Institute of Biological Sciences, Edward Llwyd Building, University
of Wales, Aberystwyth, Ceredigion, SY23 3DA, United Kingdom
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INTRODUCTION |
The past two decades have witnessed
an explosion in the use of model eukaryotic organisms to aid studies on
species of significant commercial or biological interest. Historically,
specific eukaryotes (e.g. Saccharomyces cerevisiae and
Caenorhabditis elegans) have attained the status of
"models" because they reflect the individual characteristics of
species of medical, industrial, or agricultural interest and are often
small, easy to work with in large numbers, and cheap to maintain. More
recently, the power of model species has been augmented by the
development of whole genome sequencing programs. The new field of
"functional genomics" provides further challenges for model
organisms in the drive to understand the function of each gene in any
genome. This requires a plethora of tools to allow an integrative
examination of complex biological problems and relate phenotype to
genotype. There are two distinct categories of technology that need to
be in place to exploit fully any proposed model organism in a
functional genomics program (Table I).
The technology associated with "physical genomics" is often standardized, generally organism independent, and can be developed theoretically for any species, given sufficient investment of time and
resources. In contrast, the "biological genomics" capability associated with any particular organism is species dependent reflecting genome size, organization and degree of redundancy, breeding behavior, and in many cases, the development of gene transfer procedures and
mutagenesis strategies (e.g. transposon tagging and gene trapping technology). Pragmatically, the utility of a model organism is dependent also on its possession of a range of biological features, for
instance, small physical size, rapid life cycle, and undemanding growth
requirements that make it amenable to high-throughput screening routines. Such characteristics allow easy adoption by many laboratories internationally, which accelerates the process of discovery and the
development of bioinformatic tools (e.g. sequence databases) that are
essential to the success of a functional genomic program.
All these features are exemplified in what is without doubt the most
highly developed plant model system, the dicotyledon Arabidopsis
(Meyerowitz and Sommerville, 1994
; Meinke et al., 1998). This species
is a small crucifer that is an inbreeding annual with a rapid life
cycle (Redei, 1970). The Arabidopsis nuclear genome size has been
estimated by flow cytometry to be 164 Mbp (Bennett et al., 2000),
whereas a recent calculation following completion of the whole genome
sequence (The Arabidopsis Genome Initiative, 2000) has indicated a
figure as low as a 125 Mbp. However, phylogenetically, Arabidopsis is
only distantly related to the Poaceae, which includes all of the
world's major cereals crops and forage grasses (Keller and Feuillet,
2000). Hopes that Arabidopsis could serve as an "anchor" genome to
help locate important chromosomal locations in cereal species have not
been substantiated by recent studies (Bennetzen et al., 1998; Devos et
al., 1999). Thus, it is clear that grass (Poaceae) model systems are a
key requirement for the future identification of genes of agronomic interest from cereals and forage grasses.
With its international status as a staple food source and many years of
intensive plant breeding, rice (Oryza sativa), with its
compact genome (approximately 441 Mbp; Bennett et al., 2000) has been
promoted as a model for cereal genomics (for review, see Havukkala,
1996; Goff, 1999). Considerable international effort has developed rice
genetic maps, expressed sequence tag programs, and assembled a
considerable germplasm collection (highlighted in McCouch, 1998), and
the completed rice genomic sequence has just been announced (Dickson
and Cyranoski, 2001). Furthermore, the representation of all grass
genome sectors by less than 30 linkage blocks (with centromeric sites
often defining the breakpoints) within a consensus grass map
"anchored" by reference to the rice genome offers the prospect of
easing mapping in cereals with larger genomes (Gale and Devos, 1998).
However, the value of rice as a model for the temperate cereals and
forage grasses in the relatively distantly related Pooideae subfamily
(see Fig. 1A) may be, on occasion,
questionable. For instance, to effectively use the rice genomic map to
isolate a corresponding genic region in the larger genomes of temperate
cereals, "microsynteny" will have to be conserved at the size of
DNA inserts found in bacterial artificial chromosome (BAC) or
yeast artificial chromosome (YAC) clones (approximately 100 kb and 0.5 Mb, respectively). This does not always appear to be the case. For
example, although the Sh2 locus appears to be colinear in
many cereals (Chen et al., 1997), regions flanking Adh1
locus from maize (Zea mays), sorghum (Sorghum
bicolor), and rice were dissimilar (Bennetzen et al.,
1998), and molecular analysis has detected multiple small
rearrangements (Tikhonov et al., 1999). Also the "physical and
biological genomics" infrastructure, though impressive, is
incomplete. For instance, large scale, organized, and publicly
available insertion mutagenesis resources (Izawa et al., 1997; Enoki et
al., 1999) are not yet available, and a routine transgenic capability,
even after decades of concerted effort, is restricted to a relatively
few laboratories. Furthermore, the simple logistics of handling rice
(as a large, outbreeding plant with a long life cycle and demanding
growth requirements) will complicate the future development of rice as
a model species for high-throughput functional genomics. Finally, and
crucially, rice does not necessarily exhibit all the traits that are
relevant to study in temperate crops, especially forage grasses. For
example, resistance to specific types of pathogens, overwintering and
freezing tolerance, vernalization, perenniality (including meristem
dormancy mechanisms), wear and injury tolerance (amenity grasses),
sward behavior, and post-harvest biochemistry of silage are all
important areas of research relevant to temperate grasses, which are
rarely studied in rice.
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Figure 1.
A, Schematic phylogenetic relationship of
B. distachyon to other Poaceae adapted from the
data presented by Catalan et al. (1995, 1997; Catalan and Olmstead,
2000). B, Nuclear genome sizes (Mbp/1C) in different grass
genera. Data derived from The Kew Gardens Angiosperm C-
value database
(http://www.rbgkew.org/cval/homepage.html).
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Against this background, it would seem appropriate to reexamine the
Pooideae to identify a grass species that has the potential to be
developed into a useful model representative of important temperate
cereals and forage grasses. The Kew Gardens Angiosperm C-
value Database (http://www.kew.org/cval/homepage.html) shows that the genus Brachypodium is distinct from other genera in
the Pooideae in that all species examined to date have a narrow range of genome sizes with the smallest 1-C values being very
similar to that of rice (Fig. 1B). Various molecular phylogenetic
analyses have demonstrated that the genus Brachypodium
diverged from the ancestral stock of Pooideae immediately prior to the
radiation of the modern "core pooids" (Triticeae, Bromeae, Poeae,
and Aveneae; see Fig. 1A), which includes the majority of important
temperate cereals and forage grasses (Shi, 1991; Shi et al., 1993;
Catalan et al., 1995, 1997; Catalan and Olmstead, 2000). Its
phylogenetic position and small genome size prompted Moore and
colleagues (Aragon-Alcaide et al., 1996) to use Brachypodium
sylvaticum (2n = 18) in a search for archetypal
grass centromere sequences by screening for repetitive DNA conserved
between wheat (Triticum aestivum), maize, and rice and
Brachypodium. Brachypodium species have small
chromosomes with a variable base number (x = 5, 7, 8, or 9),
making them unusual in the Pooideae that tend to have large chromosomes
and a base number of 7 (Shi et al., 1993). An analysis of ribosomal DNA
structure revealed that Brachypodium had the smallest (150 bp) 5S rDNA spacer region found in the grasses (Shi, 1991; Catalan et
al., 1995) and a very simple rDNA repeat unit with a low degree of
methylation (Shi et al., 1993). Further characterization revealed that
genomes of Brachypodium species contained typically less
than 15% highly repeated DNA (Shi, 1991; Catalan et al., 1995).
Therefore, we consider that the genus Brachypodium has
several attributes in relation to its ancestry and genome
characteristics that make it a useful focus for studies relating to the
evolution of form and function in the Pooideae. The present paper
describes the development of B. distachyon, the
only true annual species within the genus Brachypodium, as a
potential model species for functional genomics and a representative of
the temperate cereals and forage grasses.
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RESULTS |
Diploid Ecotypes of B. distachyon Have the Smallest
Reported Genome Size in the Poaceae
The genome size of several species of Brachypodium was
estimated in preliminary studies by scanning densitometry of
Feulgen-stained nuclei prepared from root tip squashes (Table
II). Representative accessions of each
species had a 1C nuclear genome size of less than 0.5 pg,
equivalent to 
410 Mbp. Of particular note was the large discrepancy
between the genome sizes of two ecotypes of B. distachyon ABR99 and ABR1 (0.3 pg/1C and 0.15 pg/1C, respectively).
Propidium iodide was used to stain nuclei isolated from our collection
of 52 ecotypes of B. distachyon, and their genome
size was determined by flow cytometry (Dolezel et al., 1989, 1998). To
estimate genome size, the flow cytometer was calibrated against stained
nuclei prepared from representative species with known genome sizes
(Bennett et al., 2000). This analysis (Table II) revealed that the
genome size in several B. distachyon accessions was indistinguishable from that of Arabidopsis, which is taken to be
164 Mbp/1C.
Diploid B. distachyon Has a Simple, Distinctive
Karyotype and Displays High Levels of Recombination
Somatic metaphase chromosomes were examined in seven ecotypes of
B. distachyon (ABR1-ABR7), which had all been
found to have a genome size of less than 175 Mbp. The analysis revealed
that their karyotypes were morphologically the same (Fig.
2A), which justified the construction of
a consensus karyotype for this species. The chromosomes have been
arranged in descending order of short-arm length and were designated 1 to 5, in accordance with normal conventions. Chromosome 1 is
submetacentric, distinctly the largest of the complement, and unlikely
to be confused with chromosome 2, which is more acrocentric and
considerably smaller. The short-arms of chromosomes 2 and 3 are of
similar length, but 3 is shorter and characteristically the only
metacentric of the complement. Chromosome 4 shares similar features
with 3, which could ordinarily be the source of potential mislabeling.
However, FISH reveals that chromosome 4 only has a major 5S rDNA locus,
which is proximally located in its long-arm (Fig. 2, B and C).
Chromosome 5 is acrocentric and by far the smallest of the complement.
In addition, it is the only chromosome to bear a major 45S rDNA locus,
which occupies a distal site in the short arm (Fig. 2, B and C). In
summary, each chromosome has diagnostic features enabling unequivocal
identification of every chromosome of the complement (Fig. 2D).
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Figure 2.
Somatic and meiotic chromosomes of B. distachyon ABR1 showing light micrograph of the somatic
chromosome complement (A) in which the five pairs of chromosomes are
readily identified and fluorescence in situ hybridization (FISH; B) of
5S rDNA (red) and 45S rDNA (green) to the five pairs of somatic
chromosomes. C, Karyogram derived from the image shown in B. D,
Idiogram showing the distinctive and diagnostic shapes and lengths of
the haploid set of chromosomes. The sites of the two rDNA loci are
indicated. E, Light micrograph of two pollen mother cells at metaphase
I. Note the five ring bivalents in each. Bars = 10 µm.
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Examination of 20 pollen mother cells at metaphase I of one ecotype
(ABR1) revealed that 16 form five ring bivalents and four form four
ring bivalents and one rod involving chromosome 5 in all cases. Two
example cells are presented in Figure 2E, which also clearly shows that
chiasmata are not strictly localized to any particular region of the chromosomes.
Diploid B. distachyon Ecotypes Display Growth and Life
Cycle Characteristics Suitable for High-Throughput Genetics
Preliminary experiments established that all ecotypes performed
well under standardized conditions (see "Materials and Methods"). The B. distachyon ecotypes were then
characterized in terms of size at maturity, general growth habit,
vernalization requirement, duration of life cycle, and amount of seed
set. ABR1 was typical and exhibited undemanding maintenance
requirements, growing successfully under sterile conditions in glass
jars (Fig. 3A) on vermiculite supplemented with 0.5× Hoagland solution (Draper et al., 1988) or at
high-density (2,000 seedlings 18- × 30-cm
tray
1) in compost (Fig. 3B). With only two
exceptions (ABR13 and ABR15), all of the diploid ecotypes (including
ABR1) benefited from a standard vernalization treatment (6 weeks at
5°C) to ensure synchronous induction of flowering and synchronized
embryo development. Floral spikelet emergence occurs around 3 to 4 weeks after removal from the cold room (Fig. 3C). By 4 to 5 weeks
following vernalization, visible anthesis occurs (Fig. 3D) with each
spikelet eventually containing typically around 10 to 12 seeds. At
maturity (4-5 mo), the diploid ecotypes ranged from 15 to 30 cm in
height and very rarely shed any seed prematurely, thus aiding easy
harvesting (Fig. 3E; Table IV). For all polyploids and two diploid
ecotypes (ABR13 and ABR15), flowering is accelerated by approximately 6 weeks, as no vernalization stage is required (see Table IV).
Furthermore, the smaller stature of B. distachyon
compared with, for instance, rice (Fig. 3F), allows typical planting
densities of at least 300 plants square meter1
in ordered arrays (Fig. 3G) for M2 mutant seed production or M3 mutant
screening.
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Figure 3.
Growth habit and anatomy of the diploid
B. distachyon ecotype ABR1 grown in glass jars
(A) on vermiculite supplemented with 0.5× Hoagland solution (Draper et
al., 1988) at 1 week (left jar) and 2 weeks (right jar), and at high
density (B) in 30- × 18-cm trays grown on 1:1 mixes of
Levington's:gravel. Bar = 5 cm. Flower morphology (C) prior to
dehiscence and indicating hairy palea (p) and lemea (l), stigma (s),
and anthers (a). Bar = 1 mm. Each plant has 6 to 10 flowering
spikes that actually set seed and seed heads (D) have a
"brome-like" appearance and typically carry 10 viable seeds.
Bar = 4 mm. At maturity (E), ABR1 plants were 15 cm high with
short nonrhizomatous roots. Bar = 5 cm. F, B. distachyon ABR1 (8 weeks post-sowing) is compared in size
with rice cv IR64 (20 weeks post-sowing). G, 2,000 M1 progeny of
 -irradiated (at the Vienna Atomic Energy Institute) B. distachyon seeds grown under typical temperate greenhouse
conditions.
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B. distachyon Is Readily Responsive to Tissue
Culture
The diploid ecotype ABR1 was chosen for initial tissue culture
studies as it was relatively compact and offered a high throughput of
immature embryos for minimal growth space. A detailed analysis of
embryo development in individual B. distachyon
spikelets (Fig. 4A) revealed, as
expected, a variation in maturity, with more mature embryos present in
the center at 10 to 15 d post-visible anthesis (data not shown).
Isolated immature embryos were divided into one of five size classes
(types 1-5; Fig. 4, B and C) and were placed on callus induction media
(LS 2.5 and N6 2.5; Bablak et al., 1995), and typically after 10 to
15 d had formed a mass of callus on the surface of the scutellum
(see Fig. 4, D and E). This included large areas of creamy-white, type
II embryogenic tissue (dry, friable, and pale) easily identified by
scanning electron microscopy (Fig. 4F). Immature embryos with the
greatest potential for somatic embryogenesis were in the size range of 0.3 to 0.7 mm (see Table IIIA) and were
generally off-white with a translucent scutellum margin and were
suspended in a soft endosperm (see Fig. 4, B, class 2 and C, class 3).
LS 2.5 medium proved superior for the induction of embryogenic callus,
with around 45% of isolated embryos responding within this size range
(Table IIIA). Type II callus could be separated from callus growing on the original explants and maintained on LS 2.5 for up to 9 to 12 mo
after which it was normally discarded.
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Figure 4.
Tissue culture and transformation of B. distachyon. A, B. distachyon ABR1 seed
head at 15 d postanthesis (bar = 4 mm) from which (B)
isolated seeds have had their paleas and lemmas removed (embryos
arrowed, bar = 0.5 mm) or (C) the embryos are isolated from
endosperm to indicate embryo development (classes 1-5, bar = 0.5 mm). D, Scanning electron micrograph showing immature embryo structure.
Indicated are the coleoptile (col), scutellum (scut), radical (rad),
and coleorhiza (chz). Bar = 0.1 mm. E, Embryogenic callus (c)
formation around the edge of the scutellum (scut) after 15 d of
culture (bar = 0.1 mm), which (F) scanning electron micrography
revealed to contain many organized structures with a distinctive
embryoid shape (arrowed; coleoptilar pore; bar = 20 µm). G,
Propagated embryogenic callus of ABR100 stained for GUS activity
24 h following biolistic bombardment with pACt1GUSHm. Bar = 1 mm. H, Selection of ABR100 transgenic tissue on Hm- (40 µg
mL1) selective media. Bar = 3 mm. I, The
second subculture of regenerating plants from bombarded embryogenic
callus of ABR100 on selective media. Bar = 5 mm. J, Isolated
Hm-resistant plantlet of ABR100 exhibiting tiller formation. Bar = 5 mm. K, Hm-resistant ABR100 shoot stained for GUS activity (bar = 1 cm). L, Rooted T0 transgenic lines in soil
producing viable seeds. M, The PCR amplification of hgh gene
internal sequences (516-bp product) from five independent
T1 transgenic lines (1-5). N, Southern blot of
BamHI-digested genomic DNA from T1
transgenic lines (1-5) and wild-type ABR100 probed with hgh
sequences. Indicated is the 1.07-kb BamHI internal
hgh gene fragment.
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The regeneration potential of type II callus after subculture on LS 2.5 (approximately 6 weeks) was examined by inoculating onto a range of
established regeneration media. Plantlets were produced on all media
tested, with the highest regeneration potential realized on MS0 and N60
(Table IIIB). Although embryogenic callus could be obtained at a high
frequency when immature embryos were placed on LS 2.5 or N6 2.5 media,
albino shoots were recovered at a much higher frequency from tissues
maintained on N6 2.5 (45% compared with 7% on LS2.5), and thus
LS 2.5 was used for all future work on transformation.
Transgenic Plants Can Be Recovered at a High Frequency from
Embryogenic Callus Using Microprojectile Technology and Hygromycin
(Hm) Selection
Tissue from the hexaploid accession ABR100 remained highly
embryogenic when maintained on LS 2.5 medium and so was used to bulk up
material for development of transformation technology. Embryogenic
callus from ABR100 was bombarded with microprojectiles loaded with
the plasmid pACt1-GUSHm (pAGH). A small sample of bombarded callus
tissue with well-dispersed cauliflower mosaic virus
35S-
-glucuronidase (GUS) activity is shown in Figure 4G. One week
after bombardment, callus was subcultured to LS 2.5 medium containing
40 mg L1 Hm where it rapidly became brown and
necrotic, but after 2 weeks, small nodes of actively growing cells were
visible. Once these had developed to a diameter of 1 to 2 mm, these
tissues were transferred twice at weekly intervals for further growth
on selection medium containing 40 mg L1 Hm. In
typical experiments, an average of seven Hm-resistant clones were
recovered per gram of target tissue (Table IIIC).
Hm-resistant calli were removed from selection plates and were
transferred onto regeneration medium (see "Materials and Methods") containing 30 mg L1 Hm and they produced
plantlets within 7 to 10 d (Fig. 4H). Callus containing young
shoots and viable somatic embryos were transferred subsequently to
germination medium (MS0) and were incubated in the light. An average of
five Hm-resistant plants were recovered per gram of bombarded tissue
(Table IIIC). The formation of roots was initially rather poor on the
regeneration medium (Fig. 4I), but a well-developed root system could
be produced following further subculture on the same hormone-free media
once the plantlets had been separated from necrotic tissue (Fig. 4J).
Histochemical staining with 5-bromo-4-chloro-3-indolyl--glucuronic
acid of regenerated plantlets surviving on Hm revealed clear evidence
of GUS activity (Fig. 4K). All rooted plants that were established
successfully in soil produced fertile flowers and set seed (Fig. 4L).
T1 progeny of five independent transgenic lines
were examined for the presence of the Hm gene by PCR and Southern
blotting to confirm that stably transformed lines had been generated.
PCR amplified a 516-bp fragment from all transgenic lines (Fig. 4M),
which hybridized to a hgh probe following Southern blotting
(data not shown). In addition, probing BamHI-digested
genomic DNA extracted from these transgenic lines with a hgh
probe indicated hybridization to a 1.07-kb fragment that corresponded
to the size predicted from the plasmid used for the initial bombardment
(Fig. 4N).
B. distachyon Displays Traits That Are Important for
Temperate Cereal Research
We have characterized the responses of B. distachyon ecotypes to challenge with a range of pathogens
that are the cause of significant crop loss in cereals. Blumeria
graminis is the causal agent of powdery mildew on cereals and
occurs in several forma specialis (f. sp.). Isolates of
B. graminis f.s.p hordei, avenae, and
tritici were used to challenge ecotypes (ABR1-ABR7 and
ABR100) of B. distachyon and failed to elicit
disease symptoms that were observable to the naked eye. However, light
microscopic examination revealed single epidermal cell death and also
papillae-based resistance that are typical of a hypersensitive response
(Fig. 5A). Attempts to isolate a
Blumeria sp. capable of establishing an infection on
B. distachyon by exposing plants to the outdoor
environment have, to date, been unsuccessful.
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Figure 5.
Targets for B. distachyon
research. Responses to pathogen challenge and grain development. A, The
responses of ABR1 to challenge with condiophores of Blumeria
graminis f. sp. Triticae. Bar = 0.1 mm. Arrowed
are the condiophore (c), appressorial germtube (a) and papillae
formation (p) and single cell-death (d) in the host cell. Challenging
with Puccinia striformis f. sp. triticae (wheat
yellow stripe rust) elicits (B) localized necrotic flecking on ABR105
and (C) yellow uridea (pustule) formation on ABR100 that develop from
(D) extensive areas of necrotic tissue. (Uridea forming within the
necrotic tissue are arrowed.) E, Variable responses by B. distachyon ecotypes to challenge with M. grisea Guy-11. F, Comparison of mature seed size and
morphology of B. distachyon ABR1 with rice and
wheat cv Kalyansona). Embryos are arrowed on each seed. Bar = 2 mm.
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The responses of B. distachyon ecotypes
(ABR1-ABR7, and ABR100, 101, 105, and 113) were examined following
challenge with the rust pathogens Puccinia reconditia f. sp.
hordei and f. sp. triticae (barley and wheat
brown rust, respectively) as well as P. striformis f. sp. hordei and f. sp.
triticae (barley and wheat yellow stripe rust,
respectively). ABR100 displayed a "brown flecking" (BF) following
challenge with wheat brown rust strains with all other tested ecotypes
eliciting no macro- or microscopic responses. Ecotypes ABR1, ABR3,
ABR100, and ABR105 also exhibited BF symptoms with barley brown rust
strains. In contrast, all ecotypes exhibited some form of visible
response to wheat and barley yellow stripe rusts ranging from BF
(ABR1-ABR7, and 101 and 111; Fig. 5B) or the more extensive "brown
tissue" response. It is interesting that ABR100 and ABR105 displayed
uridinea (raised pustule) formation (Fig. 5C), indicating that the
fungus has successfully colonized the host, though these formed within
areas of extensive necrosis (Fig. 5D).
A range of symptoms were also elicited (Fig. 5E) following challenge of
B. distachyon ecotypes (ABR1-ABR7) with the
causal agent of rice blast, Magnaporthe grisea (strain
Guy-11). On ABR7 and ABR1, an extensive and spreading necrosis was
observed that was reminiscent of blast symptoms on rice. In contrast,
highly localized necrotic lesions formed on ABR5 that did not change significantly in phenotype over time and were consistent with the
exhibition of full resistance to M. grisea
Guy-11.
Seed development in B. distachyon has yet to be
extensively analyzed. However, in terms of overall size and external
anatomy, mature seeds of the diploid ABR1 are very similar to those of the major grain crops rice and wheat, the only major structural difference being a smaller endosperm volume in B. distachyon (Fig. 5F).
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DISCUSSION |
New "post-genomic" techniques are offering increasingly
powerful ways to link plant phenotype to the transcriptome, proteome (Gura, 2000), or the metabolome (Fiehn et al., 2000), allowing the
development of a "blueprint" of plant form and function (Chory et
al., 2000). Optimal exploitation of these technologies is dependent on
possession of suitable model species. It is now becoming clear that
Arabidopsis cannot be considered as an ideal model for the grasses
(Devos et al., 1999; Tikhonov et al., 1999; Keller and Feuillet, 2000),
and there is significant international effort to develop rice as a
model species more suitable for the Poaceae (Havukkala, 1996; Goff,
1999). However, against this background, the limitations of rice to
provide such a model and the complementary opportunities offered by
other species needs to be recognized.
Analysis of the B. distachyon Genome Will Provide a
Valuable Resource for Physical Genomics in Temperate Cereals and Forage
Grasses
Differing analytical techniques pose different problems when
attempting to estimate genome size. The commonly used flow cytometry technique is dependent on accurate calibration, and even apparently definitive DNA sequencing approaches do not easily include regions of
highly repeated sequence and may therefore underestimate genome sizes.
Nevertheless, we have taken The Arabidopsis Genome Initiative (2000)
estimate (approximately 125 Mbp) as the more accurate and, given that
we failed to distinguish any size difference between diploid
B. distachyon ecotypes and Arabidopsis genomes by
flow cytometry (Table IV), we propose
that they should be considered to be approximately the same. This
genome size is somewhat at odds with a previous report
(4C = 3 pg; Bennett and Leitch, 1995). However, our
present data suggest the presence of a polyploid series within
B. distachyon (2x = 10, 4x = 20, and
6x = 30) and, therefore, the discrepancy can be explained by the
fact that these authors used a hexaploid accession for their
determination (e.g. ABR100 2n = 6x = 30, 4C approximately 2.6 pg, derived from Table II).
The flow cytometry screen identified 12 diploids, eight
tetraploids, and 32 hexaploids in our germplasm collection.
We recognize that the utility of B. distachyon
will be augmented by the development of genetic and physical chromosome
markers. Given the small chromosome size in this species, there is a
surprisingly high chiasma frequency of at least 9.8 cell1. Furthermore, this chiasma frequency is
likely to be an underestimate because of the technical problem of
resolving more than one chiasma per chromosome arm at this meiotic
stage. Thus, we expect that genetic maps of B. distachyon could be quickly generated given its high
crossover frequency and given the development of high-throughput markers such as single nucleotide repeats (Ellis, 2000). In diploid B. distachyon ecotypes, the five pairs of
chromosomes are sufficiently dissimilar to enable positive
identification in routine squash preparations of somatic tissue.
Meiotic prophase chromosomes are amenable to study in B. distachyon, and provide longer substrates for the
hybridization in situ of fluorescent probes. Thus, it should be
possible also to physically map DNA probes from large insert libraries
(such as BACs) to meiotic prophase chromosomes and DNA fibers, as has
been achieved in tomato (Lycopersicon esculentum; Zhong et al., 1999). If the chromosomes are probed simultaneously with
landmarks such as rDNA and pericentromeric repeats originally isolated
from B. sylvaticum (Abbo et al., 1995), it should
be possible to construct rapidly physical linkage maps and assign contiguous megabase tracts of DNA to particular chromosome arms. Such
an approach may aid future programs requiring the targeted sequencing
of specific regions of the B. distachyon genome.
As publicly available rice genomic sequences from the International Rice Genome Sequencing Project are only available for around 25% of
the rice genome, with the more complete sequence only available through
"research contracts" with Syngenta (Dickson and Cyranoski, 2001),
then the rapid generation of sequence information from the
B. distachyon genome could have great utility in
the academic community.
The genus Brachypodium is considered a sister group to the
"core pooid" clade, which contains all of the important temperate cereals, fodder grasses, and amenity grasses. We further propose that
B. distachyon, by occupying this key phylogenic
position and by virtue of its exceedingly "compact genome"
(allowing representation by a very small genomic library), could
provide a significant resource for the analysis of the much bigger
genomes possessed by important temperate grasses. For example, to aid
long-distance chromosome walking and quantitative trait loci
analysis in cereals with large genomes, mapping information from one
grass genome can theoretically be used to locate a likely syntenic (or
colinear) region represented in BAC/YAC clone contigs from a cereal
with a smaller genome (Moore et al., 1993). In reality, there are as yet very few examples of this approach being successful (e.g. Chen et
al., 1997), which is due largely to the breakdown of genome colinearity
at the microsyntenic level (e.g. 50 Kb-1 Mb) where the species are
relatively distantly related (Foote et al., 1997). However, considering
the phylogenetic position of Brachypodium in the Pooideae,
microsynteny is likely to be relatively more conserved within this
subfamily and thus B. distachyon could provide an
archetypal map specifically for pooids to which other colinear genomes
could be aligned. In practical terms, physical markers linked only
loosely to important traits in the large genomes of species such as
wheat and barley (Hordeum vulgare) might be located to relevant B. distachyon genomic library clones
to provide rapid access to syntenic genomic regions.
Biological Characteristics Indicate That B. distachyon
May Be Amenable for Large-Scale Mutagenesis Programs
Mutagenesis is commonly used to relate genotype to phenotype.
Large-scale mutagenic techniques may employ chemical, physical, or
genetic mutagens, and the latter especially has proved a powerful tool
for gene tagging in Arabidopsis (for example, Tissier et al., 1999).
Successful mutagenesis of a plant species is dependent on a small
diploid genome, available mapping strategies, ease of crossing,
transformability, and not inconsequential features such as a small
physical stature, a rapid life cycle, and good seed yield, which eases
mutant screening and collecting selected lines (Vizir et al., 1996).
Table IV illustrates how Arabidopsis fulfills all these requirements,
but B. distachyon also scores highly. As stated
above, genetic maps now can be generated relatively quickly, and so the
only remaining unfavorable feature is the smaller seed yield compared
with Arabidopsis. However, compared with rice, B. distachyon has a more rapid life cycle, smaller stature, and
an inbreeding reproductive strategy with anthers and stigmas enclosed
tightly within the palea and lemma. The latter makes crossing different
plants slightly more demanding technically. Floral spikelet emergence
proved to be the best stage to remove the three anthers and apply
pollen to the stigmas when conducting crossing experiments. However,
this inbreeding reproductive behavior and the absence of seed head
"shatter" in most B. distachyon ecotypes means that F1 seed can be collected without the
need for hand pollination or the time-consuming bagging of flowering
plants. Thus, individual plants do not have to be isolated when grown in large populations to avoid outcrossing, which is a great advantage for mutagenesis studies. We have already generated -irradiated populations, and transposon-based mutagenic approaches are under development (J. Draper, L.A.J. Mur, G. Jenkins, and P. Bablak, unpublished data).
B. distachyon, A Potential High-Throughput
Transformation System
A key technology for a model plant species is the availability of
a facile transformation system. For many dicot species, high efficiency
Agrobacterium tumefaciens-mediated transformation is well
established, but though the approach has been used to generate
transgenic rice (Chan et al., 1992), wheat (Mooney et al., 1991), maize
(Gould et al., 1991), and barley (Tingay et al., 1997), this technique
is far from routine. For Poaceae, particle bombardment of embryogenic
callus followed by selection of transgenic tissue (for review, see
Potrykus, 1990; Hansen and Wright, 1999) has proven robust and has been
used to transform maize (Klein et al., 1989; Fromm et al., 1990), wheat
(Vasil et al., 1991), and rice (Cao et al., 1992). Nevertheless, the
number of publications describing the use of transgenic cereals or
forage grasses for basic studies in biology is still very limited in
comparison with dicots. The success of the transformation techniques is
dependent upon the optimal culture of highly embryogenic callus (Hansen and Wright, 1999). This is derived commonly from immature zygotic embryos, as this tissue is very responsive to in vitro culture and has
a high plant regenerative capacity. Immature embryos from B. distachyon were not an exception. Large numbers of immature embryos can be isolated from B. distachyon plants
grown under simple greenhouse conditions, without the need for
specialist environmentally controlled growth chambers. For example, a
single 18- × 30-cm tray containing 24 flowering plants can provide
sufficient embryos to supply embryogenic cultures for a single
researcher for 1 mo. The low frequency of gross morphological
abnormalities (e.g. albinism and male sterility) suggested that
significant somaclonal variation did not occur under the culture
conditions used. Based on this behavior in tissue culture, we report a
transformation system for a hexaploid ecotype of B. distachyon that is comparable with the best rice systems
currently available in terms of ease of use and final transformation
efficiency (Tables IIIC and IV; Li et al., 1993; Biswas et al., 1998).
As testing a particular transgene in wheat can still take up to 5 years
(Dunwell, 2000), given the rapid life cycle of B. distachyon, our development of a facile, low-cost
transformation system will offer a rapid "test bed" for transgenic
studies in grasses. We also demonstrate that embryogenic callus can be
generated routinely from several diploid ecotypes, and current
experiments aim to develop transposon tagging and gene trapping
resources in diploid ecotypes of B. distachyon (J. Draper, L.A.J. Mur, G. Jenkins, and P. Bablak, unpublished data).
B. distachyon Displays Many Traits That Are
Relevant for Cereal and Forage Grass Improvement
In considering a potential model for temperate cereals, the value
of any plant species obviously depends on whether the particular organism displays key traits representing those targeted currently in
plant breeding and biotechnology programs. Crop loss through pathogen
attack is significant and represents a key aspect for research. We also
note that in simple practical terms, a small plant, which is easy to
maintain and which will support several classes of important cereal
diseases may find utility in fungicide screening programs. All ecotypes
of B. distachyon tested appeared to exhibit
single cell death and papillae formation following challenge with
powdery mildew pathogens adapted to cereals. These responses are
symptomatic of resistance in other grass/cereal species (Carver et al.,
1995) and may be indicative of lack of race structure. The molecular
basis of such "non-host" HR is being investigated in model dicots
(e.g. Lauge et al., 2000), and B. distachyon
could serve in a similar role for the Poaceae, where race-specific
resistance exhibits little longevity in the field. Different ecotypes
of B. distachyon exhibited great variability in
response to infection with individual rust species ranging from no
visible symptoms or BF associated with a HR, to pustule formation
(albeit associated with necrotic tissue). These data suggest that
B. distachyon may prove to be a useful host for
future studies on the molecular biology and genetics of these important plant-pathogen interactions. In contrast, we observed clear evidence of
susceptibility and resistance exhibited by different ecotypes to
challenge with Magnaporthe grisea Guy-11 and additionally, the phenotypes closely resembled those observed on rice cultivars (data
not shown). M. grisea is undoubtedly one of the
most virulent and economically devastating plant pathogens, causing
losses of between 11% and 30% of the annual world crop and
representing up to 157 million tons of rice (Baker et al., 1997). Thus,
we are extensively characterizing the B. distachyon/M. grisea pathosystem to identify key
resistance determinants and to understand defense-associated signaling
(A.P.M. Routledge, L.A.J. Mur, and G. Shelley, unpublished data).
An even more important trait than pathogenic interactions for a
Pooid model is the analysis of genetic and biochemical events underlying grain-filling and quality. The large size of the seeds in
the genus Brachypodium has been highlighted previously
(Catalan et al., 1997) and there have already been some basic studies
on seed storage proteins (Khan and Stace, 1999). Thus, it is
envisaged that resource allocation, grain filling, and endosperm
development in particular will be a valuable focus for mutagenesis
program in B. distachyon. Further features,
including freezing tolerance, perenniality, repetitive injury (mowing
and trampling) tolerance, meristem dormancy mechanisms, post-harvest
biochemistry of silage and hay, mycorrhizae, and sward ecology
all of
which are important to temperate forage grasses and many temperate
cerealsare traits that are not exhibited by or are difficult to study
in rice, but are possible targets for functional genomics in
Brachypodium.
In summary, the present data demonstrate that B. distachyon has great potential to be adapted for
high-throughput genetics. In many aspects of its biology such as genome
size, chromosome number, height, planting density, breeding system, and
duration of life cycle, it is very similar to Arabidopsis. We propose
that B. distachyon is best seen as a
complementary model to rice offering, as it does, the opportunity to
study grass traits that are not well exhibited by rice. In
addition, the simpler logistics of handling large B. distachyon populations, as compared with rice, may well make
B. distachyon an attractive prospect where
investigative resources, such as access to controlled growth
environments, are limited.
| |
MATERIALS AND METHODS |
Plant Growth Conditions
Full details of all Brachypodium distachyon
ecotypes can be found at
http://www.aber.ac.uk/plantpathol/Brachyomics. Seed
samples of different Brachypodium ecotypes were obtained
from Brachyomics (Botany Gardens, Aberystwyth, Ceredigion, UK) under a
"Research Only" Materials Transfer Agreement. All B.
distachyon ecotypes were grown under a 16-h light period
at 23°C ± 2°C. The plants were illuminated with 55W (Osram,
Sylvania, Munich) high-frequency lighting tubes (4,580 lumen
output) and were supplemented with 2 × 30W clear tube cooled
lighting (Osram) and placed between 60 and 100 cm of the light bank.
Light intensities always exceeded 10 µmol m2
s1. Plants were grown routinely on Levington's Universal
Compost (Levington Horticulture, Suffolk, UK) supplemented with gravel (the longest axis was approximately 0.5 cm) to approximately 50% (v/v)
to improve drainage. Plants were usually watered at 2-d intervals and
were never allowed to stand in water.
Nuclear Genome Size Estimations: Scanning Microdensitometry and
Flow Cytometry
For microdensitometry, root tips were fixed in 4% (w/v)
formaldehyde for 2 h, and were then washed with distilled water
prior to acid-hydrolysis by treatment with 5 M HCl at
20°C for 45 min. Following washing with distilled water, Feulgen
stain was added and the samples were kept in the dark for 45 min. The
stain was washed off with SO2 water, and then root tip
squashes were prepared. The density of well-stained prophase nuclei was
scanned using an M86 scanning microdensitometer (Vickers Instruments,
York, UK). The relative amount of DNA in each nucleus was calculated using the following formula: absorbance units of test
species/absorption units of a standard species × 4C value of standard species = 4C value of test species. Mung bean (Vigna radiata var.
Berken Mung Bean; 2C = 1.05 pg) was used as the
standard species (seeds supplied by W. Atley Burpee Seed Company,
Leicester, UK).
Nuclei were isolated for flow cytometry using the chopping technique
developed by Galbraith et al. (1983) using LB01 buffer at pH 7.5 (Dolezel et al., 1989, 1998) supplemented with 50 µg mL1 propidium iodide and 50 µg mL1 RNase
(Sigma, Poole, UK). The fluorescence of stained nuclei was analyzed
using PA or III flow cytometers (Partec, Münster, Germany).
Calibration standards (Bennett et al., 2000) used to estimate the
B. distachyon 1C genome
size were Lotus japonicus (approximately 445 Mbp;
Bennett and Smith, 1976), Aesculus hippocastanum (approximately 110 Mbp; Bennett et al., 1982), pea (Pisum
sativum; approximately 4,150 Mbp; Bennett and Leitch, 1997),
Arabidopsis (approximately 164 Mbp; Bennett et al., 2000), rice subsp.
indica cv IR34 (approximately 441 Mbp; Bennett et al.,
2000), and barley cv Sultan (approximately 4,116 Mbp; Bennett et al.,
2000).
Karyotyping and FISH
After flow cytometry experiments, seeds of seven putative
diploid accessions of B. distachyon
(ABR1-ABR7) were germinated on filter paper moistened with tap water
at 22.5°C in the dark. Whole seedlings with roots of about 1 cm long
were incubated in a saturated solution of 1-bromonaphthalene at 0°C
overnight, or in 2 mM aqueous 8-hydroxyquinoline for 1 to
2 h at room temperature. After washing and fixing for at least
2 h in a 3:1 mixture of methanol:acetic acid, root-tips destined
for bright-field microscopy were hydrolyzed in 1 M HCl at
60°C for 10 min, stained in Feulgen solution, and mounted in 2%
(w/v) orcein in 45% (w/v) propionic acid. Material for FISH was washed
after fixation in 10 mM citrate buffer and was digested for
1.5 to 2 h at 37°C in a mixture comprising 1% (w/v) cellulase
(Calbiochem, La Jolla, CA), 1% (w/v) cellulase (Onozuka RS, Yakult
Honsha C. Ltd., Tokyo), and 20% (v/v) pectinase (Sigma, St. Louis).
After washing, root-tips were detached and their meristems were
dissected out into 45% (w/v) acetic acid and squashed onto microscope
slides. Coverslips were removed by freezing and the preparations were
post-fixed in 3:1 ethanol:acetic acid, dehydrated in absolute ethanol,
and air dried. Immature inflorescences were fixed in Carnoy's
solution. Anthers at first metaphase of meiosis were macerated in
propionic orcein and squashed under coverslips. Somatic and meiotic
chromosomes were photographed onto Imagelink HQ microfilm
(Eastman-Kodak, Rochester, NY) with an MC100 camera attached to a
Axioplan microscope (Zeiss, Welwyn Garden City, UK), and they were
electronically scanned and processed in CorelDraw (Corel Corporation,
Ottawa, Ontario, Canada).
The 5S rDNA probe was amplified and labeled with rhodamine-4-dUTP
(Amersham Pharmacia, Uppsala) from the wheat clone pTa 794 (Gerlach and
Dyer, 1980), using PCR with universal M13 sequencing primers
under the following conditions: 94°C for 1 min, 35 cycles of 94°C
for 40s, 55°C for 40s, 72°C for 1 min, and 1 cycle of 72°C for 5 min. The 45S rDNA probe was obtained by nick translation with
digoxigenin-11-dUTP (Roche, Basel) of a 2.3-kb subclone of the 25S rDNA
unit of Arabidopsis (Unfried and Gruendler, 1990).
FISH was adapted with some modifications from Schwarzacher and
Heslop-Harrison (2000). In short, slides were pre-treated with RNAse
for 1 h at 37°C, post-fixed in 1% (w/v) aqueous formaldehyde in
phosphate-buffered saline buffer for 10 min, and dehydrated in an
ethanol series. Probe DNA was mixed to a concentration of 100 ng
slide1 with 50% (w/v) deionized formamide, 10% (w/v)
Dextran sulfate, 2× SSC, and 1% (w/v) SDS. The probe DNA was allowed
to hybridize with the chromosome preparations overnight at 37°C in an
Omnislide in situ hybridization system (Thermo Hybaid, Ashford, Kent,
UK). Slides were washed stringently in 20% (w/v) deionized formamide in 0.1% (w/v) SSC at 42°C, followed by detection of digoxigenin by
fluorescein isothiocyanate-conjugated anti-digoxigenin antibodies. The
chromosomes were counterstained with 4',6-diamino-phenylindole (2 µg
mL1), mounted in Vectashield (Vector Laboratories,
Burlingame, CA), and photographed onto Provia 400 color reversal film
(Fuji Photo Film, Tokyo) with an MC100 camera attached to a Axioplan
epifluorescence microscope (Zeiss, Jena, Germany). Images were scanned
electronically and processed using Micrografx Picture Publisher software.
Tissue Culture and Transformation
All media were as described previously by Bablak et al. (1995)
except, when required, maltose was substituted for Suc at a level of
30g L1. Immature embryos or callus material was viewed by
scanning electron microscopy as described previously (Bablak et al.,
1995). Seedlings were germinated and grown as described above, and
immature embryos were isolated from sterilized seeds (Bablak et al.,
1995) under a dissecting microscope approximately 14 d after
anthesis and their size was estimated (when required) using an
eye-piece graticule. Approximately 50 embryos were cultured in the dark
in a 9- × 1.5-cm petri dish containing 25 mL of LS 2.5 medium (Bablak
et al., 1995). After 4 weeks, the developed calli were detached from
the explants and were subcultured onto the same medium. In several
experiments, LS 2.5 was substituted with N6 2.5 or SH 2.5 (Bablak et
al., 1995). Type II callus (creamy-white, dry, and friable) was
constantly selected at each subculture to bulk up tissue for
regeneration and transformation studies. Media used for regeneration
were MS0; 190-2 (Lolium regeneration medium), MWW
(Winter wheat regeneration medium), and RM1 (Barley regeneration media;
Bablak et al., 1995).
For microprojectile bombardment, 1.0-µm gold particles were coated
with the plasmid and "fired" using the procedure described in the
PDS1000/He biolistic gun instruction manual (Bio-Rad, Hercules, CA).
The plasmid used was pACt1GUSHm (McElroy et al., 1991), which contained
an Hm-resistance gene (hgh) driven by a cauliflower mosaic virus 35S promoter (35S) for transformant selection and a
35S-GUS gene for transient transformation assays. In preliminary transformation experiments, it was discovered that the substitution of
Suc with maltose increased the regeneration potential of tissue bombarded with microprojectiles. The bombardment procedure was optimized by selecting conditions that achieved routinely >1,000 GUS-positive regions per target plate when examined by histochemical staining. Approximately 1.0 g fresh weight of embryogenic callus was centered in petri dishes containing LS 2.5 supplemented with 140 g L1 maltose and 2.5 g L1 of
Phytagel and incubated for 2 h. Calli were bombarded with a single
microprojectile firing using a PDS1000 particle acceleration device
(Bio-Rad) with a helium pressure of 1,300 psi, under a chamber pressure
of 27 mm Hg at a distance of 13 cm below the microprojectile stopping
plate. For transient assays, calli were stained for GUS activity
(Warner et al., 1993) after 24 to 36 h, and only callus batches
that exhibited 1,000 blue GUS spots or more were used for stable
transformation experiments. For stable transformation, all target
materials were bombarded once with pACt1GUSHm and were then transferred
to LS 2.5 (with maltose as a carbon source) for 1 week in the dark at
25°C. Bombarded calli were then transferred to the same medium
supplemented with 40 mg L1 Hm (Duchefa, Haarlem, The
Netherlands). Two weeks later, growing tissue was picked out and
transferred to fresh medium containing 40 mg L1 Hm, a
process that was repeated twice at 7 d intervals. Resistant calli
were transferred to regeneration medium (LS containing 0.2 mg
L1 kinetin, 2.5 g L1 Phytagel, and
30 g L1 maltose) containing 30 mg L1
Hm. After 5 to 7 d, the callus sections containing germinating shoots and viable embryos were transferred onto MS0 medium (Bablak et
al., 1995) supplemented with 30 mg L1 Hm and were placed
in the light. When plantlets had reached a size of 3 to 4 cm in height,
they were separated gently from any remaining necrotic callus and
removed to one-half strength MS0 to enhance root development. The
transformation frequency was expressed in terms of average number of
transgenic plants derived per gram of tissue. After rooting, plants
were transferred to soil as described previously (Bablak et al.,
1995).
Genomic Analysis of Transgenic B. distachyon
Lines
Total genomic DNA was isolated from leaves using a modified
cetyl-trimethyl-ammonium bromide protocol (Murray and Thompson, 1980)
and was quantified after RNase treatment. Plants were screened using
PCR amplification of the introduced hgh gene. PCR
primers (5'-CCTGAACTCACCGCGAC-3' and 3'-GCTCATCGAGA-GCCTGC-5') were
used to amplify a 516-bp fragment encoding the hgh gene,
which was analyzed by electrophoresis in 0.8% (w/v) agarose/ethidium
bromide gels. For Southern analysis, BamHI-digested
genomic DNA (10 µg lane1) was separated on an agarose
gel, blotted onto a membrane, and probed with a radioactive probe
following a standard protocol (Sambrook et al., 1989). The radioactive
probe was prepared by the random primer method (Feinberg and Volgstein,
1983), and consisted of a 1.07-kb BamHI fragment
containing the coding sequence of the hgh gene.
Challenge with Fungal Pathogens
All fungal infections were performed on batches of 24 B. distachyon plants with each challenge
repeated at least three times on seedlings aged from 3 to 4 weeks
post-germination. Diseased cereal plants with confirmed infections of
Blumeria graminis f. sp. avenae,
hordei, or triticae were used to infect
B. distachyon ecotypes by simply shaking
the condiophores on the recipient plants. Challenging with the rust
fungal pathogens Puccinia striformis f. sp.
hordei (strains BWR 80-1 and PB 60-7), f. sp.
triticae (strains WYR 95-6 and IPO 86053; yellow stripe
rust), and Puccinia recondita f. sp.
hordei (strains BBR 79-1 and PB60-2-2), f. sp. triticae (strains WYRP96-8 and WBRP90-25; brown leaf
rust) involved powder spraying a talc/urideospore suspension on to 3- to 4-week-old B. distachyon seedlings.
Plants were then bagged for 24 h in high humidity and were
incubated at 10°C, after which the bag was removed and the
temperature was increased to 24°C. Symptoms were first observed by 16 to 20 d following challenge. M.
grisea strain Guy-11 was cultured on Potato Dextrose
Agar (Sigma) and the spores were harvested into 0.2% (w/v) gelatin and
diluted to 105 spore mL1. The spore
suspension was sprayed onto B. distachyon
3- to 4-week-old seedlings to run off and the challenged material was
bagged for 24 h to maintain a high humidity. Symptoms were first
observed 3 to 4 d after spraying.
Received February 23, 2001; returned for revision May 3, 2001; accepted June 1, 2001.
Article, publication date, and citation information can be found at
www.plantphysiol.org/cgi/doi/10.1104/pp.010196.
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ABSTRACT
INTRODUCTION