Molecular Biology and Genetics
Plant Biotechnology
EJB Electronic Journal of Biotechnology ISSN: 0717-3458 Vol. 5 No. 2, Issue of August 15, 2002
© 2002 by Universidad Católica de Valparaíso -- Chile Received February 12, 2002 / Accepted August 7, 2002
DOI: 10.2225/vol5-issue2-fulltext-9  
RESEARCH ARTICLE


Analysis of genetic diversity in the Oryza officinalis complex

María Teresa Federici*
Unidad de Biotecnologia
Instituto Nacional de Investigación Agropecuaria
Estación Experimental “Las Brujas”
Ruta 48, km 10, Rincón del Colorado
Canelones, Uruguay
Tel: 598 2 0327 7641
Fax: 598 2 0327 7609
E- mail: maritefe@inia.org.uy

Andrei B. Shcherban
Laboratory of Molecular Genetics of Cereals
Institute of Cytology and Genetics,
Lavrentieva Ave.10, 630090
Novosibirsk, Russia
E- mail: atos@bionet.nsc.ru

Fabián Capdevielle
Unidad de Biotecnologia
Instituto Nacional de Investigación Agropecuaria
Estación Experimental “Las Brujas”
Ruta 48, km 10, Rincón del Colorado
Canelones, Uruguay
Tel: 598 2 0327 7641
Fax: 598 2 0327 7609
E- mail: fabian@inia.org.uy

Marta Francis
Unidad de Biotecnologia
Instituto Nacional de Investigación Agropecuaria
Estación Experimental “Las Brujas”
Ruta 48, km 10, Rincón del Colorado
Canelones, Uruguay
Tel: 598 2 0327 7641
Fax: 598 2 0327 7609
E- mail: mfrancis@inia.org.uy

Duncan Vaughan
Crop Evolutionary Dynamics Laboratory
National Institute of Agrobiological Resources (NIAR)
Kannondai 2- 1- 2, Tsukuba
Ibaraki, 305, Japan
Tel: 81 298 38 7406
Fax: 81 298 389 7408
E- mail: duncan@abr.affrc.go.jp

* Corresponding author

Financial support: Japan Cooperation Agency – individual training of Group Course “Plant Genetic Resources”.

Keywords: dendrogram, genetic diversity, Oryza officinalis complex, RFLP´s.


Abstract

The genetic relationships among 34 accessions of wild rice from Asia, Africa, America and Australia were analysed using RFLP technique. After southern blotting, DNA digestion pattern was hybridised with a highly repetitive DNA sequence of a retrotransposon from a gypsy family of mobile elements. A dendrogram was constructed from RFLP data in which the species clustered according to their genome designation (CC, BB, BBCC and CCDD genomes). Some species did not appear in the same group, for example, O. eichingeri from Africa and Sri Lanka clustered separately from each other. The same situation was observed for the accessions from China of O. officinalis, which cluster together showing a close relationship with O. rhizomatis, and O. eichingeri (both of CC genome). Also, the tetraploid BBCC from India of O. officinalis appears in the same cluster of O. eichingeri and O. punctata (both from Africa) suggesting close phylogenetic relationship with the African genomes BB, CC and BBCC.

Article

The genus Oryza consists of about 22 species having a pan-tropical distribution (Vaughan, 1994). Taxonomists have divided this genus into several species complexes among which the O. officinalis species complex has the most species and greatest number of different genomes (Tateoka, 1962; Vaughan, 1989). Nine species and two distinct chromosome races within two of these species have been described in the O. officinalis complex (Table 1). Several traits of potential economic importance to rice improvement have been found in this complex, for example, resistance to brown planthopper which has been incorporated from O. officinalis into varieties of rice released in Vietnam (Brar and Khush, 1997).

The O. officinalis complex is of particular interest because, in contrast to the single AA genome of all species in the O. sativa complex to which the rice cultigens belong, the O. officinalis complex has 4 of the 10 genomes so far designated for species in the genus Oryza. In addition, the O. officinalis complex includes both diploid and allotetraploid species. In the genus Oryza, all the other species complexes include either diploid species, such as species in the O. sativa complex, or allotetraploid species such as species in the O. ridleyi complex. Thus the O. officinalis complex not only furnishes broad Oryza genomic diversity for study but also may give insights into polyploidy in the genus Oryza.

The taxonomy of the O. officinalis complex is based mainly on morphological and cytological data. It includes 5 diploid species with the CC, BB and EE genomes and 4 allotetraploid species together with two allotetraploid races of diploid species having BBCC or CCDD genome constitution. The phylogeny within the complex is complicated due to the presence of morphologically similar forms of the same taxa completely isolated from each other such as O. eichingeri that occurs in Africa and Asia. In addition, three allotetraploid taxa with the same genome designation, BBCC, are found in widely separated locations in Africa, South Asia and Southeast Asia. Further the allotetraploid taxa of Latin America with CCDD genome are sympatric for part of their range and isolation barriers between them have not been determined yet. Application of different techniques based on DNA markers is necessary to better understanding of phylogenetic relationships within the complex.

Various molecular methods have been used to clarify phylogenetic relationships within the Oryza genus, mainly within the O. sativa complex, but information and data concerning genome molecular organisation in the O. officinalis complex, is still limited. Genetics of A- genome rice has been extensively studied (for review, Oka, 1988) (Kazuyuki et al 2000). RFLP´s methodology using single copy probes from O. sativa was previously reported to analyse genetic diversity within Asian A- genome rice species by Nakano et al. 1992 and Kazuyuki et al. 2000.

Molecular approaches such as RFLP´s (Wang et al. 1992) and DNA fingerprinting using hypervariable minisatellite probes (Aggarwal et al. 1994) provide genetically interpretable variability with extensive genomic coverage and have thus become immensely important in studies on population biology and systematics. Based on classical isozyme, and RFLP studies, all species in the genus Oryza except O. brachyantha (FF genome) have been grouped into four main species complexes: (1) Sativa, (2) Officinalis, (3) Ridleyi, and (4) Meyeriana (Tateoka, 1962; Vaughan 1989; Second, 1991; Wang et al. 1992; Vaughan 1994). The complexes Meyeriana and Ridleyi have only 5 species with the recently assigned new genomes, GG and HHJJ (Aggarwal et al. 1997; Aggarwal et al. 1999). Species with CCDD genome of the genus Oryza L. were analysed by RFLP markers (Jena and Kochert, 1991) and a very powerful technique, the AFLP molecular markers were applied and revealed phylogenetic relationships among Oryza species (Aggarwal et al. 1999).

Repetitive DNA markers are very useful for studying genetic diversity. There are several advantages that make these markers an informative tool for study of genetic diversity. First of all, they represent a largest part of the plant genome (Flavell et al. 1977). They change rapidly compared with single copy sequences (Jelinek and Schmid, 1982). Finally, repetitive DNA sequences show low intraspecific variation so they are suitable to study species divergence and inter specific relationships (Dvorak and Dubcovsky, 1996). Recently, many common and species- or genome- specific repetitive DNA sequences have been isolated from a number of Oryza species. These repetitive sequences have been used as markers to study phylogeny within the Oryza genus (Zhao et al. 1989; Cordesse et al. 1992; Motohashi et al. 1997; Uozu et al. 1997; Iwamoto et al. 1999; Kumekawa et al. 1998). These sequences represent different types of repetitive DNA including tandem repeats, rRNA genes, short interspersed sequences and LTR retrotransposons.

In the O. officinalis complex two sequence families have been studied in detail: tandem repeat TrsC that is specific for the CC- genome and retrotransposon RIRE- 1 highly amplified in the genome of O. australiensis (Nakajima et al. 1996; Shcherban et al. 2000). The isolation and characterisation of the pOe.49, a clone isolated form O. eichingeri, that represents a part of the integrase domain of a gypsy- like retrotransposon and its use in analysis of diversity within the Oryza officinalis complex was reported by Shcherban et al. 2000. Also, a Tourist element of the 5´-flanking region of the catalase gene Cat. A, reveals evolutionary relationships among Oryza species with various genome types (Iwamoto et al. 1999).

In this study, a dispersed repetitive element, a Gypsy- like retrotransposon (Shcherban, 2000) was used as a probe for the RFLP analysis (restriction fragment length polymorphisms). This technique consists in the digestion of genomic DNA with diferent restriction enzimes, gel electrophoresis and southern blot hybridisation of fragments with a labeled probe (a repetitive element in this case). In this study detection of polymorphic bands was performed by a process called autorradiography. Specific procedures used will be explained in materials and methods section. Polymorphisms resulted from the presence or absence of the restriction sites (4-8 bp sequences) as well as punctual mutations, and other changes like insertions, deletions, invertions, etc which alter the distance between restriction sites.

This report includes some different accessions than previously mentioned report that represent all O. Officinalis species and genomes. Also, another set of enzymes was tested. The results obtained confirmed previous studies but also gave new insights into phylogeny in the complex and the origin of some taxa.

Materials and Methods

Plant material, DNA isolation and quantification. Thirty four accessions of different species within the O. officinalis complex were used to represent the diversity of germplasm in this species complex. The species names, genome composition, chromosomes, accession numbers, and origin of accession are shown at Table 1.

Preparation of total genomic DNA was carried out according to the following procedure: 1,5 gr of young leaf tissue were frozen in liquid nitrogen, powered, and then quickly homogenised using a cold mortar and pestle in 3 ml of homogenisation buffer (2X CTAB). The homogenate was incubated at 60ºC for 45 min. An equal volume of chloroform/ isoamyl acid was added and mixed gently by a rotor for 45 min. Then, the tubes were centrifuged at 5000 rpm for 15 min and the supernatant was transferred to another tube. A 10% of the total volume of 2X CTAB and equal amount of precipitation buffer were then added. After DNA became visible, samples were centrifuged for 15 min at 12000 rpm. The DNA pellet was dried slightly and resuspended in 500 µl of HSTE (high salt TE buffer) containing RNAase (50 µg/ ml). The samples were incubated overnight at 37ºC and DNA was then precipitated by adding two volumes of isopropanol. After centrifugation at 15000 rpm for 5 min, pellet was dried at room temperature and finally resuspended in 500 µl of TE. The DNA samples were stored at 4ºC.

DNA was checked for quality in 1-% agarose gel and DNA concentration was estimated by spectrophotometer (absorbance at 260 nm) followed by agarose gel electrophoresis for final estimation against a defined amount of lambda DNA as standard.

RFLP technique

DNA digestion by restriction enzymes and electrophoresis. An amount of 2-5 µg of genomic DNA of each accession was digested with a total of 8 restriction endonucleases (Eco RI, Eco 47I, Eco RV, Hind III, the combination of enzymes Dpn/ Xba I and Bgl II/ Bam HI) for between 12-16 hrs. The reactions were performed in a total volume of 100 ul in the presence of the appropriate buffer with 5 units of endonuclease per 1 µg of DNA. After digestion 10 µl of each sample was electrophoresed in 1- % agarose gel at 75 volts during 6-8 hrs.

Probe labeling. The cloned repetitive DNA sequence pOe.49 (Shcherban et al. 2000) was used as a probe. The DNA of insert was amplified and labeled in 50 µl of reaction mixture containing the unlabelled nucleotides dATP, dGTP, dCTP (2.5 mM of each), labeled DIG- dUTP (10X solution contains 0.125 mM DIG- dUTP, 0.375 mM dTTP), the specific direct and reverse primers for pUC/ M13 (5-10 pg. each), the plasmid DNA of clone (10 ng), buffer (standard PCR buffer containing 1.8 mM MgCl2), Taq. - DNA polymerase (1 unit). Before addition of Taq. - polymerase the mixture was boiled to denature DNA for 5 minutes.

The PCR program includes 40 cycles consisting of a denaturation step (1-min at 93ºC), annealing step (1 min at 55ºC) and DNA extension step (0.5 min at 72ºC). After PCR the aliquot of labeled DNA (5 µl) was checked by electrophoresis. The rest of DNA was precipitated with ethanol and after centrifugation for 15 min at 12000 rpm the pellet was dissolved in 50 µl of TE.

Southern blot hybridisation. DNA fragments were transferred from the agarose gel to a nylon membrane by capillary blotting overnight. After transfer membranes were rinsed with 2x SSC and baked at 80ºC for 1 hr to cross link DNA. Hybridisation was carried out overnight in 5x SSC, 1% Blocking Reagent (Boehringer – Mannheim), 0.1% N-lauryl sarcosine and 0.02% SDS at 65ºC (high stringency). The amount of DNA probe added was 1/10 part of the final volume (see Probe labeling) that corresponds to about 50-100 ng of DNA. Before adding, probe was boiled in the water bath for 5 min. After hybridisation membranes were consecutively washed in 2x SSC, 0.1% SDS; 0.5x SSC, 0.1- % SDS for 20 minutes each at 65ºC.

Detection procedure. After washing membrane was incubated in the blocking solution (1% of Blocking Reagent dissolved in the AP7.5 buffer containing 0.1 M Tris- HCl, 0.1 M NaCl, 2mM MgCl2) for 1-2 hrs at room temperature. Then the membrane was transferred into the same solution containing the antibody conjugate to digoxigenin (anti-DIG-AP) which was previously diluted 100 times in the blocking solution up to 75 mU/ ml. After that 2 washing steps of 15 min each were performed by shaking of membrane in the AP 7.5 buffer. After equilibrating of membranes in buffer AP 9.5 (0.1 M TrisHCl, 0.1 M NaCl, 50 mM MgCl2) it was incubated in 1-2 ml of developing solution within a saran bag for 5 min. Developing solution contains chemoluminescent substrate CSPD (Boehringer – Mannheim) diluted 100 times in buffer AP 9.5. The membrane was rinsed briefly in AP 9.5 buffer to discard the excess of substrate and transferred to a new saran bag. Before autoradiography the membrane was put in the oven at 37ºC for 15 min to enhance the luminescent signal. Then, the membrane was exposed up to 20 min to an X-ray film at room temperature.

Genetic analysis. RFLP bands were scored as present (1) and absent (0) and only bands showing unambiguous polymorphism were entered into a data matrix that was used to construct a phylogenetic tree. Genetic similarity was calculated with the simple matching coefficients (Sokal and Michener, 1958) using NTSYS software. Then, the similarity matrices were subjected to cluster analysis by the unweighted pair- group method with the arithmetic averages (UPGMA) cluster method and Plus analysis (Innan et al. 1999).

Results

Genomic organisation of pOe.49 among O. officinalis complex species

The repetitive DNA sequence pOe.49 used in this study was taken from a genomic library of O. eichingeri (Shcherban et al. 2000). This sequence has a similar very intensive signal of hybridisation with genomic DNA from O. officinalis, O. rhizomatis, O. eichingeri, O. punctata (BB) and O. australiensis, diploid species of the O. officinalis complex. The primary structural analysis of this sequence and database searching revealed it is homologous to different retrotransposon elements of gypsy class widely spread within genomes of many plants (Suoniemi et al. 1998).

The organisation of the pOe.49 repetitive sequence in 34 accessions of different taxa of the O. officinalis complex was determined by Southern hybridisation using genomic DNA digested by eight restriction endonucleases (Hind III, Eco47 I, EcoRI, Eco RV, Dnp/ Xba I, Bgl II/ Bam HI). The accessions represent all known species and chromosome races of the complex and each species/chromosome race is represented by 2 - 3 accessions. Each enzyme or combination produced polymorphic patterns containing multiple discrete bands with high intensity of hybridisation to pOe. 49. No obvious variation in total intensity of hybridisation was found between species.

Diversity analysis based on RFLP assay

High polymorphism of the blot-hybridisation patterns was observed between different species of the O. officinalis complex. The level of polymorphism was lower within species than between species or between different genomes.

Polymorphism between species with different genomes

All genomes groups including diploid CC, BB, EE and tetraploid BBCC and CCDD could be recognised on the basis of the polymorphism revealed by blot hybridisation. The dendrogram (Figure 1) based on the RFLP data clearly separated the diploid genomes CC (O. officinalis, O. eichingeri and O. rhizomatis), BB (O. punctata) and EE (O. australiensis). The accessions of O. minuta (BBCC) and the BBCC tetraploid accession of O. punctata showed closest affinity with the diploid O. punctata and were clustered with the latter. The cluster of CCDD species (O. latifolia, O. alta and O. grandiglumis) has a separate position in the dendrogram (Figure 1) and the out-group O. australiensis (EE genome) clustered apart, as expected.

Interspecific polymorphism

Each species has specific hybridisation patterns and could be distinguished from one another. However, accessions of O. eichingeri from Africa (Uganda) and Asia (Sri Lanka) clustered separately from each other.

The accessions with CC genome of O. officinalis and O. rihizomatis, together with O. eichingeri from Sri Lanka were in the same cluster. Some CC genome accessions (three of O. eichingeri from Uganda and one of O. officinalis from India) clustered together showing a closer relationship with O. punctata diploid accessions than other CC genomes of O. eichingeri, O. officinalis and O. rhizomatis. All O. punctata accessions (diploids and tetraploids), cluster together followed by the tetraploid O. minuta which show a clear relationship between genomes.

The CCDD cluster contains species that are distant from all species of the complex. O. grandiglumis and O. alta had almost identical hybridisation patterns and are clearly separated from O. latifolia.

Intraspecific polymorphism

A low level of intraspecific variation was found. The highest level of intraspecific polymorphism was found in O. officinalis and O. eichingeri.

The eco- geographical forms of O. officinalis from China clustered together clearly separated from the Myanmar, Brunei, Philippines, Papua New Guinea and India accessions. On the other hand, the O. officinalis accession from India clustered separately from all other O. officinalis accessions mentioned above, closer to O. eichingeri from Uganda and O. punctata.

O. eichingeri consists of two clearly distinguished forms, which correspond to accessions from Uganda and Sri Lanka. The accessions from Uganda are clearly divergent form the other CC species while the accessions from Sri Lanka clustered together with O. rhizomatis, which is indigenous to Sri Lanka.

Discussion

The phylogenetic tree constructed with RFLP data shows the CC genome species O. officinalis, O. eichingeri and O. rhizomatis clustering together. Another cluster is formed for BB and BBCC genomes of O. punctata, O. minuta, O. officinalis from India and O. eichingeri from Uganda followed by a cluster of CCDD genome species (O. latifolia, O. alta and O. grandiglumis). The out group species O. australiensis (EE genome) clustered apart from other species, as expected.

Variation in the hybridisation patterns was observed among different accessions of O. officinalis. The accessions from Brunei, Philippines and Papua New Guinea formed a separated group. The accessions from China and Myanmar are quite distinct and have diverged from the first group. These 3 groups of accessions probably correspond to distinct eco- geographical forms of O. officinalis located in China, South and Southeast Asia (Hu and Chang, 1967).

The most striking divergence was observed within O. eichingeri. The taxonomic status of this specie has been clearly established (Biswal and Sharma, 1987). However, information presented here suggests that it may be necessary to re-evaluate this specie and determine whether infra-specific taxa for the African and Sri Lankan forms are warranted. In this study O. eichingeri was represented by six accessions. Four from Africa showed hybridisation patterns quite different from other CC genome species. The hybridisation patterns of the two accessions form Sri Lanka and those of O. rizomatis, reported only form Sri Lanka, are similar implying their close relationships. Such a high level of genetic divergence within one species suggests that O. eichingeri is likely to be the ancestral species of the CC genome group which is supported by its wide distribution in West and East Africa and Sri Lanka (Vaughan, 1994).

Diploid O. punctata, the only BB genome species, is genetically clearly distinguished from its tetraploid chromosome race. However, based on dendrogram (Figure 1) diploid O. punctata is more closely related to its tetraploid race than the other two BBCC taxa. Results presented here, in addition to morphological, ecological and physiological differences between the diploid and tetraploid races of O. punctata suggest that these two chromosome races should be considered separated species (Sano, 1980; Sasahara et al. 1982).

There are three tetraploid BBCC taxa, O. punctata (4x), O. officinalis (4x) and O. minuta. The BBCC taxa is not genetically as close to the diploid CC genome species as diploid O. punctata (BB genome). Diploid and tetraploid O. officinalis are clearly differentiated and this supports the view that this chromosome race deserves specific rank (Krishnawamy and Chandrasekharan, 1957).

The diploid BB genome species O. punctata were found to be genetically closer to the tetraploid O. punctata than to either other BBCC taxa.

The putative CC genome donor of the tetraploid O. punctata from Africa is O. eichingeri from Africa. But the CC donor of O. officinalis (4x) and O. minuta were not clearly identified because of the similar genetic distances between these tetraploid species and each of the CC diploid species (data not published). The comparatively low values for genetic distance among CC species suggests that they might have evolved from relatively recent hybridisation and polyploidisation events between BB and CC genome species.

The specie O. minuta was found to be clearly differentiated from both tetraploid O. punctata and O. officinalis. This suggests that O. minuta evolved independently from other BBCC species. The morphology, habit and present distribution of O. minuta also clearly separate this species from other in the complex. The specie O. minuta has closer affinity to diploid O. punctata than diploid O. officinalis.

The species with the CCDD genome from Latin America are O. latifolia, O. alta and O. grandiglumis. This group is distantly related to other species of the O. officinalis complex. This is in agreement with previous data (Aggarwal et al. 1999) and implies that this group of species evolved independently over a much longer period than other genomes within the complex did (with the exception of O. australiensis).

Genetic differences among these CCDD species have been clearly demonstrated by total genomic DNA hybridisation and RFLP analysis (Aggarwal et al. 1996). However, other research suggested that the three taxa form a single complex species (Chen and Matsunaka, 1991; Jena and Kochert, 1991). RFLP data present here shows that O. latifolia is clearly distinguished from O. alta and O. grandiglumis. The species O. alta and O. grandiglumis are closely related to each other and form a separate cluster within the CCDD group. Observations of O. alta and O. grandiglumis in their natural habitat, including sympatric populations, have also suggested these two species are very closely related (Morishima and Martins, 1994).

In conclusion, the data presented in this work has demonstrated that the retrotransposon- like sequence pOe.49 is useful for studying phylogenetic relationships within the genus Oryza. The results obtained by RFLP markers are generally consistent with previous morphological, cytological, and molecular marker analysis. Besides confirmation of previous results new information on the divergence and differentiation of some species and genomes within the complex has been presented.

Acknowledgments

This research was conducted during the individual training of JICA (Japan International Cooperation Agency) course “Plant Genetic Resources”. I want to express my thanks to the NIAR Institute, to Dr. Duncan Vaughan, head of “Crop Evolutionary Dynamics Laboratory”, and Dr. B. Shcherban for providing the material used in this study and directly supervise my work. I also express my thanks to Ing. Agr. Marta Francis, Ph.D. and Ing. Agr. Fabián Capdevielle, MSc. from INIA Las Brujas, Unit of Biotechnology for promoting my training course in Japan.

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