomics: reciprocal chromosome painting between domestic chicken (Gallus gallus) and the stone curlew (Burhinus oedicnemus, Charadriiformes)—An atypical species with low diploid number. Chromosome Res. 2009, 17, 99–113. [Google Scholar] [CrossRef] [Green Version]
- de Oliveira, E.H.C.; Tagliarini, M.M.; Rissino, J.D.; Pieczarka, J.C.; Nagamachi, C.Y.; O’Brien, P.C.M.; Ferguson-Smith, M.A. Reciprocal chromosome painting between white hawk (Leucopternis albicollis) and chicken reveals extensive fusions and fissions during karyotype evolution of accipitridae (Aves, Falconiformes). Chromosome Res. 2010, 18, 349–355. [Google Scholar] [CrossRef]
- Kretschmer, R.; Ferguson-Smith, M.A.; de Oliveira, E.H.C. Karyotype evolution in birds: from conventional staining to chromosome painting. Genes 2018, 9, 181. [Google Scholar] [CrossRef] [Green Version]
- Nanda, I.; Benisch, P.; Fetting, D.; Haaf, T.; Schmid, M. Synteny Conservation of Chicken Macrochromosomes 1–10 in Different Avian Lineages Revealed by Cross-Species Chromosome Painting. Cytogenet. Genome Res. 2011, 132, 165–181. [Google Scholar] [CrossRef]
- Sasaki, M.; Ikeuchi, T.; Makino, S. A feather pulp culture technique for avian chromosomes, with notes on the chromosomes of the peafowl and the ostrich. Experientia 1968, 24, 1292–1293. [Google Scholar] [CrossRef]
- Telenius, H.; Ponder, B.A.J.; Tunnacliffe, A.; Pelmear, A.H.; Carter, N.P.; Ferguson-Smith, M.A.; Behmel, A.; Nordenskjöld, M.; Pfragner, R. Cytogenetic analysis by chromosome painting using DOP-PCR amplified flow-sorted chromosomes. Genes Chromosomes Cancer 1992, 4, 257–263. [Google Scholar] [CrossRef]
- Christidis, L. The Quarterly Review of Biology; Gebrüder Borntraeger: Berlin, Germany, 1990; pp. 88–108. [Google Scholar]
- Shibusawa, M.; Nishibori, M.; Nishida-Umehara, C.; Tsudzuk, M.; Masaband, J.; Griffin, D.K.; Matsuda, Y. Karyotypic evolution in the Galliformes: An examination of the process of karyotypic evolution by comparison of the molecular cytogenetic findings with the molecular phylogeny. Cytogenet. Genome Res. 2004, 106, 111–119. [Google Scholar] [CrossRef]
- De Oliveira, E.H.; de Moura, S.P.; dos Anjos, L.J.; Nagamachi, C.Y.; Pieczarka, J.C.; O’Brien, P.C.; Ferguson-Smith, M.A. Comparative chromosome painting between chicken and spectacled owl (Pulsatrix perspicillata): Implications for chromosomal evolution in the Strigidae (Aves, Strigiformes). Cytogenet. Genome Res. 2008, 122, 157–162. [Google Scholar] [CrossRef]
- Degrandi, T.M.; Garnero, A.D.V.; O’Brien, P.C.M.; Ferguson-Smith, M.A.; Kretschmer, R.; de Oliveira, E.H.C.; Gunski, R.J. Chromosome Painting in Trogon s. surrucura (Aves, Trogoniformes) Reveals a Karyotype Derived by Chromosomal Fissions, Fusions, and Inversions. Cytogenet. Genome Res. 2017, 151, 208–215. [Google Scholar] [CrossRef]
- Nanda, I.; Karl, E.; Griffin, D.K.; Schartl, M.; Schmid, M. Chromosome repatterning in three representative parrots (Psittaciformes) inferred from comparative chromosome painting. Cytogenet. Genome Res. 2007, 117, 43–53. [Google Scholar] [CrossRef]
- Seabury, C.M.; Dowd, S.E.; Seabury, P.M.; Raudsepp, T.; Brightsmith, D.J.; Liboriussen, P.; Halley, Y.; Fisher, C.A.; Owens, E.; Viswanathan, G.; et al. A multiplatform draft de novo genome assembly and comparative analysis for the Scarlet Macaw (Ara macao). PLoS ONE 2013, 8, e62415. [Google Scholar] [CrossRef] [Green Version]
- Seibold-Torres, C.; Owens, E.; Chowdhary, R.; Ferguson-Smith, M.A.; Tizard, I.; Raudsepp, T. Comparative Cytogenetics of the Congo African Grey Parrot (Psittacus erithacus). Cytogenet. Genome Res. 2015, 147, 144–153. [Google Scholar] [CrossRef]
- Volker, M.; Backstrom, N.; Skinner, B.M.; Langley, E.J.; Bunzey, S.K.; Ellegren, H.; Griffin, D.K. Copy number variation, chromosome rearrangement, and their association with recombination during avian evolution. Genome Res. 2010, 20, 503–511. [Google Scholar] [CrossRef] [Green Version]
- Warren, W.C.; Clayton, D.F.; Ellegren, H.; Arnold, A.P.; Hillier, L.W.; Künstner, A.; Searle, S.; White, S.; Vilella, A.J.; Fairley, S.; et al. The genome of a songbird. Nature 2010, 464, 757–762. [Google Scholar] [CrossRef]
- Skinner, B.M.; Griffin, D.K. Intrachromosomal rearrangements in avian genome evolution: Evidence for regions prone to breakpoints. Heredity 2012, 108, 37–41. [Google Scholar] [CrossRef] [Green Version]
- Potter, S.; Bragg, J.G.; Blom, M.P.K.; Deakin, J.E.; Kirkpatrick, M.; Eldridge, M.D.B.; Moritz, C. Chromosomal Speciation in the Genomics Era: Disentangling Phylogenetic Evolution of Rock-wallabies. Front. Genet. 2017, 8, 10. [Google Scholar] [CrossRef]
- Ruan, L.; Wang, Y.; Hu, J.; Ouyang, Y. Polyphyletic origin of the genus Amaurornis inferred from molecular phylogenetic analysis of rails. Biochem. Genet. 2012, 50, 959–966. [Google Scholar] [CrossRef]
- He, K.; Ren, T.; Zhu, S.; Zhao, A. The complete mitochondrial genome of Fulica atra (Avian, Gruiformes, Rallidae). Mitochondrial DNA A DNA Mapp. Seq. Anal. 2016, 27, 3161–3162. [Google Scholar] [CrossRef]
Figure 1.
Partial karyotypes (pair 1–10 and ZW) of (A) Aramides cajaneus (2n = 78) and (B) Psophia viridis (2n = 80) (from pair 11 on, chromosomes correspond to indistinguishable microchromosomes, with the same size and morphology; for this reason, only the macrochromosomes are shown).
Figure 1.
Partial karyotypes (pair 1–10 and ZW) of (A) Aramides cajaneus (2n = 78) and (B) Psophia viridis (2n = 80) (from pair 11 on, chromosomes correspond to indistinguishable microchromosomes, with the same size and morphology; for this reason, only the macrochromosomes are shown).
Figure 2.
Experiments of chromosome painting using G. gallus probes in metaphases of Aramides cajaneus. (A,B) Examples of conserved syntenic groups (GGA1 and GGA2); (C,D) Examples of rearranged syntenic groups, showing an association between GGA5/ GGA7 on ACA4.
Figure 2.
Experiments of chromosome painting using G. gallus probes in metaphases of Aramides cajaneus. (A,B) Examples of conserved syntenic groups (GGA1 and GGA2); (C,D) Examples of rearranged syntenic groups, showing an association between GGA5/ GGA7 on ACA4.
Figure 3.
Representative examples of chromosome painting using macrochromosomes of G. gallus in Psophia viridis: GGA2 (A), GGA3 (B), GGA5 (C) and GGA 9 (D). The large pink fluorescence area on the top left corner of the (C) represent signals produced by the probes in interphase nucleus.
Figure 3.
Representative examples of chromosome painting using macrochromosomes of G. gallus in Psophia viridis: GGA2 (A), GGA3 (B), GGA5 (C) and GGA 9 (D). The large pink fluorescence area on the top left corner of the (C) represent signals produced by the probes in interphase nucleus.
Figure 4.
Homology maps with GGA probes in (A) Aramides cajaneus and (B) Psophia viridis.
Figure 5.
Schematic representation of chromosome rearrangements during evolution of the Gruiformes based on comparative chromosome painting and literature results (Nanda et al., 2011). We propose that the A. cajaneus would be more basal within the Rallidae family and P. viridis close to F. atra and G. chloropus. Legend: Fulica atra (FAT), Aramides cajaneus (ACA), Gallinula chloropus (GCH), Psophia viridis (PVI), Gallus gallus (GGA).
Figure 5.
Schematic representation of chromosome rearrangements during evolution of the Gruiformes based on comparative chromosome painting and literature results (Nanda et al., 2011). We propose that the A. cajaneus would be more basal within the Rallidae family and P. viridis close to F. atra and G. chloropus. Legend: Fulica atra (FAT), Aramides cajaneus (ACA), Gallinula chloropus (GCH), Psophia viridis (PVI), Gallus gallus (GGA).
Table 1.
Chromosomal homologies among Gruiformes species and Gallus gallus (GGA1-10).
| Chicken Chromosome Paint Number | F. atra, FAT, 2n = 92 [17] | G. chloropus, GCH, 2n = 78 [17] | A. cajaneus, ACA, 2n = 78 (Present Study) | P. viridis, PVI, 2n = 80 (Present Study) |
|---|---|---|---|---|
| GGA1 | FAT1 | GCH1 | ACA1 | PVI1 |
| GGA2 | FAT2 | GCH2 | ACA2 | PVI2 |
| GGA3 | FAT3 | GCH3 | ACA3 | PVI3 |
| GGA4q | FAT4p | GCH4p | ACA5 | PVI5 |
| GGA5 | FAT4q, FAT12 | GCH4q, GCH12 | ACA4q | PVI6 |
| GGA6 | FAT5q | GCH5q | ACA6 | PVI4q |
| GGA7 | FAT5p | GCH5p | ACA4p | PVI4p |
| GGA8 | FAT6 | GCH6 | ACA8 | PVI7 |
| GGA9 | FAT8 | GCH8 | ACA9 | PVI8 |
| GGA4p | FAT7, FAT13 | GCH7, GCH13 | ACA7 | PVI9, PVI11 |
| GGA10 | FAT9 | GCH9 | ACA10 | PVI9 |
Table 2.
Chromosomal rearrangements observed in Gruiformes, according to comparative chromosome painting with G. gallus probes.
Table 2.
Chromosomal rearrangements observed in Gruiformes, according to comparative chromosome painting with G. gallus probes.
| Family | Species | Rearrangements (GGA) | References | ||||
|---|---|---|---|---|---|---|---|
| Associations | Fission | ||||||
| GGA6/7 | GGA5/7 | GGA4 (2 pairs) | GGA4 (3 pairs) | GGA5 | |||
| Psophiidae | Psophia viridis | * | * | Present study | |||
| Rallidae | Aramides cajaneus | * | * | Present study | |||
| Rallidae | Fulica atra | * | * | * | [17] | ||
| Rallidae | Gallinula chloropus | * | * | * | [17] | ||
The presence of the rearrangement is indicated by *.
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Furo, I.d.O.; Kretschmer, R.; O’Brien, P.C.M.; Pereira, J.C.; Ferguson-Smith, M.A.; de Oliveira, E.H.C. Phylogenetic Analysis and Karyotype Evolution in Two Species of Core Gruiformes: Aramides cajaneus and Psophia viridis. Genes 2020, 11, 307. https://doi.org/10.3390/genes11030307
AMA Style
Furo IdO, Kretschmer R, O’Brien PCM, Pereira JC, Ferguson-Smith MA, de Oliveira EHC. Phylogenetic Analysis and Karyotype Evolution in Two Species of Core Gruiformes: Aramides cajaneus and Psophia viridis. Genes. 2020; 11(3):307. https://doi.org/10.3390/genes11030307
Chicago/Turabian StyleFuro, Ivanete de Oliveira, Rafael Kretschmer, Patrícia C. M. O’Brien, Jorge C. Pereira, Malcolm A. Ferguson-Smith, and Edivaldo Herculano Corrêa de Oliveira. 2020. "Phylogenetic Analysis and Karyotype Evolution in Two Species of Core Gruiformes: Aramides cajaneus and Psophia viridis" Genes 11, no. 3: 307. https://doi.org/10.3390/genes11030307
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