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Assessment of EST-SSR markers for genetic analisys on coffee

Potencial de marcadores EST-SSR para análise genética em café

Abstracts

EST-SSR markers were used to investigate the genetic diversity among and within coffee populations, to explore the possibility of their use for fingerprinting of cultivars and to assist breeding programs. Seventeen markers, developed from ESTs (Expressed Sequence Tags) from the Brazilian Coffee Genome Project, were used. All markers showed polymorphism among the genotypes assessed. The average number of allele per primer was 5.1. The highest polymorphisms were found within C. canephora (88.2%) and rust-resistant varieties (35.3%). About 29.4% of the markers differentiated C. arabica from Híbrido de Timor; it was also possible to identify those closest and farthest from C. arabica . The analysis of population-grouped genotypes revealed a 64.0% genetic diversity among and a 36.0% genetic diversity within populations. The differentiation index was 0.637. Six markers distinguished four rust-resistance varieties, showing their fingerprinting potential. These results demonstrate the usefulness of EST-SSR markers for cross orientation, in diversity and introgression studies, and in genetic mapping.

DNA markers; Coffea sp.; UPGMA; amova; microsatellite markers


No estudo da diversidade genética entre e dentro de populações de café, foram usados marcadores EST-SSR, visando avaliar seu potencial para identificar cultivares comerciais e assistir programas de melhoramento. Os 17 marcadores utilizados foram desenvolvidos a partir das seqüências ESTs do Projeto Brasileiro do Genoma Café. Em todos os marcadores observou-se polimorfismo entre os genótipos avaliados, com um número médio de 5,1 alelos por primer. Os maiores polimorfismos foram constatados dentro de C. canephora (88,2%) e em variedades resistentes à ferrugem (35,3%). Dos marcadores analisados, 29,4% distinguiram C. arabica dos Híbridos de Timor (HDT), sendo possível identificar os mais próximos e os mais distantes de C. arabica . A análise dos genótipos agrupados por população revelou diversidade genética de 64% entre populações e 36% dentro delas, com um índice de diferenciação de 0,637. Em seis marcadores distinguiram-se quatro variedades resistentes à ferrugem, constando seu potencial para fingerprint. Esses resultados demonstram a utilidade dos EST-SSR para orientações dos cruzamentos e estudos de diversidade, introgressão e mapeamento genético.

Marcadores de DNA; Coffea sp.; UPGMA; AMOVA; marcadores microssatélites


BASIC AREAS

Assessment of EST-SSR markers for genetic analisys on coffee

Potencial de marcadores EST-SSR para análise genética em café

Robson Fernando MissioI; Eveline Teixeira CaixetaI, II, * * Correspondent author. ; Eunize Maciel ZambolimI; Guilherme Ferreira PenaI; Ana Paula RibeiroI; Laércio ZambolimI; Antônio Alves PereiraIII; Ney Sussumu SakiyamaI

IUniversidade Federal de Viçosa, Laboratório de Biotecnologia do Cafeeiro – Biocafé, BIOAGRO, 36570-000 Viçosa (MG) ,Brasil. E-mail: eveline.caixeta@embrapa.br

IIEmpresa Brasileira de Pesquisa Agropecuária (EMBRAPA), Viçosa (MG), Brasil

IIIEmpresa de Pesquisa Agropecuária de Minas Gerais (EPAMIG), Viçosa (MG), Brasil

ABSTRACT

EST-SSR markers were used to investigate the genetic diversity among and within coffee populations, to explore the possibility of their use for fingerprinting of cultivars and to assist breeding programs. Seventeen markers, developed from ESTs (Expressed Sequence Tags) from the Brazilian Coffee Genome Project, were used. All markers showed polymorphism among the genotypes assessed. The average number of allele per primer was 5.1. The highest polymorphisms were found within C. canephora (88.2%) and rust-resistant varieties (35.3%). About 29.4% of the markers differentiated C. arabica from Híbrido de Timor; it was also possible to identify those closest and farthest from C. arabica . The analysis of population-grouped genotypes revealed a 64.0% genetic diversity among and a 36.0% genetic diversity within populations. The differentiation index was 0.637. Six markers distinguished four rust-resistance varieties, showing their fingerprinting potential. These results demonstrate the usefulness of EST-SSR markers for cross orientation, in diversity and introgression studies, and in genetic mapping.

Key words: DNA markers, Coffea sp., UPGMA, amova, microsatellite markers.

RESUMO

No estudo da diversidade genética entre e dentro de populações de café, foram usados marcadores EST-SSR, visando avaliar seu potencial para identificar cultivares comerciais e assistir programas de melhoramento. Os 17 marcadores utilizados foram desenvolvidos a partir das seqüências ESTs do Projeto Brasileiro do Genoma Café. Em todos os marcadores observou-se polimorfismo entre os genótipos avaliados, com um número médio de 5,1 alelos por primer. Os maiores polimorfismos foram constatados dentro de C. canephora (88,2%) e em variedades resistentes à ferrugem (35,3%). Dos marcadores analisados, 29,4% distinguiram C. arabica dos Híbridos de Timor (HDT), sendo possível identificar os mais próximos e os mais distantes de C. arabica . A análise dos genótipos agrupados por população revelou diversidade genética de 64% entre populações e 36% dentro delas, com um índice de diferenciação de 0,637. Em seis marcadores distinguiram-se quatro variedades resistentes à ferrugem, constando seu potencial para fingerprint. Esses resultados demonstram a utilidade dos EST-SSR para orientações dos cruzamentos e estudos de diversidade, introgressão e mapeamento genético.

Palavras-chave: Marcadores de DNA, Coffea sp., UPGMA, AMOVA, marcadores microssatélites.

1. INTRODUCTION

The Coffea genus comprises 103 species, of which Coffea arabica L. is commercially the most important (DAVIS et al., 2006). Genetic breeding for this species is limited, due to its narrow genetic base and susceptibility to the main diseases. Thus, the use of molecular markers for genetic diversity studies, crossings orientation and genetic mapping is particularly useful for breeders. Different types of molecular markers, such as RAPD, AFLP, RFLP and SSR, have been used in coffee genetic studies (LASHERMES et al., 2001, COMBES et al., 2000, TEIXEIRA-CABRAL et al., 2004, DINZ et al., 2005, MALUF et al., 2005). New classes of molecular markers have been developed as a result of genome sequencing projects, such an EST-SSR. EST-SSR are microsatellite markers (SSR) developed from ESTs (Expressed Sequence Tags). With the increasing of ESTs datasets, the SSR identification and primer design are done in time and cost-effective manner.

ESTs are sequenced portions of cDNA that are part of a transcribed region of the genome under certain biological conditions. Therefore, ESTs are relatively conserved region of the genome. Because EST-SSR markers are present in conserved not always sequences it is expected that they are less polymorphic compared to genomic SSRs. The main advantages of EST-SSR are their high transferability among phylogenetically related species and even genera and a probability of being associated with functional regions of the genome (PONCET et al., 2006). This marker has been used for different studies such as for evaluating the genetic diversity of grapevine (SCOTT et al., 2000), sugar cane (CORDEIRO et al., 2003) and coffee (AGGARWAL et al., 2007; PONCET et al., 2006), genetic map integration in soybean (SONG et al., 2004) and genetic mapping of wheat (GAO et al., 2004), potato (FEINGOLD et al., 2005) and cotton (HAN et al., 2006).

The characterization of genetic diversity among accessions in germplasm collections is extremely important for breeding programs. Selecting and assessing genotypes in germplasm with SSR markers may optimize and facilitate breeding processes by separating closely related genotypes, thus increasing the efficiency and orientation of future crossings and genetic studies. The current study aimed to investigate the genetic diversity among and within coffee populations, to explore the possibility of using EST-SSR markers for fingerprinting of cultivars, and to estimate genetic distances between Coffea arabica and Híbrido de Timor genotypes. According to BETTENCOURT (1973), Híbrido de Timor was probably originated from a natural interspecific crossing between C. arabica and C. canephora. This germplasm has been used in breeding programs as a source of resistant genes against rust, anthracnose, bacteriosis and nematodes. This study will be the basis for selecting genitors to built mapping populations and to develop new cultivars in the C. arabica breeding program.

2. MATERIAL AND METHOD

Genetic material

Seventeen accessions were analyzed, including six C. arabica genotypes, five C. canephora genotypes, three Híbrido de Timor ( C. arabica x C. canephora), and three Triploids ( C. arabica x C. racemosa). These accessions belong to the 'Universidade Federal de Viçosa (UFV) / Empresa de Pesquisa Agropecuária de Minas Gerais (EPAMIG)' genetic breeding program. Six commercial varieties of rust-resistant C. arabica were also analyzed (Table 1).

DNA extraction and EST-SSR primer design

DNA was extracted from young leaves, according to the protocol described by DINIZ et al. (2005). DNA quality was analyzed in agarose gel and the quantification was done in a BioRad Smart Spec spectrophotometer. The SSR markers derived from non-redundant EST of the Brazilian Coffee Genome Project. The sequence could not be available due to a confidentiality agreement signed by the institutions involved in this Project. Primers flanking the EST-SSRs were designed using Primer3 (ROZEN and SKALETSKY, 2000) according to the following parameters: primer size ranged 18 to 22 bp (optimum – 20 bp), annealing temperature between 55 and 60ºC (optimum – 57ºC) and amplification product length of 100-300 bp. Seventeen primer pairs were used for the genetic diversity study of the 23 coffee accessions.

PCR amplification and electrophoresis

The PCR amplification was done in a final volume of 20 µL containing 50 ng of DNA, 0.6 units of Taq DNA polymerase, 1x reaction buffer, 1 mM of MgCl2, 150 mM of each dNTPs, and 0,1 mM of each primer. Amplification was done in a thermalcycler using a PCR-touchdown procedure, which consisted of denaturing at 94ºC for 2 min, followed by 13 cycles of denaturing at 94ºC for 30 s, annealing at 67ºC to 55ºC for 30 s, decreasing 1ºC at each cycle, and extension at 72ºC for 30 s. The next 30 cycles consisted of denaturing at 94ºC for 30 s, annealing at 55ºC for 30 s and extension at 72ºC for 30 s followed by a final extension at 72ºC for 8 min. The amplified products were separated on denaturing 6% polyacrylamide gel and visualized by silver staining solution (CRESTE et al., 2001).

Statistical analysis

For data analysis, each band was defined as a single character. The allelic data for all genotypes was scored in the form of binary matrix where 1 represented presence and 0 (zero) absence of bands. The genetic distance for all the pairwise combinations was calculated using Jaccard's similarity coefficient (JACCARD, 1908). A simplified representation of genetic distances was based on a dendrogram obtained from the Unweighted Pair Group Method based on Arithmetic Averages (UPGMA). Thousand bootstrap interations were calculated to test the robustness of the nodes, using the GENES software (CRUZ, 2006).

Genotypes were also grouped into five populations: (1) C. arabica genotypes; (2) C. canephora genotypes; (3) Híbridos de Timor; (4) triploid hybrids; and (5) commercial varieties of rust-resistant C. arabica. The distance and genetic identity matrix were estimated according to Nei's coefficient (NEI, 1978) using PopGene version 1.3 software (YEH and BOYLE, 1997). Analysis of molecular variance (AMOVA) was used to investigate genetic diversity among and within populations (EXCOFFIER et al., 1992), using the GENES software (CRUZ, 2006).

3. RESULTS AND DISCUSSION

The codominance feature of SSR markers was not taken into account in this genetic diversity study. There are difficulties in using the SSR marker as codominant in polyploid genome species such as C. arabica allotetraployd genotypes. This may be explained by limitations in establishing heterozygosis or homozygosis levels in specific locus, given the inability of SSR markers to distinguish alleles from homoeologous chromosome, as well as the possibility of null alleles in polyploids (CORDEIRO et al., 2003).

Polymorphism among and within Coffea genus species

The 17 EST-SSR primer pairs amplified 87 alleles from 23 coffee genotypes, a mean of 5.12 alleles per primer (Table 2). In a genetic diversity study of 28 accessions of C. arabica and C. canephora, MALUF et al. (2005) used 23 SSR primers, 66 alleles amplified, with an average of 2.87 alleles per locus. PONCET et al. (2006) investigated the level of polymorphism in a set of 25 EST-SSR primers in different species of the Coffea genus, and found a mean of 10.5 alleles per locus. These findings demonstrate that the total number of alleles in a population depends highly on its size and genetic constitution assessed.

All of the 17 primers investigated showed polymorphism among the 23 genotypes analyzed. The highest level of polymorphism were found within the C. canephora genotypes (88.2%), and within the six rustresistant commercial varieties of C. arabica (35.3%). The lowest level of polymorphism (11.8%) was found within the C. arabica genotypes (Table 3). The selfing nature and narrow genetic base of C. arabica may explain the low polymorphism found in this species. Furthermore, EST-SSR markers originated from highly conserved genomic regions, which may present lower degree of polymorphism compared to microsatellites originating from genomic libraries (VARSHNEY et al., 2005).

All primer pairs detected genetic differences among C. arabica and C. canephora populations, and among C. canephora and other populations. This might be due mostly to C. canephora species cross-pollination, which results in high genetic variability. About 29.4% of primers differentiated C. arabica from Híbrido de Timor accessions. This finding is extremely relevant for breeding programs that use Híbrido de Timor as the main source of rust resistance. These EST-SSR markers may be used for mapping studies of segregating populations derived from crossings between C. arabica and Híbrido de Timor. EST-SSR may also be used efficiently for the saturation and integration of preexisting genetic maps (TEIXEIRA-CABRAL et al., 2004), particularly facilitating QTL identification and marker-assisted selection (AKAFFOU et al., 2003; COULIBALY et al., 2003).

Five of the rust-resistant commercial varieties derived from crossings between C. arabica and Híbrido de Timor (Table 1). Many selection cycles, aimed at obtaining a higher number of homozygotic loci and maintaining cultivar genetic homogeneity, were undertaken to launch these commercial varieties. However, the primers that were investigated were polymorphic among the rust-resistant commercial varieties and the C. arabica (35.3%) and Híbrido de Timor (47.1%) accessions, indicating the potential of this class of molecular markers in variety identification studies and in genetic fingerprinting.

Six EST-SSR primers (EST-SSR 007, 010, 012, 013, 023, 029) of the 17 analysed differentiated the commercial coffee varieties Catiguá MG2, IAPAR 59, Oeiras MG6851 and Sacramento MG1 (four of six varieties). No primer was able to genetically distinguished Catucai Amarelo 2SL and Obatã Amarelo 4932 from the other varieties. A minor introgression of C. canephora may have contributed to the polymorphism among the rust-resistant cultivars.

Cluster analysis

The dendrogram obtained based on Jaccard's genetic similarity matrix (Figure 1), taking into account all genotypes individually, generated three groups: (I) C. arabica genotypes, the commercial rust-resistant varieties, Híbrido de Timor accessions and triploid genotypes; (II) C. canephora genotypes 'T 3751', 'T 3580', 'Apoatã IAC 2258' and 'Guarini UFV 514'; (III) C. canephora 'Conillon UFV 513'. Group I was subdivided into arbitrary three groups: (a) C. arabica genotypes, Híbrido de Timor accessions and five commercial varieties (Catucai Amarelo 2SL, Obatã Amarelo IAC 4932, Sacramento MG1, Oeiras MG6851 and IAPAR 59); (b) Triploid genotypes; and (c) the Catiguá MG2 variety. The commercial varieties remained genetically closer to C. arabica genotypes. The triploid individuals composed an intermediate group between tetraploid genotypes ( C. arabica , Híbrido de Timor and cultivated varieties) and diploid genotypes (C. canephora).


C. canephora 'T 3751', 'T 3580', 'Apoatã IAC 2258' and 'Guarini UFV 514' belong to the Robusta group, and were genetically grouped closer to the commercial varieties and to the Híbrido de Timor accessions rather than to the 'Conillon UFV 513' group genotype. This may suggest that the rust-resistance genes in commercial varieties result from genomic introgressions of Robusta group genotypes.The dendrogram (Figure 1) made possible to identify the Híbrido de Timor accessions that are closer and more distant from C. arabica genotypes. This data is extremely significant for breeding programs to incorporate one or more C. canephora disease resistance genes, while maintaining the remaining C. arabica traits. In this case, the genetically closest Híbrido de Timor accession to C. arabica should be chosen, as the Híbrido de Timor 'CIFC 1343/269'. On the other hand, genetically divergent genitors are more appropriate if the priority is to increase the genetic base of the breeding program. Thus crossing the most divergent C. arabica genotypes from Híbrido de Timor, as 'CIFC 832/2' and 'CIFC 4106' (Figure 1), is recommended for obtaining new mapping populations.

Analysis of genotypes grouped according to each population (Table 4 and Figure 2) revealed that the commercial varieties and the Híbrido de Timor accesions were genetically highly similar to C. arabica genotypes. The lowest genetic similarity values were found between the Triploid and C. canephora genotypes.


The genetic similarity coefficients for each population are shown in figure 3. The highest genetic similarity coefficients were found within C. arabica (0.94), Híbrido de Timor (0.93) and Triploid genotypes (0.91). C. canephora genotypes showed the lowest genetic similarity coefficient (0.54), which demonstrates the wide genetic variability of this species. Notwithstanding the low polymorphism found within C. arabica , Híbrido de Timor, Triploid and commercial variety populations, the EST-SSR markers used in this study were effective for differentiating these populations.


Genetic diversity among and within the Coffea genus

The genetic diversity study revealed that about 64% of variation was found among populations, and 36% within these populations (Table 5). SILVEIRA et al. (2003), in a genetic diversity study of C. arabica progenies using RAPD markers, found a fixation index (FST) of 0.385, attributing the main cause of decreased genetic diversity to the many selection cycles done on genotypes. Similarly, ANTHONY et al. (2001), using 29 RAPD primers to study genetic diversity among and within natural C. arabica populations collected in Ethiopia, found a FST of 0.375. In the current study, EST-SSR markers effectively detected a high rate of genetic polymorphism among the sample populations, as revealed by a FST of 0.637.

4. CONCLUSION

The EST-SSR markers used in this study showed a relative high degree of polymorphism, efficient to study genetic diversity in coffee trees. In addition, it was showed that it is possible to use these EST-SSRs for coffee variety identification studies. Through these SSR markers, the most distant Híbrido de Timor accessions (CIFC 832/2 and CIFC 4106) from C. arabica genotypes were identified; these may be used to increase the genetic base of breeding programs. The Híbrido de Timor 'CIFC 1343/269' was found to be closest to the arabica coffees, it may, thus, be useful for breeding programs to incorporate one of more C. canephora rust-resistance genes while maintaining other C. arabica traits. Our data showed that EST-SSR markers may be useful in coffee breeding programs, particularly for crossings orientation, diversity studies, genetic introgression and genetic mapping.

ACKNOWLEDGMENTS

We wish to acknowledge the Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES), the Fundação de Amparo a Pesquisa do Estado de Minas Gerais (FAPEMIG) and the Consórcio Brasileiro de Pesquisa e Desenvolvimento do Café (CBP&D) for funding.

Receipt for publication in July 28, 2008 and accepted in April 1.º, 2009.

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  • *
    Correspondent author.
  • Publication Dates

    • Publication in this collection
      07 Dec 2009
    • Date of issue
      Sept 2009

    History

    • Accepted
      01 Apr 2009
    • Received
      28 July 2008
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