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Analysis of genomic sequences from peanut (Arachis hypogaea) Jayashree
B. Morag Ferguson Dan Ilut Jeff Doyle Jonathan
H. Crouch* *Corresponding author Financial
support: Legume genomics, bioinformatics and molecular breeding
research at ICRISAT has benefited from unrestricted grants from
the governments of Keywords: Arachis hypogaea, codon usage, gene-based markers, peanut, SSR markers.
Peanut is an important legume crop across the world. However, in contrast to most legume crops, groundnut lacks taxonomic proximity to any major model genome. A relatively large number of genomic sequences were generated from groundnut as part of a microsatellite marker development project. In the current study, a total of 1312 sequences were analyzed of which 448 contained microsatellite motifs. All sequences (GenBank Accessions: BZ999351-CC000573) were analyzed after clustering for possible similarity with publicly available sequences from Arabidopsis, Lotus, soybean and Medicago. At least 39% of the sequences analyzed had significant BLAST similarities with sequences from the four databases searched, of which nearly half (47%) found significant similarity with Lotus japonicus sequences. Over one quarter (26.7%) of sequences found similarity with Arabidopsis thaliana, while the remainder aligned with publicly available sequences from the legumes soybean and Medicago truncatula. At least 17% of microsatellite containing sequences could be assigned an identity. The codon usage pattern for Arachis hypogaea most closely resembles that of L. japonicus reflecting the similarly high sequence similarity observed in BLAST searches at the protein level. The implications of these findings for the taxonomy, and comparative genomics of groundnut and its legume family relatives are discussed.
Peanut
(Arachis hypogaea), also known as groundnut, is an important
legume crop across the Most of the major legume crops and model legume species are concentrated in a very limited region of the legume phylogenetic tree: viz. the sister clades of "halogalegina" (Lotus and Medicago) and "phaseoloid/millettioids" (soybean and Phaseolus). In contrast, Arachis falls in the "dalbergioid" clade, which includes no other major crops and is differentiated from all others by possession of a unique 50 kb inversion (Doyle and Luckow, 2003). Members of this clade are known to be diverse and relationships amongst members of this group and with members of other clades are still somewhat unclear. It is believed that a large majority (>90%) of plant sequences have close homologs within most other plant genomes (Bennetzen, 2000). Thus, comparisons of DNA sequences from taxa whose genomes have been partially or fully sequenced can to a certain extent provide estimates of relationships, such as the comparisons between Arabidopsis genomic sequences and rice ESTs (Eckardt, 2001), wherein it was concluded that Arabidopsis could not be used as a model system for monocots. Thus, having generated 1312 new genomic sequences from groundnut (Ferguson et al. 2004) we took the opportunity to compare these sequences with major crops and model genomes, with the intention of better understanding the relationship between the genomes of groundnut, Lotus, soybean, Medicago and Arabidopsis. This approach was also expected to provide functional annotations for some of the new SSR markers that we have reported previously (Ferguson et al. 2004), which can then be used for the development of candidate gene-based markers. This is consistent with previous reports indicating that microsatellites are highly abundant in protein coding regions (Cardle et al. 2001). Since the methylation sensitive restriction enzymes PstI and Sau3A1/BamH1 were used during genomic library construction we expected the library to be enriched for low-copy sequences, which could find homologs during database searches. We report here, putatively annotated SSR markers, sequences that may be used as gene-based markers and the choice of codons amongst the dicots studied. Sequence generation and analysis Genomic
libraries were sequenced as reported elsewhere (Ferguson
et al. 2004). Two peanut genomic DNA libraries were constructed,
one following PstI digestion of the whole genome and the other after
Sau3AI/BamHI digestion. Both libraries were probed using γP32-dATP
labeled oligonucleotide probes: (GT)15, (GA)15,
(AAC)10, (ATC)10, (AGT)10, (ATT)10,
(CAC)10, (CTT)10 and (CTG)10. The
PstI library was also probed with (ATCC)10, (GATA)10
and (AAAT)10. Filters were screened with genomic DNA to
eliminate those clones containing repetitive DNA. Sequencing was performed
using an ABI3700 automated DNA Analyzer (Applied
Biosystems, Vector sequences were trimmed using Sequencher v.4 software and low quality bases (quality score <20) were trimmed from both ends of sequences. A total of 1312 sequences were selected for the analysis of which 448 contained SSR motifs. All sequences containing interspersed or simple repeats were masked with the RepeatMasker software (http://www.repeatmasker.org/). The sequences were assembled using cap3 sequence assembly software (Huang and Madan, 1999) with default parameters. The singletons and consensus sequences were screened using tBLASTx against Arabidopsis, soybean, Medicago truncatula and Lotus japonicus TIGR Gene Indices. An in-house script was used to retrieve best matches from the outputs of tBLASTx text files, retaining the following information: gene identifier, description, BLAST score, percent identity, alignment length, reading frame, and database name from the top-scoring alignments from each database. A transformation of e-values was carried out to pick up the best e-value across hits from all four databases. The e-value transformation was carried out using the following formula: E = (m*n)/(2^S') where m = length of query sequence, n = reference target database length, S'= the normalized HSP score, based on the method of Altschul et al. 1997. The resultant best hit was then used to annotate the sequence if there was a minimum of 30% identity over at least 20% of the protein sequence (Quackenbush et al. 2000; Quackenbush et al. 2001). Such matches were considered to provide a reasonable putative annotation. Tandem repeats were searched for using RepeatFinder (http://tandem.bu.edu/trf/trf.advanced.submit.html). Alignment parameters (2,3,5) were used for match, mismatch and indels, and a maximum period size of 10 was applied. The EMBOSS tool 'cusp' was used to calculate the amino acids and codon usage frequencies of Arachis sequences (http://bioweb.pasteur.fr/seqanal/interfaces/cusp.html). Previously reported codon usage tables for Arabidopsis, soybean, Medicago and Lotus were obtained from http://www.kazusa.or.jp/codon/ (Nakamura et al. 2000). Relative Synonymous Codon Usage values (RSCU) were calculated using the formula RSCUij = Xij/1/niΣ Xij, where Xij is the frequency of occurrence of the jth codon for the ith amino acid, and ni is the number of codons for the ith amino acid. The degree of preference for a particular codon was examined. In the absence of any codon usage bias, the RSCU value would be 1.00. A codon that is used less/more frequently than expected will have a value of less/more than 1.00. A total of 1312 sequences were analyzed of which 448 contained microsatellite motifs. The average length of sequences in this dataset was 542 bp. When assembled using cap3, 135 sequences assembled into 56 contiguous sequences (generally comprising 2-4 sequences), while 1177 sequences remained as singletons. In silico comparative legume genomics Comparative genomics enables the application of data from one species to investigations of taxonomically disparate species, as has been achieved for example in the annotation of wheat sequences using information from E. coli, human, A. thaliana and rice (Heslop-Harrison, 2000). Thus, large-scale genome sequencing projects have been partially justified on the basis of the premise that knowledge of the whole sequence of Arabidopsis, for example, will help in the isolation from crop plants of agronomically important genes that bear homology to Arabidopsis genes. While sequence-based comparisons using BLASTn have been used to identify similar sequences from other taxa (rice ESTs compared with A. thaliana genomic sequences for instance), it has been suggested that BLASTn may not always be reliable when dealing with divergent, partially sequenced genomes (Devos et al. 1999). A comparison at the amino-acid level is considered more effective. About 38.5% (475 singletons and contigs from a total of 1233 sequences) of the Arachis sequences had significant similarity with sequences in public databases at the amino acid level. All contigs and singletons were searched against Arabidopsis, soybean, Lotus and Medicago Gene Indices. Of the sequences that found matches in any of the four databases, the maximum number of matches was with sequences from the L. japonicus Gene Indices (581 hits), followed by 491 hits against the Arabidopsis Gene Indices, 358 hits against the soybean Gene Indices and only 221 hits against Medicago Gene Indices (Figure 1). A total of 325 Arachis sequences found matches with both the Lotus and Arabidopsis data bases, while 203 sequences found matches with both the Lotus and soybean databases. Finally 116 Arachis sequences found hits with all three databases (Lotus, Arabidopsis and soybean), while only 25 sequences found matches in all four databases searched. These numbers depict the numbers of Arachis sequences finding matches in each of the four databases searched; they do not indicate numbers after e-value transformation and selection of the best match across databases. The TIGR Gene Indices integrate data from international EST sequencing and gene research projects, and their process of clustering ESTs into contigs or TCs (tentative consensus sequences) reduces redundancy levels. As expected, the Arabidopsis Gene Indices dataset size is far larger than the other databases that were screened. Though there are a considerable number of sequences from the model legumes Medicago, soybean and Lotus in the public domain, the size of these databases is still smaller than Arabidopsis, which is almost 5 times the size of the Lotus dataset. Thus, when carrying out searches against several databases it is important to account for the differences in sizes amongst target databases, so that abundance in target data set does not bias the distribution of the best hits. The process of transforming e-values by calculating an equivalent e-value for a reference database using a formula based on Altschul et al. 1997 (see Materials and Methods) helps to overcome the effect of variation in database size, when comparing searches against several databases. Thus, the best match from across the four species was used for the process of putative annotation. Furthermore, parameters such as "percent identity" and length of alignment of the query sequence with subject were used to determine whether the alignment could be considered for annotation. Using this process 475 of the 1233 non-redundant sequences were assigned a putative identity. Of the 475 sequences that have been annotated, 222 were assigned their putative annotations from L. japonicus sequences (46.7%), 127 (26.7%) from Arabidopsis, 89 from soybean and 37 from Medicago. The large disparity between the frequency of matches with Medicago versus Lotus and soybean suggests that genome relationships amongst the legumes are highly complex. Moreover, the genomic relationships between legumes and Arabidopsis may also be more complex than previously expected. The low degree of sequence redundancy as evidenced from the clustering process (56 contigs and 1177 singletons) suggests that the use of methylation sensitive restriction enzymes has enriched for low copy number sequences. However, the annotation of only 38.5% of the sequences, suggests that Arachis is relatively diverged from all the other species studied here. Comparative studies have revealed that (a) the evolution of essential gene coding regions has proceeded relatively slowly, as a result of which reproductively isolated taxa have retained recognizable intragenic regions and (b) a large majority (>90%) of plant sequences have close homologs within most other plant genomes (Bennetzen, 2000; Paterson et al. 2000). Comparisons of DNA sequences from taxa whose genomes have been fully sequenced can to a certain extent provide estimates of relationships, such as the comparisons between Arabidopsis genomic sequences and rice EST's (Eckardt, 2001), wherein it was concluded that Arabidopsis could not serve as a model system for monocots. While the present study is limited to sequence comparisons, which cannot by themselves explain relationships at the species level, they do provide valuable practical insight into the similarities, differences and relative distances amongst the legumes and beyond. Thus, it appears from these preliminary comparisons (Figure 1) that L. japonicus could be the most appropriate model species for peanut comparative genomics and genome evolution studies. Putative
functional annotations for the sequences were obtained from the most
significant match obtained from database searches. The putative annotations
were grouped under nine general categories based on similarity of
biochemical function, which is summarized in Figure
Patterns of codon usage were also assessed in the A. hypogaea sequences, and compared with those of the other three legumes and Arabidopsis. Codon usage can be surprisingly biased in different species. It is well known that the pattern of synonymous codons used varies depending on the organism involved, and each type of genome has a particular codon usage profile (Grantham et al. 1981). Knowing an organism's preferred codon usage is of direct practical relevance in minimizing degeneracy of PCR primers, while trends in codon usage can also be used in molecular phylogenetic reconstruction. The codon usage table for A. hypogaea was compared with previously reported codon usage tables for Arabidopsis, soybean, Medicago and Lotus. We have studied the computed relative synonymous codon usage value (RSCU) of each codon, the RSCU being the observed frequency of that codon divided by the frequency expected if usage of synonymous codons was uniform. The overall codon usage for A. hypogaea is presented in Table 3 along with that of Arabidopsis, soybean, Medicago and Lotus for comparison. These data illustrate similar codon usage patterns amongst these dicots, with 8 of the 18 frequently used codons being common amongst all the five plant species. The codon usage pattern for A. hypogaea most closely resembles that of L. japonicus, with 15 of the 18 most frequently used codons in A. hypogaea being the most commonly used in L. japonicus. A. hypogaea and L. japonicus differ from the other dicots in their usage of codons for two-fold degenerate amino acids cysteine, glutamine, phenylalanine, histidine, tyrosine and the three-fold degenerate isoleucine. A. hypogaea and L. japonicus differ from each other only in the use of codons for six-fold degenerate amino acids leucine and serine, and the four-fold degenerate proline. Amongst the other two legumes and Arabidopsis, soybean and Arabidopsis are closest, all 18 frequently used codons in Arabidopsis are also the most frequently used codons in soybean, while 17 of the 18 frequently used codons are common between Arabidopsis and Medicago. This is consistent with comparative data at the structural level, where comparisons of Arabidopsis with soybean report significant synteny along the entire length of Arabidopsis chromosome 1 and soybean linkage group A2 and blocks of synteny were found among other chromosomes as well (Grant et al. 2002). Soybean and Arabidopsis are estimated to have diverged from a common ancestor 92 million years ago. In contrast, a comparative study between Medicago truncatula and Arabidopsis concluded low levels of microsynteny (Zhu et al. 2003). Finally, there is a bias towards C/G in the third position in Arachis and Lotus whereas soybean, Medicago and Arabidopsis tend to choose codons ending with A/T in the third position. Codon usage is broadly similar in closely related species and tends to diverge with increasing phylogenetic distance. As codon usage divergence is correlated with evolutionary distance (Grantham et al. 1981; Long and Gillespie, 1991), it has been suggested that codon usage can help unravel the evolutionary relationships between species (Goldman and Yang, 1994; Nesti et al. 1995). The very similar pattern of codon usage in A. hypogaea and L. japonicus relative to the other three dicots, reflects the sequence similarity observed during the BLAST searches at the protein level, although the coding strategy will vary at the level of the individual gene. Thus, codon usage profiles also support the genomic relationship between the dicot species investigated in this study. A primary objective of this analysis was to infer biological function from the conservation of homologous DNA sequences between plant species. This approach was expected to provide functional annotations for new SSR markers and facilitate the development of gene-based markers in A. hypogaea. This analysis also has the potential for contributing to the understanding of genome evolution from the DNA/protein sequence perspective. Only 38.5% of the sequences found putative annotations, this may be due to the fact that not all Arachis sequences generated in this study are coding sequences, and non-coding sequences are known to evolve much faster than coding regions do. This is highly relevant given that the target legume sequences used in searches are transcribed sequences (TIGR Gene Indices). Several of the microsatellite-containing sequences have been assigned a putative identity and at least some of these will now be useful as gene-based markers in peanut research and breeding. The remaining sequences with putative identity assigned can also serve as candidate genes. In particular those sequences putatively identified to be involved with disease resistance/defence and retroelement-containing sequences can serve as candidate gene-based markers in diversity analysis and trait mapping studies. Combining expression studies with computational analysis using publicly available tools and curation should help in assigning an identity to the sequences with unknown function, as has recently been shown with "hypothetical" genes from the H. influenzae dataset (Kolker et al. 2004). All the Arachis sequences studied here are available at GenBank (Accessions: BZ999351-CC000573) and could be used in comparative and functional genomic studies. In this study we have found that L. japonicus has considerable sequence similarity with A. hypogaea. To evaluate codon choice trends for each plant species and to help explain the observed similarity, the codon usage tables for all the five-plant species were studied. Though the overall coding strategy in Arachis appears similar to that of other dicots, there is reason to believe that based on comparison with those legume species with large-scale public repositories, Arachis is closer to Lotus, from which Medicago is more distant and soybean the most distant. While the data presented here is from the complete protein coding sequences available in GenBank, and not from individual genes, they still provide an overall picture of the relationships between the five dicots and in particular the differences amongst the legumes. The observed similarities correlate with relationships proposed from the sequence analysis data. This data can be a useful consideration when studying the levels of gene expression in these plants. We anticipate that these sequences and their annotations will prove useful for those interested in plant comparative genomics in general, and for legume researchers and molecular breeders in particular. 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