Cytogenetic characterization of Partamona cupira (Hymenoptera, Apidae) by fluorochromes

Marthe, Jefferson de Brito; Pompolo, Silvia das Graças; Campos, Lucio Antônio de Oliveira; Salomão, Tânia Maria Fernandes; Tavares, Mara Garcia

doi:10.1590/S1415-47572010005000029

Abstract

Four colonies of the stingless bee Partamona cupira (Hymenoptera: Apidae) were cytogenetically analyzed using conventional staining and the fluorochromes CMA3 e DAPI. The females have 2n = 34 chromosomes (2K=32<img border=0 src="../../../../../../../img/revistas/gmb/2010nahead/ah06a04CarM.gif" align=absmiddle>+2<img border=0 src="../../../../../../../img/revistas/gmb/2010nahead/ah06a04CarA.gif" align=absmiddle>). Some females, however, presented an additional large B acrocentric chromosome, to a total of 2n = 35. Chromosome B and the chromosomal pairs 2, 9 and 10 showed CMA3+ bands, indicating an excess of CG base-pairs. A clear association was verified between the P. helleri B chromosome SCAR marker and the presence of a B chromosome in P. cupira. The data obtained suggests that B chromosomes in P. helleri and P. cupira share a common origin.

B chromosome; SCAR; stingless bees

ANIMAL GENETICS

SHORT COMMUNICATION

Cytogenetic characterization of Partamona cupira (Hymenoptera, Apidae) by fluorochromes

Jefferson de Brito Marthe; Silvia das Graças Pompolo; Lucio Antônio de Oliveira Campos; Tânia Maria Fernandes Salomão; Mara Garcia Tavares

Departamento de Biologia Geral, Universidade Federal de Viçosa, Viçosa, MG, Brazil

^{Send correspondence to} Send correspondence to: Mara Garcia Tavares Departamento de Biologia Geral, Universidade Federal de Viçosa 36570-000 Viçosa, MG, Brazil E-mail: mtavares@ufv.br.

ABSTRACT

Four colonies of the stingless bee Partamona cupira (Hymenoptera: Apidae) were cytogenetically analyzed using conventional staining and the fluorochromes CMA₃e DAPI. The females have 2n = 34 chromosomes (2K=32+2). Some females, however, presented an additional large B acrocentric chromosome, to a total of 2n = 35. Chromosome B and the chromosomal pairs 2, 9 and 10 showed CMA₃⁺bands, indicating an excess of CG base-pairs. A clear association was verified between the P. helleri B chromosome SCAR marker and the presence of a B chromosome in P. cupira. The data obtained suggests that B chromosomes in P. helleri and P. cupira share a common origin.

Key words: B chromosome, SCAR, stingless bees.

Stingless bees of the genus Partamona (Hymenoptera, Apidae) are widely distributed geographically. Their range extends from the south of Mexico to south Brazil, spreading northwards along the Pacific coast until Peru (Camargo, 1980).

The cytogenetic characterization of eight species of the genus Partamona, viz., P. pearsoni, P. helleri (cited as P. cupira by Costa et al., 1992), P. mulata, P. ailyae, P. vicina, P. sp. aff. nigrior, P. peckolti and P. seridoensis (revision in Brito et al., 2005) showed that all of the females have 2n = 34 chromosomes and that only P. helleri presented 0 to 7 B chromosomes.

B chromosomes of P. helleri were cytogenetically characterized using C, Q and NOR banding, GTG method, CMA3, DAPI and FISH (Brito et al., 2005). Brito et al. (2005) concluded that P. helleri B chromosomes are heterochromatic. Genomic DNA treatment with the EcoRI restriction enzyme, and Southern blot analysis using an 18S rDNA probe from maize, demonstrated that individuals with B chromosomes displayed bands which were not present in individuals that did not bear this chromosome (RM Brito and SG Pompolo, unpublished data). Thus, the presence of specific sequences in the B chromosomes of this species can be suggested.

Using molecular techniques, Tosta et al. (2004) identified one RAPD marker in B chromosome-bearing individuals of P. helleri. This RAPD marker was cloned, sequenced and then transformed into a SCAR marker (Tosta et al., 2007). Further on, the presence of this SCAR marker was noted in P. cupira and P. criptica (VC Tosta, personal communication).

Considering that in P. helleri the SCAR marker is present exclusively in individuals possessing B chromosomes, and that this marker was also identified in P. cupira, the aim of this study was to cytogenetically characterize the latter species, to check for the presence of B chromosomes. As the presence of a B chromosome was detected in some individuals of P. cupira, an additional molecular analysis was carried out by using the SCAR marker previously described, in order to check whether there is an association between this sequence and the presence of B chromosomes in this species.

The cytogenetic analyses were carried out with 19, 17, 21 and 11 post-defecating larvae from four Partamona cupira colonies (GUI 1, GUI 2, GUI 3 and GUI 11) collected at Guimarânia (18º50'38" S, 46º47'35''W), State of Minas Gerais. Metaphasic chromosomes were obtained from P. cupira cerebral ganglia according to Imai et al. (1988). The remaining parts of each larva were frozen in an ultra-low temperature freezer at -80 ºC, to be subsequently used for DNA analysis. After 24 h, the slides were stained with Giemsa diluted in Sorensen's buffer for 20 min at room temperature.

Sequential staining was performed with the use of the fluorochromes: Distamycin/Chromomycin A₃ (DA/CMA₃) and Distamycin/4, 6-diamine-2-phenylindole (DA/DAPI) (Schweizer, 1980).

An average of 10 metaphases per specimen was observed. The best images were selected and captured with a Q Color 30 Olympus camera coupled to an Olympus BX-60 microscope. In order to obtain the metaphase images of slides treated with DA/CMA₃, the WB (l = 330 to 385 nm) filter was used; for DA/DAPI, the WU filter (l = 450-480 nm) was used.

Chromosomes were classified according to Imai (1991) and the karyotypes were mounted using Corel Photo-Paint from CorelDraw X3 and Adobe Photoshop 7.0 softwares.

For the molecular analyses, the larval DNA was obtained according to Waldschmidt et al. (1997) and amplified by using SCAR primers specific for P. helleri B chromosomes (Tosta et al., 2007). PCR products were separated by electrophoresis in 1% agarose gels in TBE (90 mM Tris-borate pH 8.0, 10 mM EDTA) buffer, stained with ethidium bromide (0.2 µg/mL) and visualized under UV light with AlphaDigiDoc 1201 software.

A comparison between the presence of SCAR marker and the presence of B chromosome in the studied individuals was carried out after the analyses of the gels.

The cytogenetic analyses revealed that P. cupira possesses 2n = 34 chromosomes (Figure 1A). The diploid karyotype is comprised of 5 metacentric, 11 submetacentric and a single pair of acrocentric chromosomes, or 2K=32+2, according to the nomenclature proposed by Imai (1991), whereby may include metacentric and submetacentric chromosomes, and acrocentric and telocentric ones. Partamona cupira, therefore, presented the same chromosome number as other species of the same genus that had already been cytogenetically studied (Costa et al., 1992; Brito et al., 1997, 2003, 2005; Brito-Ribon et al., 1999; Tosta et al., 2004). Nevertheless, an analysis of chromosome morphology demonstrated that the P. cupira karyotype is different from that of P. helleri and P. seridoensis (Brito et al., 2005). Partamona helleri and P. seridoensis have only metacentric chromosomes (M), whereas the species studied herein have acrocentric (A) and metacentric chromosomes.

The obtained data also revealed that, in addition to the regular chromosomal complement, some individuals of P. cupira (10 individuals of the GUI 1 colony and 3 individuals of GUI 11) possessed one B chromosome (Figure 1B). These individuals, therefore, had 2n = 35 chromosomes. This B chromosome was considerably larger when compared to those found in P. helleri (Costa et al., 1992; Tosta et al., 2004), and in two other species of stingless bees, Melipona quinquefasciata (Pompolo, 1992) and M. rufiventris (Lopes et al., 2008).

DA/DAPI staining did not reveal the presence of fluorescent bands in any chromosome. DA/CMA₃ staining, in turn, revealed bands in the terminal portions of the chromosome pairs 2, 9 and 10, as well as on the short arm of the B chromosome, thus demonstrating the existence of repetitive sequences rich in CG in these regions (Figure 1C). These same chromosomes, plus chromosome pair 15, presented CMA3 positive bands in P. helleri and P. seridoensis (Brito et al., 2005). The difference in the number of chromosomes stained by DA/CMA₃, as observed in P. cupira, and P. helleri/P. seridoensis, may be related to a process of chromosome evolution. Nevertheless, confirmation requires further comparative studies. Furthermore, Brito et al. (2005), using an in situ hybridization assay noted that the chromosome pairs 2, 9, 10 and 15 carried cistrons for ribosomal RNA in P. helleri and P. seridoensis. An association between CMA₃ bands and the presence of ribosomal DNA sequence sites in the same chromosomal region, had already been observed in other species of Hymenoptera, such as Trypoxylon albitarse (Araújo et al., 2000), Melipona asilvae (Rocha et al., 2002) and Partamona peckolti (Brito et al., 2003). Thus, it is possible that the CMA₃ positive regions observed in P. cupira may be related to rDNA genes.

Molecular analysis revealed a correspondence of the SCAR marker specific for P. helleri B chromosomes, and the presence of B chromosomes in P. cupira, since in all B-chromosome-bearing individuals in the colonies GUI 1 and GUI 11, the band corresponding to the SCAR marker specific for P. helleri B chromosomes was also observed (Figure 2). Moreover, the presence of this marker was not observed in individuals lacking B chromosomes.

The origins of these B chromosomes and their effects on the bearers, although well discussed (López-León et al., 1994; Gutknecht et al., 1995; MacAllister and Werren, 1997; Camacho et al., 2000; Araujo et al., 2001), are far from clear. However, the sequence of the P. helleri SCAR marker and that of P. cupira, P. criptica and P. rustica showed a high degree of similarity (data not shown). This, together with the association of this marker to the presence of the B chromosome in P. cupira, as demonstrated herein, implies that P. cupira B chromosomes may have the same origin as those of P. helleri, and that P. rustica and P. criptica may also posses B chromosomes, although the latter have not yet been characterized cytogenetically. These analyses may clarify the origin of B chromosomes in the genus Partamona.

Acknowledgments

We are grateful to the Fundação de Amparo à Pesquisa do Estado de Minas Gerais (FAPEMIG), Conselho Nacional de Pesquisa e Desenvolvimento Tecnológico (CNPq), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) and the Universidade Federal de Viçosa (UFV) for financial support. We also wish to thank Margarete do Valle Werneck, Íris Raimundo Stanciola and Geraldo Paiva for help with bee collecting.

Received: May 27, 2009; Accepted: November 3, 2009.

Associate Editor: Yatiyo Yonegaga-Yassuda

License information: This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Araújo SMR, Pompolo SG, Dergam JA and Campos LAO (2000) The B chromosome system of Tripoxylon (Trypargilum) albitarse (Hymenoptera, Sphecidae). 1. Banding analysis. Cytobios 101:7-13.
Araújo SMR, Pompolo SG, Perfectti F and Camacho JPM (2001) Integration of a B chromosome into the genome of a wasp. Proc R Soc Lond 268:1127-1131.
Brito RM, Costa MA and Pompolo SG (1997) Characterization and distribution of supernumerary chromosomes in 23 colonies of Partamona helleri (Hymenoptera, Apidae, Meliponinae). Braz J Genet 20:185-188.
Brito RM, Caixeiro APA, Pompolo SG and Azevedo GG (2003) Cytogenetic data of Partamona peckolti (Hymenoptera, Apidae, Meliponini) by C banding and fluorochrome staining with DA/CMA3, And DA/DAPI. Genet Mol Biol 26:53-57.
Brito RM, Pompolo SG, Martins MF, Barros EG and Saka-moto-Hojo ET (2005) Cytogenetic characterization of two Partamona species (Hymenoptera, Apinae, Meliponini) by fluorochrome staining and localization of 18 rDNA clusters by FISH. Cytologia 70:373-380.
Brito-Ribon M, Miyazawa CS and Pompolo SG (1999) First karyotype characterization of four species of Partamona (Friese, 1980) (Hymenoptera, Apidae, Meliponinae) in Mato Grosso State, Brazil. Cytobios 100:19-26.
Camacho JPM, Sharbel TF and Beukeboom LW (2000) B-chromosome evolution. Phil Trans R Soc Lond 355:163-178.
Camargo JMF (1980) O grupo Partamona (Partamona) testacea (Klug): Suas espécies, distribuição e diferenciação geográfica (Meliponinae, Apidae, Hymenoptera). Acta Amazonica 4:7-175 (Abstract in English).
Costa MA, Pompolo SG and Campos LAO (1992) Supernumerary chromosomes in Partamona cupira (Hymenoptera, Apidae, Meliponinae). Rev Bras Genet 15:801-806.
Gutknecht J, Sperlich D and Bachmann LA (1995) A species specific satellite DNA family of Drosophila subsilvestris appearing predominantely in B chromosomes. Chromosoma 103:533-544.
Imai HT (1991) Mutability of constitutive heterochromatin (Cbands) during eukaryotic chromosomal evolution and their cytological meaning. Jpn J Genet 66:635-661.
Imai HT, Taylor RW and Crozier RH (1988) Modes of spontaneous chromosomal mutation and karyotype evolution in ants with reference to the minimum interaction hypothesis. Jpn J Genet 63:159-185.
MacAllister BF and Werren JH (1997) Hybrid origin of a B chromosome (PSR) in the parasitic wasp Nasonia vitripennis Chromosoma 106:243-253.
Lopes DM, Pompolo SG, Tavares MG and Campos LAO (2008) Cytogenetic characterization of Melipona rufiventris Lepeletier 1836 and Melipona mondury Smith 1863 (Hymenoptera, Apidae) by C banding and fluorochromes. Genet Mol Biol 31:49-52.
Lopez-León MD, Neves D, Schwarzacher T, Heslop-Harrison TS, Hewitt GM and Camacho JPM (1994) Possible origin of a B chromosome deduced from its DNA composition using double FISH technique. Chromosome Res 2:87-92.
Pompolo SG (1992) Estudos citogenéticos em Meliponinae. Naturalia (special issue):62-66.
Rocha MP, Pompolo SG, Dergam JA, Fernandes A and Campos LAO (2002) DNA characterization and karyotypic evolution in the bee genus Melipona (Hymenoptera, Meliponini). Hereditas 136:19-27.
Schweizer D (1980) Simultaneous fluorescent staining of R bands in a specific heterochromatin regions (DA/DAPI - bands) in human chromosomes. Cytogenet Cell Genet 27:190-193.
Tosta VC, Tavares MG, Fernandes A, Barros EG, Campos LAO and Camacho JPM (2004) A RAPD marker associated with B chromosomes in Partamona helleri (Hymenoptera, Apidae). Cytogenet Genet Res 106:279-283.
Tosta VC, Tavares MG, Fernandes A, Barros EG, Campos LAO and Camacho JPM (2007) Development of a SCAR marker for the analysis of B chromosome presence in Partamona helleri (Hymenoptera, Apidae). Cytogenet Genome Res 116:127-129.
Waldschmidt AM, Salomão TMF, Barros EG and Campos LAO (1997) Extraction of genomic DNA from Melipona quadrifasciata (Hymenoptera, Apidae, Meliponinae). Braz J Genet 20:421-423.

Send correspondence to:

Mara Garcia Tavares

Departamento de Biologia Geral, Universidade Federal de Viçosa

36570-000 Viçosa, MG, Brazil

E-mail:

mtavares@ufv.br.

Publication Dates

Publication in this collection
02 Apr 2010
Date of issue
2010

History

Received
27 May 2009
Accepted
03 Nov 2009

This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License.

[1] Araújo SMR, Pompolo SG, Dergam JA and Campos LAO (2000) The B chromosome system of Tripoxylon (Trypargilum) albitarse (Hymenoptera, Sphecidae). 1. Banding analysis. Cytobios 101:7-13.

[2] Araújo SMR, Pompolo SG, Perfectti F and Camacho JPM (2001) Integration of a B chromosome into the genome of a wasp. Proc R Soc Lond 268:1127-1131.

[3] Brito RM, Costa MA and Pompolo SG (1997) Characterization and distribution of supernumerary chromosomes in 23 colonies of Partamona helleri (Hymenoptera, Apidae, Meliponinae). Braz J Genet 20:185-188.

[4] Brito RM, Caixeiro APA, Pompolo SG and Azevedo GG (2003) Cytogenetic data of Partamona peckolti (Hymenoptera, Apidae, Meliponini) by C banding and fluorochrome staining with DA/CMA3, And DA/DAPI. Genet Mol Biol 26:53-57.

[5] Brito RM, Pompolo SG, Martins MF, Barros EG and Saka-moto-Hojo ET (2005) Cytogenetic characterization of two Partamona species (Hymenoptera, Apinae, Meliponini) by fluorochrome staining and localization of 18 rDNA clusters by FISH. Cytologia 70:373-380.

[6] Brito-Ribon M, Miyazawa CS and Pompolo SG (1999) First karyotype characterization of four species of Partamona (Friese, 1980) (Hymenoptera, Apidae, Meliponinae) in Mato Grosso State, Brazil. Cytobios 100:19-26.

[7] Camacho JPM, Sharbel TF and Beukeboom LW (2000) B-chromosome evolution. Phil Trans R Soc Lond 355:163-178.

[8] Camargo JMF (1980) O grupo Partamona (Partamona) testacea (Klug): Suas espécies, distribuição e diferenciação geográfica (Meliponinae, Apidae, Hymenoptera). Acta Amazonica 4:7-175 (Abstract in English).

[9] Costa MA, Pompolo SG and Campos LAO (1992) Supernumerary chromosomes in Partamona cupira (Hymenoptera, Apidae, Meliponinae). Rev Bras Genet 15:801-806.

[10] Gutknecht J, Sperlich D and Bachmann LA (1995) A species specific satellite DNA family of Drosophila subsilvestris appearing predominantely in B chromosomes. Chromosoma 103:533-544.

[11] Imai HT (1991) Mutability of constitutive heterochromatin (Cbands) during eukaryotic chromosomal evolution and their cytological meaning. Jpn J Genet 66:635-661.

[12] Imai HT, Taylor RW and Crozier RH (1988) Modes of spontaneous chromosomal mutation and karyotype evolution in ants with reference to the minimum interaction hypothesis. Jpn J Genet 63:159-185.

[13] MacAllister BF and Werren JH (1997) Hybrid origin of a B chromosome (PSR) in the parasitic wasp Nasonia vitripennis Chromosoma 106:243-253.

[14] Lopes DM, Pompolo SG, Tavares MG and Campos LAO (2008) Cytogenetic characterization of Melipona rufiventris Lepeletier 1836 and Melipona mondury Smith 1863 (Hymenoptera, Apidae) by C banding and fluorochromes. Genet Mol Biol 31:49-52.

[15] Lopez-León MD, Neves D, Schwarzacher T, Heslop-Harrison TS, Hewitt GM and Camacho JPM (1994) Possible origin of a B chromosome deduced from its DNA composition using double FISH technique. Chromosome Res 2:87-92.

[16] Pompolo SG (1992) Estudos citogenéticos em Meliponinae. Naturalia (special issue):62-66.

[17] Rocha MP, Pompolo SG, Dergam JA, Fernandes A and Campos LAO (2002) DNA characterization and karyotypic evolution in the bee genus Melipona (Hymenoptera, Meliponini). Hereditas 136:19-27.

[18] Schweizer D (1980) Simultaneous fluorescent staining of R bands in a specific heterochromatin regions (DA/DAPI - bands) in human chromosomes. Cytogenet Cell Genet 27:190-193.

[19] Tosta VC, Tavares MG, Fernandes A, Barros EG, Campos LAO and Camacho JPM (2004) A RAPD marker associated with B chromosomes in Partamona helleri (Hymenoptera, Apidae). Cytogenet Genet Res 106:279-283.

[20] Tosta VC, Tavares MG, Fernandes A, Barros EG, Campos LAO and Camacho JPM (2007) Development of a SCAR marker for the analysis of B chromosome presence in Partamona helleri (Hymenoptera, Apidae). Cytogenet Genome Res 116:127-129.

[21] Waldschmidt AM, Salomão TMF, Barros EG and Campos LAO (1997) Extraction of genomic DNA from Melipona quadrifasciata (Hymenoptera, Apidae, Meliponinae). Braz J Genet 20:421-423.

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