Skip to main content
PLOS ONE logoLink to PLOS ONE
. 2018 Apr 18;13(4):e0195034. doi: 10.1371/journal.pone.0195034

Chloroplast variation is incongruent with classification of the Australian bloodwood eucalypts (genus Corymbia, family Myrtaceae)

Tanja M Schuster 1,2,*, Sabrina D Setaro 3, Josquin F G Tibbits 4, Erin L Batty 1, Rachael M Fowler 1, Todd G B McLay 1, Stephen Wilcox 5, Peter K Ades 6, Michael J Bayly 1
Editor: Tzen-Yuh Chiang7
PMCID: PMC5905893  PMID: 29668710

Abstract

Previous molecular phylogenetic analyses have resolved the Australian bloodwood eucalypt genus Corymbia (~100 species) as either monophyletic or paraphyletic with respect to Angophora (9–10 species). Here we assess relationships of Corymbia and Angophora using a large dataset of chloroplast DNA sequences (121,016 base pairs; from 90 accessions representing 55 Corymbia and 8 Angophora species, plus 33 accessions of related genera), skimmed from high throughput sequencing of genomic DNA, and compare results with new analyses of nuclear ITS sequences (119 accessions) from previous studies. Maximum likelihood and maximum parsimony analyses of cpDNA resolve well supported trees with most nodes having >95% bootstrap support. These trees strongly reject monophyly of Corymbia, its two subgenera (Corymbia and Blakella), most taxonomic sections (Abbreviatae, Maculatae, Naviculares, Septentrionales), and several species. ITS trees weakly indicate paraphyly of Corymbia (bootstrap support <50% for maximum likelihood, and 71% for parsimony), but are highly incongruent with the cpDNA analyses, in that they support monophyly of both subgenera and some taxonomic sections of Corymbia. The striking incongruence between cpDNA trees and both morphological taxonomy and ITS trees is attributed largely to chloroplast introgression between taxa, because of geographic sharing of chloroplast clades across taxonomic groups. Such introgression has been widely inferred in studies of the related genus Eucalyptus. This is the first report of its likely prevalence in Corymbia and Angophora, but this is consistent with previous morphological inferences of hybridisation between species. Our findings (based on continent-wide sampling) highlight a need for more focussed studies to assess the extent of hybridisation and introgression in the evolutionary history of these genera, and that critical testing of the classification of Corymbia and Angophora requires additional sequence data from nuclear genomes.

Introduction

The bloodwood eucalypts are sclerophyllous trees (c. 100 species) [1], currently classified in the genus Corymbia K.D.Hill & L.A.S.Johnson, which was taxonomically segregated from the genus Eucalyptus L'Her. in 1995 [2]. Bloodwoods include several morphologically distinct groups that have been formally or informally classified at a range of taxonomic levels (e.g. [2,3,4,5]), and are here identified (following Parra-Osorio et al. [6]) as the red bloodwoods (subg. Corymbia), yellow bloodwoods (subg. Blakella sect. Naviculares), ghost gums or paper-fruited bloodwoods (subg. Blakella sect. Abbreviatae), spotted gums (subg. Blakella sect. Maculatae), and cadaghi (monotypic subg. Blakella sect. Torellianae). These groups occur primarily in northern or eastern Australia (Fig 1), where they are well-represented in monsoonal, tropical savannahs, and there are two small groups of red bloodwoods restricted to the south-west and south-east of Australia (sections Calophyllae and Corymbia, respectively) in areas with Mediterranean, temperate climates. Bloodwoods are dominant trees in many of the areas in which they occur (Fig 2) and are thus ecologically important [7]; they also have a history of traditional and modern uses, and some species are widely grown for timber, for pulp, or as ornamental trees [7,8,9]. Traditional uses include kino (hardened sap), which is blood-red and confers the groups’ common name, utilised for art and medicinal purposes [10,11,12], and C. citriodora yields essential oils used as insect repellent and that have antimicrobial and antifungal properties [13,14,15]. Corymbia is part of the "eucalypt group" [16] (tribe Eucalypteae) [17] that also includes the sclerophyll genera Eucalyptus (>665 species) [1] and Angophora (9–10 species) [1,18], and the rainforest genera Arillastrum (1 species) [19], Stockwellia (1 species) [20], Allosyncarpia (1 species) [21], and Eucalyptopsis (2 species) [22].

Fig 1. Distribution of infrageneric groups in Corymbia (adapted from [2] and following the classification of [6]).

Fig 1

Colour coding of groups matches that used in other figures, i.e., taxonomic sections of Corymbia sensu Parra-Osorio et al. [6].

Fig 2. Photographs of Corymbia and Angophora.

Fig 2

(A) Woodland dominated by Corymbia cliftoniana (a red bloodwood, sect. Septentrionales), near Victoria River, Northern Territory; (B) woodland dominated by Corymbia grandifolia (a ghost gum, sect. Abbreviatae), near Daly Waters, Northern Territory; (C) partially opened flower bud of Corymbia ficifolia (sect. Calophyllae), showing operculate perianth (O) separating from hypanthium; (D) open flower of Angophora floribunda showing perianth composed of five, free sepals (S) and five, free petals (P).

The taxonomic splitting of Corymbia from Eucalyptus was contentious (e.g. [4,23]), with the key motivation for the separation of Corymbia being that the bloodwoods, on the basis of both morphological analyses [2,24] and early molecular analyses [25], were more closely related to Angophora than to Eucalyptus. That relationship has been unequivocally supported by all subsequent molecular phylogenetic analyses of the group (e.g. [6,26,27,28,29,30,31]), and is supported by some morphological characters, including patterns of leaf venation, features of trichomes, and the presence of oil ducts in the pith of branches [2,24,32]. There are, nonetheless, clear differences in some macro-morphological features between the two groups that have led to the longstanding treatment of Angophora as a separate genus from the bloodwoods (whether placed in Eucalyptus or treated as Corymbia) by almost all authors (e.g., [5,8,9,18,33,34,35]) since Angophora was first described in 1797 [36]. The most notable differences between the groups are in the flowers, which in Angophora have free sepals and petals, in contrast to the calyptrate/operculate perianth of Corymbia (Fig 2). Despite such morphological differences, molecular phylogenetic analyses have presented conflicting signals regarding monophyly of Corymbia [37], with some resolving the genus as monophyletic (e.g. [6,27,38,39]), while others resolve it as paraphyletic, with Angophora nested within it [28,29,30,31,40].

Most phylogenetic analyses assessing the relationships of bloodwoods to other eucalypts have employed few DNA markers generated by conventional Sanger sequencing methods (e.g. [6,26,27,28,29,30,31]). The use of High-Throughput Sequencing (HTS) methods, which can generate larger volumes of sequence data, are only just beginning to be used in eucalypt studies (e.g. [41]). Partly as a result of the small size of most molecular datasets, some key relationships have typically been poorly supported, including that of the bloodwoods to Angophora. For example, Maximum Parsimony (MP) bootstrap support values indicating paraphyly of Corymbia have generally been in the range of 51–93% for clades showing Angophora nested in Corymbia [28,30,40], and those for a monophyletic Corymbia have ranged from 78–100% [6,27,38,39]. An exception is a recent study that used analyses of whole chloroplast (cp) genomes [41], which showed strong support for Corymbia as paraphyletic with respect to Angophora (parsimony bootstrap support and Bayesian posterior probability both 100%), with subg. Blakella being more closely related to Angophora than to subg. Corymbia. However, that study, despite using a large amount of sequence data, included only one sample each of the red bloodwoods, yellow bloodwoods, ghost gums and spotted gums, and it was unclear whether the result was an artefact of sparse taxon sampling.

In this study, we assess relationships of bloodwood eucalypts, including those among species, series, sections and subgenera of Corymbia, and those of Corymbia to Angophora. We expand on the sampling of Bayly et al. [41] to include the largest sample of species of Angophora and Corymbia in any molecular study using HTS data to date (Table 1). We specifically address questions relating to the evolutionary history of this large and ecologically and economically important group and test the current taxonomic classification, especially at the ranks of genus and subgenus. We use both chloroplast genome derived sequences and combine sequences of nuclear ribosomal internal transcribed spacer (ITS) regions from previous studies for separate phylogenetic analyses using Maximum Likelihood (ML) and MP methods, to provide assessment of phylogenetic signal from both nuclear and chloroplast markers. Specifically these methods are used to test the hypotheses that 1) Corymbia is monophyletic and 2) the currently recognised subgenera [6] are monophyletic.

Table 1. Details of accessions used in this study.

Genus and species Subgenus Section/series Collector number, herbarium voucher location Provenance/reference GenBank accession
Outgroups
Allosyncarpia ternata S.T.Blake Spokevicius A. s.n., MELU 108348 QLD, Sankowsky Arboretum, Tolga [41] NC_022413.1
Stockwellia quadrifida D.J.Carr, S.G.M.Carr & B.Hyland Spokevicius A. s.n., MELU 108349 QLD, Sankowsky Arboretum, Tolga [41] NC_022414.1
Angophora
A. bakeri E.C.Hall TMS14–27, MEL NSW, Windsor KY246359
A. costata (Gaertn.) Britten Ades P. s.n., MELU 108350 VIC, UoM, Creswick [41] NC_022412.1
A. costata subsp. costata DN2073, AD 163314 NSW, Glenbrook KY246360
A. costata subsp. euryphylla L.A.S.Johnson ex G.J.Leach DN2082 i, AD 163326 NSW, Broken Back Range KY246361
A. costata subsp. euryphylla L.A.S.Johnson ex G.J.Leach TMS14–29, MEL NSW, Yengo National Park KY246362
A. floribunda (Sm.) Sweet Spokevicius A. s.n., MELU 108351 VIC, UoM, Creswick [41] NC_022411.1
A. floribunda MJB2471, MELU 114352 VIC, Mallacoota KY246363
A. floribunda TMS14–33, MEL NSW, Ulan KY246364
A. hispida (Sm.) Blaxell KLW11152, NSW NSW, Royal National Park KY246365
A. inopina K.D.Hill DN6258, AD NSW, Wyee KY246366
A. leiocarpa (L.A.S.Johnson ex G.J.Leach) K.R.Thiele & Ladiges DN2103, AD 163292 QLD, Karara KY246367
A. melanoxylon R.T.Baker CAPO–R173–P1, MELU 107825 QLD, St George KY246368
A. melanoxylon DN2552, AD 163739 QLD, St George KY246369
A. subvelutina F.Muell. TMS14–28, MEL NSW, Windsor KY246370
A. subvelutina DN3204, AD, NSW NSW, Mulgoa KY246371
Corymbia
C. abergiana (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Abergianae CAPO23–891966, MELU 107776 NSW, Mount Annan BG, cultivated KY246372
C. aparrerinja K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Grandifoliae MJB2485, MELU 114286 NT, 108.4 km N of Alice Springs on Stuart Highway KY246373
C. aparrerinja Blakella Abbreviatae/ Grandifoliae MJB2494, MELU 114292 NT, 33 km N of Devils Marbles, Stuart Highway KY246374
C. arafurica K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Papuanae MJB2553, MELU 114349 NT, 32.2 km E Humpty Doo, Arnhem Highway KY246375
C. arafurica Blakella Abbreviatae/ Papuanae MJB2555, MELU 114351 NT, 5.8 km E Bark Hut roadhouse, Arnhem Highway KY246376
C. arnhemensis (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Arenariae MJB2534, MELU 114330 NT, Nitmiluk National Park KY246377
C. arnhemensis Corymbia Septentrionales/ Arenariae MJB2537, MELU 114333 NT, Nitmiluk National Park KY246378
C. aspera (F.Muell.) K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/Asperae MJB2501, MELU 114300 NT, Stuart Highway, turnoff to Helen Springs KY246379
C. aspera Blakella Abbreviatae/Asperae MJB2503, MELU 114302 NT, 16.7 km N Renner Springs, Stuart Highway KY246380
C. aureola (Brooker & A.R.Bean) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN2542, AD 163675 QLD, Cherwell Range KY246381
C. bella K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Papuanae DN4204, AD 164468 NT, Bulman KY246382
C. bella Blakella Abbreviatae/ Papuanae MJB2545, MELU 114341 NT, 10 km N Hayes Creek, Dorat Road KY246383
C. bella Blakella Abbreviatae/ Papuanae MJB2548, MELU 114344 NT, 25.6 km N Adelaide River, Stuart Highway KY246384
C. bleeseri (Blakely) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Collinae MJB2518, MELU 114315 NT, 54 km N Mataranka, Stuart Highway KY246385
C. bloxsomei (Maiden) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN687, AD 162445 QLD, Barakula State Forest KY246386
C. brachycarpa (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Rhodopes CAPO8–891880, MELU 107775 NSW, Mount Annan BG, cultivated KY246387
C. bunites (Brooker & A.R.Bean) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN711, AD 162630 QLD, Blackdown Tableland KY246388
C. calophylla (Lindl.) K.D.Hill & L.A.S.Johnson Corymbia Calophyllae DN1160, AD 99625330 WA, Cockleshell Gully KY246389
C. calophylla Corymbia Calophyllae KLW11208, NSW 972973 WA, 18.6 km NE of Jurien on road to Brand Highway KY246390
C. calophylla Corymbia Calophyllae DN3421, PERTH 5788722 WA, Brookton KY246391
C. chippendalei (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae NG6497, MEL 2390093 WA, Katjarra KY246393
C. citriodora (Hook.) K.D.Hill & L.A.S.Johnson Blakella Maculatae DN702, AD 162591 QLD, Springsure KY246394
C. citriodora Blakella Maculatae DN1246 ii, AD 99624278 NSW, Drake KY246442
C. clarksoniana (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Polycarpae CAPO1A–904971, MELU 107760 NSW, Mount Annan BG, cultivated KY246395
C. collina (W.Fitzg.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Collinae Ladiges P. s.n. MELU WA, Kimberly region KY246396
C. deserticola (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson subsp. deserticola Corymbia Septentrionales/ Ferrugineae DN542, PERTH 5665884 WA, Weelarrana, Kumarina Roadhouse KY246397
C. dichromophloia (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae MJB2500A, MELU 114298 NT, 28 km N Three Ways, Stuart Highway KY246398
C. dichromophloia Corymbia Septentrionales/Dichromophloiae DN4192 iii, AD 164321 NT, Barkly Tableland KY246392
C. dichromophloia Corymbia Septentrionales/ Dichromophloiae DN1928 iv, PERTH 5218063 WA, Gibb River Road KY246434
C. dunlopiana K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Ferrugineae MJB2533, MELU 114329 NT, 14.1. km E Katherine, Katherine Gorge Road KY246399
C. ellipsoidea (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae DN5112, AD QLD, Mount Garnet KY246400
C. eremaea subsp. oligocarpa (Blakely & Jacobs) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae DN1208, AD 99625502 NT, Mount Gillen KY246401
C. eximia (Schauer) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN632, AD 162956 NSW, Hawksbury River scarp near Wisemans Ferry KY246402
C. eximia Blakella Naviculares MJB2237, MELU 108352 VIC, PFP Arboretum [41] NC_022409.1
C. ferriticola (Brooker & Edgecombe) K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/Asperae DN2752, AD 163641 WA, Meekatharra KY246403
C. ferruginea (Schauer) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Ferrugineae MJB2505, MELU 114304 NT, 70.5 km N Renner Springs, Stuart Highway KY246404
C. ferruginea Corymbia Septentrionales/ Ferrugineae MJB2508, MELU 114307 NT, 12.9 km N Dunmarra, Stuart Highway KY246405
C. ficifolia (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Calophyllae KLW11249, NSW 973354 WA, Walpole, Nornalup National Park KY246406
C. flavescens K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Grandifoliae MJB2498, MELU 114296 NT, 18 km N Three Ways, Stuart Highway KY246407
C. foelscheana (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae MJB2540, MELU 114336 NT, Nitmiluk National Park, track to Edith Falls KY246408
C. grandifolia (R.Br. ex Benth.) K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Grandifoliae MJB2511, MELU 114310 NT, 4.6 km E Daly Waters, Carpentaria Highway KY246409
C. grandifolia Blakella Abbreviatae/ Grandifoliae MJB2517, MELU 114314 NT, 7.1 km S of turnoff to Forrest Hill Station KY246410
C. gummifera (Gaertn.) K.D.Hill & L.A.S.Johnson Corymbia Corymbia DN1228, AD 99624288 NSW, Ku-Ring-Gai Chase KY246411
C. gummifera Corymbia Corymbia MJB2472, MELU 114353 VIC, Mallacoota KY246412
C. gummifera Corymbia Corymbia MJB2232, MELU 108355 VIC, PFP Arboretum [41] NC_022407.1
C. haematoxylon (Maiden) K.D.Hill & L.A.S.Johnson Corymbia Calophyllae KLW11229, NSW 973332 WA, Dardanup Conservation Park KY246413
C. hamersleyana (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae DN1190, AD 99625487 WA, Mount Nameless KY246414
C. hamersleyana Corymbia Septentrionales/Dichromophloiae CAPO10–832169 v, MELU NSW, Mount Annan BG, cultivated KY246435
C. henryi (S.T.Blake) K.D.Hill & L.A.S.Johnson Blakella Maculatae DN1259, AD 99624267 QLD, Helidon Hills KY246415
C. henryi Blakella Maculatae DN2092, AD 163302 NSW, Coast Range KY246416
C. intermedia (R.T.Baker) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Intermediae DN708, AD 162627 QLD, Blackdown Tableland KY246417
C. intermedia Corymbia Septentrionales/ Intermediae GB330, MELU NSW, Nambucca Heads, Black Rock KY246418
C. jacobsiana (Blakely) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales MJB2543B, MELU 114339 NT, Mesa, N side Stuart Highway KY246419
C. leichhardtii (F.M.Bailey) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN1277, AD 99624246 QLD, Springsure KY246420
C. lenziana (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae DN5733, AD 241349 WA, Kennedy Range KY246421
C. ligans K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Polycarpae DN2527, AD 163755 QLD, Greenvale KY246422
C. maculata (Hook.) K.D.Hill & L.A.S.Johnson Blakella Maculatae DN1752, AD 99623282 NSW, Narooma KY246423
C. maculata Blakella Maculatae Spokevicius A. s.n., MELU 108353 VIC, UoM, Creswick [41] NC_022408.1
C. opaca (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/Dichromophloiae NG6494, MEL 2390090 WA, Katjarra KY246424
C. pachycarpa K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Ferrugineae DN1939, PERTH 5218012 WA, Billiluna KY246425
C. peltata (Benth.) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN2505, AD 163709 QLD, Newcastle Range KY246426
C. petalophylla (Brooker & A.R.Bean) K.D.Hill & L.A.S.Johnson Blakella Naviculares DN1262, AD 99624268 QLD, Eidsvold KY246427
C. plena K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Polycarpae DN2535, AD 163670 QLD, Torrens Creek KY246428
C. polysciada (F.Muell.) K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Polysciadae MJB2544, MELU 114340 NT, 10 km N Hayes Creek, Dorat Road KY246429
C. polysciada Blakella Abbreviatae/ Polysciadae MJB2554, MELU 114350 NT, 300 m E Bark Hut roadhouse, Arnhem Highway KY246430
C. ptychocarpa (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Ptychocarpae MJB2546A, MELU 114342 NT, Robin Falls, SW Adelaide River KY246431
C. ptychocarpa Corymbia Septentrionales/ Ptychocarpae MJB2551, MELU 114347 NT, Litchfield National Park KY246432
C. rhodops (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Rhodopes DN1306, AD 99624219 QLD, Herberton KY246433
C. serendipita (Brooker & Kleinig) Bean Corymbia Septentrionales/ Arenariae DN2502, AD 163706 QLD, Newcastle Range KY246436
C. tessellaris (F.Muell.) K.D.Hill & L.A.S.Johnson Blakella Abbreviatae/ Tessellares MJB2226, MELU 108354 VIC, PFP Arboretum [41] NC_022410.1
C. torelliana (F.Muell.) K.D.Hill & L.A.S.Johnson Blakella Torellianae TMS14–40, MEL NSW, Gwydir Highway, Nancy Coulton Lookout, cultivated KY246437
C. trachyphloia (F.Muell.) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales DN684 vi, AD 163256 QLD, Tara KY246438
C. trachyphloia Corymbia Septentrionales DN714, AD 162803 QLD, Goodwood KY246439
C. trachyphloia Corymbia Septentrionales DN5128, AD QLD, Blencoe Falls KY246440
C. umbonata (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson Corymbia Septentrionales/ Dichromophloiae MJB2513, MELU 114312 NT, 74 km N Daly Waters, Stuart Highway KY246441
Eucalyptus
E. aromaphloia L.D.Pryor & J.H.Willis Symphyomyrtus Maidenaria/Acaciiformes Ades P. s.n., MELU 108368 VIC, UoM, Creswick [41] NC_022396.1
E. baxteri (Benth.) Maiden & Blakely ex J.M.Black Eucalyptus Capillulus MJB2223, MELU 108360 VIC, PFP Arboretum [41] NC_022382.1
E. camaldulensis Dehnh. Symphyomyrtus Exsertaria/Rostratae Tibbits J. s.n., MELU 108435 VIC, La Trobe University campus, Bundoora [41] NC_022398.1
E. cladocalyx F.Muell. Symphyomyrtus Sejunctae Ades P. s.n., MELU 108383 VIC, UoM, Parkville [41] NC_022394.1
E. cloeziana F.Muell. Idiogenes - MJB2230, MELU 108357 VIC, PFP Arboretum [41] NC_022388.1
E. curtisii Blakely & C.T.White Acerosae - Spokevicius A. s.n., MELU 108358 VIC, PFP Arboretum [41] NC_022391.1
E. deglupta Blume Minutifructus Equatoria Udovicic F. s.n., MELU 108436 VIC, RBGV, Melbourne [41] NC_022399.1
E. delegatensis R.T.Baker Eucalyptus Cineraceae MJB2134, MELU 108361 VIC, Mt Macedon [41] NC_022380.1
E. diversicolor F.Muell. Symphyomyrtus Inclusae Spokevicius A. s.n., MELU 108373 VIC, PFP Arboretum [41] NC_022402.1
E. diversifolia Bonpl. Eucalyptus Longistylus MJB2229, MELU 108362 VIC, PFP Arboretum [41] NC_022383.1
E. elata Dehnh. Eucalyptus Aromatica Ades P. s.n., MELU 108363 VIC, UoM, Creswick [41] NC_022385.1
E. erythrocorys F.Muell. Eudesmia Limbatae MJB2234, MELU 108356 VIC, PFP Arboretum [41] NC_022406.1
E. globulus Labill. Symphyomyrtus Maidenaria/Globulares Anon. s.n., HO 528199 TAS [42] NC_008115.1
E. grandis W.Hill Symphyomyrtus Latoangulatae/Transversae - Brazil, Federal University of Viçosa [43] NC_014570.1
E. guilfoylei Maiden Cruciformes - Spokevicius A. s.n., MELU 108359 VIC, PFP Arboretum [41] NC_022405.1
E. marginata D.Don ex Sm. Eucalyptus Longistylus Spokevicius A. s.n., MELU 108369 VIC, PFP Arboretum [41] NC_022390.1
E. melliodora A.Cunn. ex Schauer Symphyomyrtus Adnataria/Melliodorae Spokevicius A. s.n., MELU 108380 VIC, UoM, Creswick [41] NC_022392.1
E. microcorys F.Muell. Alveolata - Spokevicius A. s.n., MELU 108375 VIC, UoM, Creswick [41] NC_022404.1
E. nitens (H.Deane & Maiden) Maiden Symphyomyrtus Maidenaria/Globulares Spokevicius A. s.n., MELU 108378 VIC, UoM, Creswick [41] NC_022395.1
E. obliqua L’Hér. Eucalyptus Eucalyptus/Eucalyptus Spokevicius A. s.n., MELU 108364 VIC, UoM, Creswick [41] NC_022378.1
E. patens Benth. Eucalyptus Longistylus/Patentes MJB2227, MELU 108370 VIC, PFP Arboretum [41] NC_022389.1
E. polybractea R.T.Baker Symphyomyrtus Adnataria/Buxeales Spokevicius A. s.n., MELU 108384 VIC, UoM, Parkville [41] NC_022393.1
E. radiata Sieber ex DC. Eucalyptus Aromatica/Radiatae Ades P. s.n., MELU 108365 VIC, UoM, Creswick [41] NC_022379.1
E. regnans F.Muell. Eucalyptus Eucalyptus/Regnantes MJB2224, MELU 108371 VIC, PFP Arboretum [41] NC_022386.1
E. saligna Sm. Symphyomyrtus Latoangulatae/Transversae Spokevicius A. s.n., MELU 108376 VIC, UoM, Creswick [41] NC_022397.1
E. salmonophloia F.Muell. Symphyomyrtus Bisectae/Salmonophloiae MJB2236, MELU 108374 VIC, PFP Arboretum [41] NC_022403.1
E. sieberi L.A.S.Johnson Eucalyptus Cineraceae/Psathyroxylon Ades P. s.n., MELU 108366 VIC, UoM, Creswick [41] NC_022384.1
E. spathulata Hook. Symphyomyrtus Bisectae/Erectae Ades P. s.n., MELU 108381 VIC, UoM, Creswick [41] NC_022400.1
E. torquata Luehm. Symphyomyrtus Dumaria/Torquatae Tibbits J. s.n., MELU 108382 VIC, UoM, Creswick [41] NC_022401.1
E. umbra R.T.Baker Eucalyptus Amentum MJB2225, MELU 108372 VIC, PFP Arboretum [41] NC_022387.1
E. verrucata Ladiges & Whiffin Eucalyptus Capillulus/Pachyphloius Tibbits J. s.n., MELU 108367 VIC, UoM, Creswick [41] NC_022381.1

Classification of subgenera and sections follows [6]; classification of series follows the informal classification of [2], where consistent with the higher-level groupings. CAPO = Carlos A. Parra-Osorio, DN = Dean Nicolle, GB = Gillian Brown, KLW = Karen L. Wilson, MJB = Michael J. Bayly, NG = Neil Gibson, TMS = Tanja M. Schuster. Herbarium codes follow Index Herbariorum: AD = State Herbarium of South Australia, HO = Tasmanian Herbarium, MEL = National Herbarium of Victoria, MELU = University of Melbourne Herbarium, NSW = National Herbarium of New South Wales, PERTH = Western Australian Herbarium. Provenance data: BG = botanic garden, NSW = New South Wales (Australia), NT = Northern Territory (Australia), QLD = Queensland (Australia), TAS = Tasmania (Australia), VIC = Victoria (Australia), WA = Western Australia (Australia). Further abbreviations are PFP = Peter Francis Points Arboretum, Coleraine, Victoria; RBGV = Royal Botanic Garden Victoria, and UoM = The University of Melbourne (, followed by the respective campus).

i Collected as A. euryphylla (G.J.Leach) L.A.S.Johnson & K.D.Hill, a name that is synonymised with A. costata subsp. euryphylla in the current Australian Plant Census (APC) [1].

ii Collected as Corymbia variegata (F.Muell.) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. citriodora in the current APC.

iii Collected as Corymbia capricornia (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. dichromophloia in the current APC.

iv Collected as Corymbia rubens K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. dichromophloia in the current APC.

v Collected as Corymbia semiclara K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. hamersleyana in the current APC.

vi Collected as Corymbia trachyphloia subsp. amphistomatica K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. trachyphloia in the current APC.

Materials and methods

Taxon sampling for chloroplast DNA study

Samples and sequences of chloroplast DNA used in this study are listed in Table 1. Names of species and infraspecific taxa generally follow the Australian Plant Census [1], and authorities are only given in the text for species names not listed in Table 1. Taxonomic works used to identify samples were [2,8,18]. For Corymbia, our sampling included 55 of the 97 species accepted by the Council of Heads of Australasian Herbaria (CHAH) [1], including all of the subgenera and sections recognised in the classification of [6], and with 19 species represented by at least two accessions. Sampling for Angophora included eight of the ten species recognised by CHAH [1], four of which were represented by at least two accessions. We also included sequences for 31 species of Eucalyptus and outgroups Allosyncarpia and Stockwellia from [41]. In total, the analysis included 123 accessions, of which 84 were newly sequenced for this study.

DNA isolation from silica dried leaves

For the cpDNA study, total genomic DNA (gDNA) was extracted from ca. 80 mg of recently collected leaf tissue (no older than one year) using a modified CTAB DNA extraction protocol [44,45]. Older silica-dried collections were difficult to extract suitable DNA from, probably due to chemical DNA degradation in this plant group rich in secondary metabolites. The CTAB lysing buffer (2% w/v cetyltrimethylammonium bromide (CTAB), 2% w/v polyvinylpyrrolidone 40,000 (PVP–40), 1.4 M NaCl, 20 mM EDTA, 100 mM Tris–HCl pH 8.0) was modified by addition of 0.6% v/v each of 2–mercaptoethanol, RNase A, and proteinase K per sample. Further modifications to the CTAB extraction protocol included a sucrose/Tris/EDTA (STE) wash (8% w/v sucrose, 1 M Tris–HCl pH 7.0, 0.5 M EDTA) before lysis using 1 mL of STE per 80 mg of ground plant tissue [46]. The STE solution was discarded after centrifugation at 5,000 rpm for 10 min, and the pellet suspended in 700 μL of preheated (65°C) CTAB lysate buffer. After adding 110 μL bovine serum albumin (BSA)/NaCl (1:10, 4% BSA:5 M NaCl) to each sample, they were left to incubate for ca. 16 hrs at 60°C. Two 2/3 volume chloroform extractions were done, centrifuging for 10 min at 14,800 rpm for the first and then 8 min at the same speed for the second. DNA was precipitated with 2/3 volume of 100% isopropanol (room temperature). After 30–60 min incubation at room temperature, the DNA was centrifuged into a pellet at 14,800 rpm for 15 min and washed twice with 70% ethanol after discarding the isopropanol. DNA was resuspended in 100 μL TE pH 8.0 (10 mM Tris–HCl:1 mM EDTA pH 8.0) after leaving the pellet to dry overnight to allow all of the ethanol to evaporate. DNA quantity and quality were checked with Nanodrop 2000 (NanoDrop Products) and Qubit 2.0 fluorometer (Invitrogen) instruments and visualised by electrophoresis (1.5% agarose gel) with ethidium bromide.

DNA library construction and sequencing

This section details a relatively cost-effective library preparation protocol at ca. AUD 35 per sample using no proprietary kits. All reagents are from New England BioLabs (NEB) if not stated otherwise. Immediately before sonication, a DNA aliquot was washed with ethanol/sodium acetate (5.5:1, 100% ethanol:2.4M NaAc) at a 1:4.7 DNA:wash solution volume, and then centrifuged at 14,800 rpm for 10 min. After discarding the wash solution, the resulting pellet was washed with 70% ethanol and resuspended in 100 μL 1 M Tris–HCl pH 8.0. DNA was quantified with a Qubit 2.0 (Invitrogen), and an aliquot of 3 μg of gDNA per sample was brought to 115 μL with ultrapure H2O. The DNA was sonicated for 50 sec with a S220 Focused-ultrasonicator (Covaris) set to 6–8°C, 120W peak incident power, 200 cycles per burst, and on duty cycle 5%, aiming for 800 bp mean fragment size.

The sonicated samples (100 μL each) were cleaned using Serapure SPRI beads [47] at a 0.6:1.0 beads:sample ratio to remove short fragments (<300 bp) by incubating this mixture for 20 min at room temperature, immobilising beads on a 96S super magnet plate (Alpaqua) for 15 min, discarding the supernatant and washing with 170 μL 80% ethanol, and then leaving the magnet-trapped beads to air dry for 2 min.

NEBNext End Repair Module produced blunt ends on the fragmented DNA by eluting the DNA from the magnet-trapped beads and incubating with 2.0 μL 10 × reaction buffer, 0.4 μL enzyme mix, and 17.6 μL ultrapure H2O per sample at 20°C for 60 min. Samples were again purified using the Serapure SPRI beads by adding 50 μL PEG:NaCl (20% PEG w/v:5 M NaCl) and 50 μL 100% isopropanol to each sample, incubating this for 15 min at room temperature, and washed using 80% ethanol as in the above steps. Then dA tails were attached to the fragments using 0.5 μL 10 mM deoxyadenosine 5'-triphosphate, 0.4 μL Klenow Fragment, 2.0 μL NEB 10 × Buffer 2, and 17.1 μL ultrapure H2O per sample to elute the DNA and incubated at 37°C for 60 min followed by 65°C for 20 min. Per sample, 2 μL of 25 μM multiplex hairpin adaptors (top plus bottom strands) in 10 mM Tris–HCl pH 8.0 [47] were ligated to the DNA fragments with 0.25 μL10 mM ATP, 0.4 μL T4 DNA ligase, 0.8 μL T4 DNA ligase buffer, and 6.55 μL ultrapure H2O at 12°C overnight and then 10 min of 65°C to stop the reaction. Exonuclease digestion degraded all non-competent molecules with 0.5 μL 10 × NEB Buffer I, 0.25 μL Lambda Exonuclease, 0.25 μL Exonuclease I, and 4.0 μL ultrapure H2O per sample at 37°C for 2 hrs, and 80°C for 20 min. After the digestion, samples were cleaned on the magnetic plate as before, but using 80 μL 20% PEG:5M NaCl and 80 μL 100% isoproplanol per sample. Samples were eluted with 60 μL 10 mM Tris–HCl pH 8.0 and stored at 4°C until q-PCR titration, after which the libraries were kept at -20°C for long term storage.

For titration, a 20 μL q-PCR reaction, using 5 μL of each 800 bp library as template, 0.5 μL 10× SYBR Green (Thermo Fisher Scientific), 10.0 μL Kapa HiFi HotStart ReadyMix (KAPA Biosystems), 2.5 μL ultrapure H2O, and 1.0 μL each of 5 μM TRUESEQ (Illumina) compatible PE primers [47] was run to 20 cycles on a BioRad CFX q-PCR machine. Settings for the q-PCR were 30 sec of 98°C for denaturation and 20 cycles of 98°C for 10 sec, 67°C for 30 sec, and 72°C for 30 sec. Once the sample appropriate cycle number was determined from this q-PCR, a 40 μL reaction and including sample-specific PE primers including indexing barcodes to allow pooling of multiple samples per sequencing was run using the same settings as before.

Samples were pooled and quality checked either with an Agilent Bioanalyser DNA1000 chip system (Agilent) for HiSeq 1500 (Illumina) sequencing or a 2200 Tape Station using the D1000 kit (Agilent) and Qubit 3.0 (Invitrogen) for sequencing on a NextSeq 500 machine (Illumina). A 250 cycle (2 × 125 paired end reads) kit (Illumina) was used for the former or a 300 cycle (2 × 150 paired end reads) kit (Illumina) for the latter sequencer.

Sequence trimming, quality control, read mapping and chloroplast sequence assembly

Base calling and quality filtering was done with Illumina pipeline software (v.1.7 or later) and samples were pre-processed with custom scripts at the Walter and Eliza Hall Institute of Medical Research (WEHI) sequencing facility.

The new sequences were assessed, trimmed and assembled with CLC Genomics Workbench v. 9.5.1 and 9.5.2 (Qiagen) and the CLC Workflow is available as supplementary material (S1 File). Paired-end reads were paired and reads shorter than 15 or longer than 1000 bp were discarded. Reads below PHRED score 20 were also discarded. The fraction of low quality bases that were allowed in a read was 5%.

The quality-filtered and paired reads were mapped against a reference chloroplast genome (Eucalyptus globulus, GenBank accession: NC_008115.1). Sequence coverage was generally sufficient to unambiguously assemble most of the chloroplast genome for each sample, but all genomes included some regions with low coverage of mapped reads. A consensus sequence of the mapped assembly was created by removing regions with low coverage and inserting ambiguity codes for bases with more than one possible nucleotide using a threshold of 50% and ‘maximum number of ambiguous nucleotides allowed after trimming = 2’.

Sequence alignment and phylogenetic analyses of chloroplast DNA

All newly generated chloroplast sequences included in the study were aligned with MAFFT v.7.299b [48] and the fast and progressive method FFT-NS-2, suitable for large alignments. One inverted repeat region (IRa) was excluded from the alignment. The alignment was viewed with SeaView v.4.6 [49] or Mesquite v.3.10 [50] and subsequently processed with GBLOCKS v.0.91b [51] using default parameters, which stringently trims alignments allowing no gaps. Hence, the final dataset only included regions with sequence coverage for all samples, and all indels were removed.

We used jModelTest v.2.1.10 [52,53] and the AIC and BIC criteria, to estimate the model of nucleotide substitution that best fits the chloroplast data. The maximum likelihood analysis was done with Standard RAxML v.8.2.8 [54] with 1000 rapid bootstrap inferences and a thorough ML search under the GAMMA model of rate heterogeneity. The maximum parsimony analysis was done with PAUP* v.4.0a151 [55] with the following settings: all characters were treated as unordered and of equal weight. Heuristic searches employed tree-bisection-reconnection branch swapping and 1000 replicates of random stepwise additions. The number of bootstrap replicates was 1000 with one tree held at each step. Trees were viewed and exported for rendering in FigTree v.1.4.3 [56].

Analysis of nuclear ribosomal DNA

For comparison with the cpDNA phylogeny, we combined sequences of the ITS regions of nuclear ribosomal DNA (nrDNA) from previous studies [6,26,29,30,31,57,58] for phylogenetic analyses. Separate analyses of these nrDNA sequences have not been presented in previous studies, with most including only a small number of Corymbia samples or, in the case of the largest study to date [31], also combining a subset of these sequences with cpDNA markers in analyses of a concatenated dataset. Our dataset included 66 accessions of Corymbia (representing all taxonomic sections), 15 of Angophora (9 of 10 species), 31 of Eucalyptus (the same species as in the cpDNA dataset, representing major lineages), two of Stockwellia, one of Eucalyptopsis, three of Allosyncarpia, and one of Arillastrum (used as outgroup). Partial sequences, or those identified as spacers associated with pseudogenes using established criteria [59,60,61,62], were excluded from analyses. We used existing nrDNA sequences for analyses, rather than assembling novel sequences from our current genomic data for Corymbia, because of the presence of substantial within-genome variation in our samples (in line with previous reports [38,59,60]), and associated difficulties in separating and assembling sequences of the various paralogues/alleles, which is a challenging task worthy of separate investigation and discussion. The nrITS sequences from GenBank were aligned using Geneious v.9.1.7 [63]. Model testing, ML and MP analyses were conducted as outlined above with the addition that gaps present in the nrDNA alignment were treated as missing data in the MP analysis.

Results

Analysis of chloroplast DNA

GBLOCKS eliminated 37% of the MAFFT alignment, resulting in 121,016 characters and 10,847 distinct alignment patterns in the final alignment (see supplementary material S2 File). Both, AIC and BIC from jModelTest indicated the General Time Reversible model using gamma and invariant sites (GTR+I+G) as the best fit. Final ML Optimization Likelihood was -254343.104231. The maximum parsimony analysis had 3771 parsimony informative characters, 4116 variable but uninformative characters, and resulted in 12 trees with length = 10413, consistency index = 0.81, retention index = 0.96. Topologies of the ML and MP trees were similar (Fig 3), and most nodes had 85–100% bootstrap support (BS) for both ML and MP analyses, with the backbone, in particular, well supported.

Fig 3. Phylogeny resulting from cpDNA analyses.

Fig 3

Best-scoring maximum likelihood tree from a RAxML analysis (final ML optimization likelihood of -254343.104231) of a cpDNA dataset (121,016 base pairs, 10,847 distinct alignment patterns, 123 accessions) of eucalypts. Names of Corymbia species are colour-coded by taxonomic section as indicated. Labelling to the right of the tree indicates the outgroup (‘OG’), major groups of Eucalyptus, including subg. Eudesmia (‘Eudesmids’), the symphyomyrt clade (‘Symph’; including subgenera Alveolata, Cruciformes Minutifructus and Syphyomyrtus), and the monocalypt clade (‘Mono’; including subgenera Acerosae, Eucalyptus and Idiogenes), as well as subclades of Corymbia clustering by geographic proximity (A1–A3 and B1–B6) referred to in the text and Fig 4 (for clade A) and Fig 5 (for clade B). Species names of species represented by multiple accessions are followed by collection number for newly generated sequences or GenBank accession number (NC) for data generated for previous studies. Bootstrap support values are shown as percent maximum likelihood/maximum parsimony (MP mapped onto ML tree) with weighted edges indicating 100% support for both ML and MP. Support values <50% are omitted or dashed when the alternate analysis method had ≥50% support.

Rooting the trees with Allosyncarpia and Stockwellia recovered relationships of a monophyletic Eucalyptus as sister to Angophora + Corymbia. Eucalyptus is composed of three clades corresponding to ‘Eudesmids’ (subg. Eudesmia, represented by E. erythrocorys) subtending a well-supported clade of ‘Monocalypts’ sensu [41] (including representatives of subg. Acerosae [E. curtisii], subg. Idiogenes [E. cloeziana], and subg. Eucalyptus [remainder of that clade]), which were sister to a ‘Symphyomyrt’ clade (including members of subg. Alveolata [E. microcorys], subg. Cruciformes [E. guilfoylei], and subg. Minutifrucuts [E. deglupta] nested in subg. Symphyomyrtus [remainder of that clade]) that was moderately supported with BS ML/MP 76/75%.

Corymbia is paraphyletic because of the inclusion of Angophora in one Corymbia clade (clade A; Fig 3). Furthermore, subgenera Blakella and Corymbia, most non-monotypic sections (Abbreviatae, Maculatae, Naviculares, Septentrionales), and several species including more than one accession here are not monophyletic. In addition to Angophora, clade A includes a basal grade of a few species of red bloodwoods from southern Australia that do not group with all other red bloodwoods in clade B. The red bloodwoods in clade A include C. gummifera (monotypic sect. Corymbia) from south-eastern Australia and C. calophylla, C. ficifolia, and C. haematoxylon that correspond to sect. Calophyllae from south-western Western Australia (Fig 1). Clade A also includes the yellow bloodwoods (sect. Naviculares), spotted gums (sect. Maculatae), cadagi or C. torelliana (monotypic sect. Torellianae), and two ghost gums (sect. Abbreviatae). Although the latter all form a clade, spotted gum and yellow bloodwood species are interdigitated and taxonomic sections based on morphology do not form groups here. The ghost gums sensu Parra-Osorio et al. [6] are polyphyletic, because clade B also includes two separate clades of sect. Abbreviatae. In addition, clade B contains most of the red bloodwood species (sect. Septentrionales), in which the ghost gums are embedded.

Of 23 species of Angophora and Corymbia represented in the dataset by two or more samples, only four species (A. melanoxylon, C. eximia, C. grandifolia, and C. gummifera) are resolved as monophyletic, whereas most are indicated as paraphyletic or polyphyletic, and two species (C. trachyphloia and C. aparrerinja) have accessions split between the two major ingroup clades (clades A and B). This widespread incongruence between morphological and chloroplast data likely points to a complex evolutionary history in this group. In conclusion, both hypotheses to be tested, 1) that Corymbia is monophyletic and 2) that the currently recognised subgenera of Corymbia are monophyletic, are not supported based on the chloroplast data.

Some phylogenetic signal in the cpDNA data is geographic, and Fig 4 (for clade A) and Fig 5 (for clade B) illustrate the proximity of accession localities that form subclades within the major two ingroup clades. For example, Fig 4B shows the geographic proximity of accessions included in clade A1 (Fig 3), which is composed of members of sections Maculatae and Naviculares, and Fig 5 shows geographic groups within clade B that each include a mix of species from different taxonomic series (see Table 1) within sections Septentrionales and Abbreviatae.

Fig 4. Distribution of samples placed in clade A in the cpDNA phylogeny (Fig 3).

Fig 4

Colour coding of groups matches that used in other figures. Accession details are shown for four samples mentioned in the text.

Fig 5. Distribution of samples placed in clade B in the cpDNA phylogeny (Fig 3).

Fig 5

(A) Samples classified in sect. Septentrionales; (B) samples classified in sect. Abbreviatae, with inset in lower right showing detail for area outlined by dashed rectangle. Details are shown for some clades, species, and accessions mentioned in the text. Colour coding of groups matches that used in other figures.

Analysis of nuclear ribosomal DNA

The nrDNA dataset included 663 aligned bases and 337 distinct alignment patterns (see supplementary material S3 File). AIC from jModelTest indicated a General Time Reversible model using gamma distribution of rates and a proportion of invariant sites (GTR+I+G), used for analysis here, and BIC indicated GTR+G as the best fit. Final ML optimization likelihood was -4709.258464. The MP analysis included 170 parsimony informative characters and the alignment had 90 variable but uninformative characters. Maximum parsimony analysis resulted in 1610 trees with length = 644, consistency index = 0.55, and retention index = 0.90. Topologies of the ML and MP trees were similar, and the ML tree is shown here, with MP bootstrap support values mapped onto it (Fig 6).

Fig 6. Phylogeny resulting from nrDNA analyses.

Fig 6

Best-scoring maximum likelihood tree from a RAxML analysis (final ML optimization likelihood of -4709.258464) of a nrITS dataset (663 base pairs, 337 distinct alignment patterns, 119 accessions) of eucalypts. The outgroup (OG), major groups in Eucalyptus (‘Eudesmids’, ‘Monocalypts’ [Mono], and ‘Symphyomyrts’ [Symph]), subgenera and infrageneric groups of Corymbia are indicated with bars or colouring scheme (see textbox) on the tree. Species names are followed by GenBank accession numbers. Bootstrap support values are shown as percent maximum likelihood/maximum parsimony (MP mapped onto ML tree) with weighted edges indicating 100% support for both ML and MP. Support values <50% are omitted or dashed when the alternate analysis method had ≥50% support. i Identified in GenBank (GB) as Angophora exul K.D.Hill, a name that is synonymised with A. bakeri in the current Australian Plant Census (APC) [1]. ii Identified in GB as Angophora euryphylla (G.J.Leach) L.A.S.Johnson & K.D.Hill, a name that is synonymised with A. costata subsp. euryphylla in the current APC. iii Identified in GB as Corymbia variegata (F.Muell.) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. citriodora in the current APC. iv Identified in GB as Corymbia dolichocarpa (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. clarksoniana in the current APC. v Identified in GB as Corymbia dampieri (D.J.Carr & S.G.M.Carr) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. greeniana in the current APC. vi Identified in GB as Corymbia dimorpha (Brooker & A.R.Bean) K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. peltata in the current APC. vii Identified in GB as Corymbia catenaria K.D.Hill & L.A.S.Johnson, a name that is synonymised with C. watsoniana subsp. capillata in the current APC.

Analyses strongly supported the monophyly of Eucalyptus and of Corymbia + Angophora (both with ML/MP BS of 100%). Relationships within Eucalyptus were similar to those in the cpDNA tree, in that they resolved the main ‘Monocalypt’ and ‘Symphyomyrt’ clades, subtended by subg. Eudesmia (E. erythrocorys), although the position of monotypic subg. Acerosae (E. curtisii) was not resolved with support.

Corymbia was resolved as paraphyletic with respect to Angophora, and that relationship received weak to moderate support (BS of<50% for ML and 71% for MP). Within Corymbia, there was support for the monophyly of subg. Corymbia (ML/MP BS of 74/75%) and subg. Blakella (BS 99/98%). Monophyly was also supported for Corymbia sections Maculatae (BS 75/83%) and Naviculares (BS 90/86%). Relationships of other Corymbia sections represented by more than one species were generally poorly supported, i.e.: sect. Septentrionales was resolved as paraphyletic, but with < 50% ML or MP BS; sect. Calophyllae was resolved as paraphyletic, on account of placement of C. gummifera (monotypic sect. Corymbia) with two samples of C. ficifolia with weak support (BS 60/58%); sect. Abbreviatae was resolved as paraphyletic with respect to monotypic sect. Torellianae, but only in the ML tree and with <50% bootstrap support. In conclusion, support was mixed for the hypotheses being tested here, 1) that Corymbia is monophyletic and 2) that the currently recognised subgenera of Corymbia are monophyletic. For hypothesis 1), the data are largely equivocal, there being only weak support for the nesting of Angophora in Corymbia (<50% BS for ML and 71% for MP); for hypothesis 2), the current subgeneric classification of Corymbia was moderately to strongly supported.

Discussion

The relationships within Eucalyptus generally confirm those of previous HTS studies [41] and therefore, our results for relationships among Eucalyptus will not be discussed further as our focus here is on Corymbia and Angophora.

Why are cpDNA relationships incongruent with nrDNA relationships and infrageneric classification of Corymbia?

A key result of the current study is that cpDNA relationships in Corymbia (Fig 3) are largely incongruent with the current circumscriptions of subgenera and sections, and with relationships inferred based on nrDNA (Fig 6). Such incongruence could occur if: A) current infrageneric groups are poorly defined and in need of taxonomic revision; B) the nrDNA gene tree does not accurately reflect phylogenetic relationships, e.g., as a result of mixing of orthologous and paralogous copies of this multi-copy cistron [60,64,65]; C) the cpDNA gene tree does not accurately reflect the phylogenetic relationships of taxa, e.g., as a result of processes such as incomplete lineage sorting [66,67,68] or chloroplast capture resulting from hybridisation and introgression [69,70]. We infer that the observed incongruence is consistent with the last explanation and, in particular, points to historical hybridisation and cpDNA introgression between lineages, as outlined below.

In conflict with the cpDNA gene tree, evidence for the monophyly of major infrageneric groups in Corymbia (subgenera and sections) comes from a general concordance between phylogenies based on nrDNA sequences (e.g., [6,29,30]) and morphologically defined infrageneric groups. For instance, the analysis of nrDNA presented here (Fig 6), based on ITS sequences, supports monophyly of the two subgenera (subg. Corymbia and subg. Blakella), the yellow bloodwoods (sect. Naviculares) and the spotted gums (sect. Maculatae), and it does not strongly contradict the monophyly of the ghost gums (sect. Abbreviatae). Most of these groups have historically been recognised on morphological grounds, although at varying taxonomic levels (e.g., [2,3,4]). Such concordance, from independent data sources, provides support for the notion that, on the whole, these taxa represent phylogenetic groups. Thus, it is striking that, among the molecular phylogenetic studies of Corymbia, it is only those including chloroplast data that show strongly supported nodes in conflict with the recognition of these groups (current study and [31,40]). Understanding the reasons for this conflict is central to gaining insight into the evolutionary history of Corymbia, and to properly testing its classification.

Chloroplast capture and incomplete lineage sorting are two processes commonly inferred to account for incongruence in plants between chloroplast DNA relationships and nuclear DNA phylogenies/morphological taxonomy. The relative importance of these processes can be difficult to infer or disentangle [71], but some clues can come from knowledge of the reproductive biology of the plants and of geographic patterns of DNA sequence variation. In terms of reproductive biology, a capacity to hybridise and interbreed is a necessary pre-requisite for the transfer of chloroplasts between lineages. In terms of geography, introgression necessarily occurs at particular locations, and can lead to geographic clustering in the sharing of related chloroplast sequences between species [71]. In contrast, such geographic clustering might not be expected in cases where incongruence with taxonomy results from incomplete lineage sorting of chloroplast genomes (e.g. [72]).

Although incomplete lineage sorting cannot be excluded as an explanation for aspects of cpDNA relationships in Corymbia, it seems likely from the reproductive biology of these trees (and that of other eucalypt genera), together with geographic patterns of cpDNA variation, that the observed patterns are largely consistent with a history of hybridisation and introgression. In terms of reproductive compatibility, pre-zygotic barriers to reproduction have been reported between some Corymbia species [73], but all members of Corymbia investigated so far have the same chromosome number (2n = 22; [74,75]). Both morphological variation and experimental crosses [2,73,76,77] provide evidence of substantial potential for hybridisation between species classified in different series, sections, and subgenera (summarised in Fig 7). Given this capacity for hybridisation across infrageneric groups, it seems likely that the taxonomic incongruence of cpDNA relationships in Corymbia could reflect similar processes to those seen in the better studied Eucalyptus. In Eucalyptus, such incongruence is clearly evident, with chloroplast variation commonly reflecting geography, rather than taxonomy, and widespread regional introgression of cpDNA between species, series, and sections is regularly inferred [71,78,79,80,81,82,83,84,85].

Fig 7. Summary of hybridisation between infrageneric groups of Corymbia inferred by previous studies [2,73,77].

Fig 7

Arrows connect taxa with inferred hybrids. (A) Inferred intersectional hybrids; (B) interseries hybrids in subg. Corymbia; (C) interseries hybrids in subg. Blakella.

Geographic patterns in Corymbia observed here (Figs 4 and 5) provide support for a history of cpDNA introgression between species, in the form of geographically clustered cpDNA clades shared among taxa that would be considered distinct lineages based on morphological or nrDNA evidence. Such patterns are consistent with cpDNA introgression between species across a range of morphological infrageneric groups.

Some of the clearest geographic patterns in our dataset relate to geographic cpDNA clades shared among species classified, on the basis of morphology [2], in different taxonomic series (Table 1) within the same section. For example, within sect. Septentrionales three geographic clades in north Queensland each contain a mixture of species placed in different taxonomic series, i.e., clade B1 (containing members of ser. Arenariae, Polycarpae, and Dichromophloiae; Fig 3), clade B2 (containing members of ser. Rhodopes and Abergianae), and clade B3 (containing members of ser. Trachyphloiae and Polycarpae). Likewise, clade B5 (including members of ser. Dichromophloiae and ser. Ferrugineae) is geographically clustered in the Mid-West region of Western Australia. Apart from the monotypic ser. Abergianae, series with species falling in clades B1, B2, B3, and B5 are also distributed across other clades in the phylogeny and hence not monophyletic (e.g., C. dichromophloia, C. hamersleyana, and C. trachyphloia). Similar patterns are also seen in clades of sect. Abbreviatae, where clade B4 includes intermixed representatives of series Polysciadae and Papuanae, and clade B6 includes intermixed members of ser. Grandifoliae and Asperae. Interestingly, in clade B4, the morphologically distinctive species C. polysciada (ser. Polysciadae) is strongly supported as polyphyletic, with the two accessions each having cpDNA haplotypes more closely related to those of closely occurring species from ser. Papuanae (compare Fig 3 and inset on Fig 5B). Although each of these morphologically defined series present in clades B1–B6 cannot be assumed a priori to represent monophyletic groups (e.g., there is no nuclear genetic evidence to support their monophyly), the presence of geographically distinct chloroplast clades found across morphologically distinctive taxa suggests a history of local chloroplast introgression between lineages, much as seen in Eucalyptus.

Geographic patterns in cpDNA clades shared across different taxonomic sections or subgenera are less clear than those among series, but geographic links can still be discerned. For instance, clade A1 (Fig 3) although ranging from north Queensland to southern New South Wales in eastern Australia, has a cluster of samples from south-east Queensland including one of C. citriodora (sect. Maculatae) that groups in the cpDNA gene tree as sister to a clade including a sample of C. leichhardtii (sect. Naviculares) that occurs nearby (Fig 4B). Similarly, clade A2, ranging from northern New South Wales to mid-east Queensland (Fig 4C), includes, in reasonably close geographic proximity, members of sect. Maculatae, together with C. torelliana of monotypic sect. Torellianae. However, the representative of sect. Naviculares in this clade is geographically more distant, and the representative of sect. Abbreviate could not be mapped because the sample is of unknown provenance. At least the geographic and cpDNA association of C. torelliana and the three samples of sect. Maculatae is consistent with known capacity for these groups to interbreed [73,76]. Again, these groups (although not these species) have previously been reported to hybridise ([77]; Fig 7).

A striking feature of the cpDNA tree is placement of two clades of ghost gums, subg. Blakella sect. Abbreviatae (clades B4 and B6; Fig 3), within the large clade B that otherwise includes almost all samples of the red bloodwood group subg. Corymbia sect. Septentrionales. This contrasts with phylogenetic analyses of nrDNA sequences (Fig 6 and [6,25,27,29,30]), in which sect. Abbreviatae groups with other members of subg. Blakella. The geographic clustering of clades B4 and B6, and their distribution in areas where members of sect. Septentrionales are common, especially in the Northern Territory, is consistent with these clades reflecting historical chloroplast transfer from red bloodwoods to ghost gums, e.g., potentially two distinct events of chloroplast transfer, in each case with a red bloodwood as the initial maternal parent. Hybridisation between these groups has not, to our knowledge, been reported (e.g. Fig 7; [2,73,77]).

It is worth noting that taxon sampling for the current study was designed primarily to sample across the major taxonomic groups of Corymbia, to assess their relationships on the basis of chloroplast sequences, and it was not designed specifically to assess geographic patterns of chloroplast variation. As such, there are substantial geographic distances between many samples, and the spread of samples is quite unbalanced, e.g., with only one sample of sect. Abbreviatae from eastern Australia (C. tessellaris, of unknown wild provenance), and none from the north-west of Western Australia. The inferences here of historical chloroplast introgression between major taxonomic groups, especially subgenera and some sections, are consistent with the observed patterns of cpDNA variation, and knowledge of bloodwood reproductive biology, but remain speculative. Our study provides insight into the potential importance of this process in the evolutionary history of Corymbia, but more detailed studies using fine-scale geographic sampling, including multiple replicates of species, are necessary both to properly test for the presence of chloroplast introgression, and to more fully appreciate its significance and any accompanying patterns of nuclear gene flow.

Chloroplast DNA relationships in Angophora

The genus Angophora was strongly supported as monophyletic, as universally found in all molecular phylogenetic studies of eucalypts that have sampled two or more Angophora species (e.g. [6,27,29,30,31]). Most previous studies have included only a small number of exemplars from Angophora and thus both species limits, which differ between some treatments [1,18,86,87], and the proposed infrageneric classification [87], have not been critically tested by molecular data. Our cpDNA study included multiple accessions of four species, three of which were strongly indicated as paraphyletic or polyphyletic (Fig 3); the one species that was resolved as monophyletic, A. melanoxylon, was represented by only two samples from the same geographic area, near St George in south-east Queensland. The sample set here is small (15 samples from 8 species), and was not collected to assess geographic variation within/between taxa, but it seems reasonable that taxonomic incongruence with cpDNA variation in Angophora, as in Eucalyptus and Corymbia (see above) reflects, at least in part, a history of cpDNA introgression between species. Consistent with this is the resolution of A. subvelutina as paraphyletic (in particular, with one sample shown as sister to a closely co-occurring sample of A. bakeri), and the polyphyly of A. floribunda, in which the northern-most sample of known provenance (TMS14–33; Table 1) falls in a clade of other samples from nearby areas, and is well separated in the phylogeny from the southernmost sample (MJB 2471). An influence of chloroplast introgression on this gene tree would be consistent with the observation of Leach [86] that hybridisation between species of Angophora "… has been observed in virtually all combinations that are geographically or ecologically conceivable". As with Corymbia, fine-scale studies of cpDNA variation could be used to test for both the presence and extent of cpDNA introgression amongst Angophora species.

Implications for genus-level taxonomy

A primary aim of this study was to use HTS chloroplast data, from a broad sample of infrageneric groups, to test the monophyly of the bloodwood genus Corymbia as currently circumscribed. The inferred chloroplast relationships strongly support nesting of Angophora in Corymbia thus making it paraphyletic (Fig 3), as also shown, with less support, in previous cpDNA studies using either more limited taxon sampling or more limited sampling of the chloroplast genome [26,28,31,40,41]. However, given the clear incongruence between the cpDNA gene tree and taxonomic boundaries that are otherwise supported by both morphological characters and analyses of nrDNA, and given the likely influence of historical cpDNA introgression between lineages (discussed above), the cpDNA data, on their own, do not provide a sound basis for assessing generic limits in this group. It is worth noting that it seems unlikely that the close cpDNA relationship of Angophora to some groups of Corymbia could be directly attributed to cpDNA introgression (at least not recently), because CorymbiaAngophora hybrids have not been reported (e.g. [2,73,77]), despite common co-occurrence of species [2] and attempts at artificial crosses (e.g. [73]).

To make sound taxonomic decisions, especially regarding the limits of genera and subgenera, among the bloodwoods and their relatives, better knowledge of relationships based on nuclear DNA sequences is essential. Analyses of nuclear DNA datasets have so far been limited to the ITS, ETS and 5S regions of nrDNA [6,25,27,29,30,38] and a small number of microsatellite markers [39], and have given mixed support for the monophyly/paraphyly of Corymbia. The nrDNA analyses here (Fig 6), for instance, using only ITS data, show 71% BS for the nesting of Angophora in Corymbia in the MP analysis but <50% support in the ML analysis, leaving open the possibility that Angophora might be sister to a monophyletic Corymbia. More thorough assessment of relationships will require analysis of more substantial datasets, for which there are now good prospects using HTS methods [37].

Even if Angophora proves to be nested in Corymbia based on nuclear data, placing them together in one genus might not be the best taxonomic solution for this group. Instead, raising one or more of the infrageneric groups of Corymbia to genus rank might be a better solution for recognising monophyletic, morphologically diagnosable (less heterogeneous) groups and minimising taxonomic upheaval (number of name changes). Adopting such a solution would first require clear understanding of the relationships of the bloodwood lineages to each other and to Angophora, informed by nuclear data, as well as the chloroplast data presented here. In the interim, and in the absence of other strongly contradictory evidence, we support continued recognition of both Angophora and Corymbia and the infrageneric groups of Corymbia as currently defined [6]. This is because there is support for most of these groups based on nrDNA data and morphology, and because name changes that are not soundly based, or might subsequently need revision in the face of stronger evidence, would cause major taxonomic instability in these economically important groups.

Supporting information

S1 File. Workflow used in CLC Genomics Workbench v. 9.5.1 and 9.5.2 (Qiagen).

Quality control and assembly of HTS chloroplast DNA sequences (Excel file).

(XLSX)

S2 File. Alignment of chloroplast data.

Alignment (121,016 base pairs) of chloroplast sequences for 123 accessions of eucalypts (phylip file format).

(PHY)

S3 File. Alignment of nuclear ribosomal data.

Alignment (663 base pairs) of nrITS sequences for 119 accessions of eucalypts (phylip file format).

(PHY)

Acknowledgments

We thank Frances Bayly, Gill Brown (BRI), Alison Kellow (La Trobe University), Pauline Ladiges (The University of Melbourne), and Karen Wilson (NSW), who either provided material or assisted with field work, and Claudine Griffin-Beale for helping to locate some Angophora species. We are grateful to Neil Gibson (WA) for collecting Corymbia during the ABRS Katjarra Region Bushblitz. In particular, we thank Dean Nicolle for access to the impressive living collection of eucalypts at Currency Creek Arboretum. We gratefully acknowledge Alex Johnson and Julien Bonneau for access to equipment (The University of Melbourne, Plant Nutrition Lab), Liz Milla (Walter and Eliza Hall Institute of Medical Research) for HTS data pre-processing, and Heroen Verbruggen (The University of Melbourne, Algae Lab) and Wake Forest University for computational resources. Will Neal and Harvey Orel assisted with the mounting and databasing of voucher specimens. Plant collecting permits were provided by the Victorian Department of Sustainability and Environment, New South Wales National Parks and Wildlife Service, and Northern Territory Parks and Wildlife Commission.

Data Availability

DNA sequences are available in GenBank (https://www.ncbi.nlm.nih.gov/genbank/), with accession numbers as listed in Table 1. DNA alignments and other files are provided as Supplementary Material.

Funding Statement

This research was funded by The Hermon Slade Foundation (grant HSF14-09 to TMS and JFGT; http://www.hermonslade.org.au), The Bjarne K. Dahl Trust (grants in 2014 and 2015 to MJB and PKA; https://dahltrust.org.au), and The University of Melbourne Botany Foundation (TMS support funds; http://science.unimelb.edu.au/engage/giving-to-science/botany-foundation). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

References

  • 1.CHAH (2017) Australian plant census [online]. Council of Heads of Australasian Herbaria. Available from: https://biodiversity.org.au/nsl/services/apc. [Google Scholar]
  • 2.Hill KD, Johnson LA (1995) Systematic studies in the eucalypts 7. A revision of the bloodwoods, genus Corymbia (Myrtaceae). Telopea 6: 185–504. [Google Scholar]
  • 3.Pryor LD, Johnson LA (1971) A classification of the eucalypts Canberra: Australian National University Press. [Google Scholar]
  • 4.Brooker MIH (2000) A new classification of the genus Eucalyptus L'Her. (Myrtaceae). Aust Syst Bot 13: 79–148. [Google Scholar]
  • 5.Nicolle D (2015) Classification of the eucalypts. version 2. Available from: http://www.dn.com.au/Classification-Of-The-Eucalypts.pdf. [Google Scholar]
  • 6.Parra O C, Bayly MJ, Drinnan A, Udovicic F, Ladiges P (2009) Phylogeny, major clades and infrageneric classification of Corymbia (Myrtaceae), based on nuclear ribosomal DNA and morphology. Aust Syst Bot 22: 384–399. [Google Scholar]
  • 7.Williams JE, Woinarski JCZ (1997) Eucalypt Ecology: Individuals to Ecosystems. Cambridge: Cambridge University Press. [Google Scholar]
  • 8.Chippendale GM (1988) Flora of Australia Vol. 19 Canberra: Australian Government Publishing Service. [Google Scholar]
  • 9.Boland DJ, Brooker MIH, Chippendale G, Hall N, Hyland B, et al. (2006) Forest trees of Australia Melbourne: CSIRO publishing. [Google Scholar]
  • 10.MacPherson J (1939) The Eucalyptus in the Daily Life and Medical Practice of the Australian Aborigines. Mankind 2: 175–180. [Google Scholar]
  • 11.Packer J, Brouwer N, Harrington D, Gaikwad J, Heron R, et al. (2012) An ethnobotanical study of medicinal plants used by the Yaegl Aboriginal community in northern New South Wales, Australia. J Ethnopharmacol 139: 244–255. doi: 10.1016/j.jep.2011.11.008 [DOI] [PubMed] [Google Scholar]
  • 12.Reid EJ, Betts TJ (1979) Records of Western Australian Plants Used by Aboriginals as Medicinal Agents. Planta Med 36: 164–173. doi: 10.1055/s-0028-1097257 [DOI] [PubMed] [Google Scholar]
  • 13.Batish DR, Singh HP, Kohli RK, Kaur S (2008) Eucalyptus essential oil as a natural pesticide. For Ecol Manage 256: 2166–2174. [Google Scholar]
  • 14.Low D, Rawal BD, Griffin WJ (1974) Antibacterial action of the essential oils of some Australian Myrtaceae with special references to the activity of chromatographic fractions of oil of Eucalyptus citriodora. Planta Med 26: 184–189. doi: 10.1055/s-0028-1097987 [DOI] [PubMed] [Google Scholar]
  • 15.Ramezani H, Singh HP, Batish DR, Kohli RK (2002) Antifungal activity of the volatile oil of Eucalyptus citriodora. Fitoterapia 73: 261–262. [DOI] [PubMed] [Google Scholar]
  • 16.Ladiges PY, Udovicic F, Nelson G (2003) Australian biogeographical connections and the phylogeny of large genera in the plant family Myrtaceae. J Biogeogr 30: 989–998. [Google Scholar]
  • 17.Wilson PG, O'Brien M, Heslewood M, Quinn C (2005) Relationships within Myrtaceae sensu lato based on a matK phylogeny. Pl Syst Evol 251: 3–19. [Google Scholar]
  • 18.Slee AV, Connors J, Brooker MIH, Duffy SM, West JG (2006) EUCLID Eucalypts of Australia. CD ROM Centre for Plant Biodiversity Research. Melbourne: CSIRO Publishing. [Google Scholar]
  • 19.Dawson JW (1970) Pacific capsular Myrtaceae 1. Reproductive morphology of Arillastrum gummiferum Panch. ex Baillon (New Caledonia). Blumea 18: 431–440. [Google Scholar]
  • 20.Carr DJ, Carr S, Hyland B, Wilson PG, Ladiges PY (2002) Stockwellia quadrifida (Myrtaceae), a new Australian genus and species in the eucalypt group. Bot J Linn Soc 139: 415–421. [Google Scholar]
  • 21.Blake S (1977) Allosyncarpia ternata, a new genus and species of Myrtaceae subfamily Leptospermoideae from northern Australia. Austrobaileya: 43–46. [Google Scholar]
  • 22.Craven L (1990) One new species each in Acmena and Eucalyptopsis and a new name in Lindsayomyrtus (all Myrtaceae). Aust Syst Bot 3: 727–732. [Google Scholar]
  • 23.Ladiges PY, Udovicic F (2000) Comment on a new classification of the eucalypts. Aust Syst Bot 13: 149–152. [Google Scholar]
  • 24.Ladiges PY, Udovicic F, Drinnan AN (1995) Eucalypt phylogeny–molecules and morphology. Aust Syst Bot 8: 483–497. [Google Scholar]
  • 25.Udovicic F, McFadden G, Ladiges P (1995) Phylogeny of Eucalyptus and Angophora based on 5S rDNA spacer sequence data. Mol Phyl Evol 4: 247–256. [DOI] [PubMed] [Google Scholar]
  • 26.Udovicic F, Ladiges PY (2000) Informativeness of nuclear and chloroplast DNA relationships of the eucalypt and related genera (Myrtaceae). Kew Bull 55: 633–645. [Google Scholar]
  • 27.Parra O C, Bayly MJ, Udovicic F, Ladiges PY (2006) ETS sequences support the monophyly of the eucalypt genus Corymbia (Myrtaceae). Taxon 55: 653–663. [Google Scholar]
  • 28.Whittock S, Steane D, Vaillancourt R, Potts B (2003) Molecular evidence shows that the tropical boxes (Eucalyptus subgenus Minutifructus) are over-ranked. Trans R Soc S Aust 1217: 27–32. [Google Scholar]
  • 29.Steane DA, McKinnon GE, Vaillancourt RE, Potts BM (1999) ITS sequence data resolve higher level relationships among the eucalypts. Mol Phyl Evol 12: 215–223. [DOI] [PubMed] [Google Scholar]
  • 30.Steane DA, Nicolle D, McKinnon GE, Vaillancourt RE, Potts BM (2002) Higher-level relationships among the eucalypts are resolved by ITS-sequence data. Aust Syst Bot 15: 49–62. [Google Scholar]
  • 31.González-Orozco CE, Pollock LJ, Thornhill AH, Mishler BD, Knerr N, et al. (2016) Phylogenetic approaches reveal biodiversity threats under climate change. Nat Clim Change 6: 1110–1114. [Google Scholar]
  • 32.Ladiges P (1984) A comparative study of Trichomes in Angophora Cav. and Eucalyptus–a question of homology. Aust J Bot 32: 561–574. [Google Scholar]
  • 33.Bentham G (1866) Flora Australiensis, III. London: Lovell Reeve. [Google Scholar]
  • 34.Maiden JH (1909) A critical revision of the genus Eucalyptus Sydney: Gullick. [Google Scholar]
  • 35.Blakely WF (1965) A Key to the Eucalypts Canberra: Forestry and Timber Bureau. [Google Scholar]
  • 36.Cavanilles A (1797) Icones et Descriptiones Plantarum, IV. Madrid: Regia Typographia. [Google Scholar]
  • 37.Bayly MJ (2016) Phylogenetic studies of eucalypts: fossils, morphology and genomes. Proc R Soc Vic 128: 12–24. [Google Scholar]
  • 38.Ochieng JW, Henry RJ, Baverstock PR, Steane DA, Shepherd M (2007) Nuclear ribosomal pseudogenes resolve a corroborated monophyly of the eucalypt genus Corymbia despite misleading hypotheses at functional ITS paralogs. Mol Phyl Evol 44: 752–764. [DOI] [PubMed] [Google Scholar]
  • 39.Ochieng JW, Steane DA, Ladiges PY, Baverstock PR, Henry RJ, et al. (2007) Microsatellites retain phylogenetic signals across genera in eucalypts (Myrtaceae). Genet Mol Biol 30: 1125–1134. [Google Scholar]
  • 40.Parra-O C (2009) Chapter 6, Chloroplast DNA (cpDNA). In: Parra-O C, editor. A phylogenetic analysis of the bloodwood eucalypts (Myrtaceae): PhD Thesis, The University of Melbourne.
  • 41.Bayly MJ, Rigault P, Spokevicius A, Ladiges PY, Ades PK, et al. (2013) Chloroplast genome analysis of Australian eucalypts–Eucalyptus, Corymbia, Angophora, Allosyncarpia and Stockwellia (Myrtaceae). Mol Phyl Evol 69: 704–716. [DOI] [PubMed] [Google Scholar]
  • 42.Steane DA (2005) Complete nucleotide sequence of the chloroplast genome from the Tasmanian blue gum, Eucalyptus globulus (Myrtaceae). DNA Res 12: 215–220. doi: 10.1093/dnares/dsi006 [DOI] [PubMed] [Google Scholar]
  • 43.Paiva JA, Prat E, Vautrin S, Santos MD, San-Clemente H, et al. (2011) Advancing Eucalyptus genomics: identification and sequencing of lignin biosynthesis genes from deep-coverage BAC libraries. BMC Genomics 12: 137 doi: 10.1186/1471-2164-12-137 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 44.Doyle JJ, Doyle JL (1987) A rapid isolation procedure for small quantities of fresh leaf material. Phytochem Bull 19: 11–15. [Google Scholar]
  • 45.McLay TG (2017) High quality DNA extraction protocol from recalcitrant plant tissues. protocols.io. Available from: https://www.protocols.io/view/high-quality-dna-extraction-protocol-from-recalcit-i8jchun?more.
  • 46.Shepherd LD, McLay TG (2011) Two micro-scale protocols for the isolation of DNA from polysaccharide-rich plant tissue. J Plant Res 124: 311–314. doi: 10.1007/s10265-010-0379-5 [DOI] [PubMed] [Google Scholar]
  • 47.Rohland N, Reich D (2012) Cost-effective, high-throughput DNA sequencing libraries for multiplexed target capture. Genome Res 22: 939–946. doi: 10.1101/gr.128124.111 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 48.Katoh K, Standley DM (2013) MAFFT multiple sequence alignment software version 7: improvements in performance and usability. Mol Biol Evol 30: 772–780. doi: 10.1093/molbev/mst010 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 49.Gouy M, Guindon S, Gascuel O (2009) SeaView version 4: a multiplatform graphical user interface for sequence alignment and phylogenetic tree building. Mol Biol Evol 27: 221–224. doi: 10.1093/molbev/msp259 [DOI] [PubMed] [Google Scholar]
  • 50.Maddison WP, Maddison DR (2013) Mesquite version 3.1: a modular system for evolutionary analysis. http://mequiteproject.org/.
  • 51.Castresana J (2000) Selection of conserved blocks from multiple alignments for their use in phylogenetic analysis. Mol Biol Evol 17: 540–552. doi: 10.1093/oxfordjournals.molbev.a026334 [DOI] [PubMed] [Google Scholar]
  • 52.Darriba D, Taboada GL, Doallo R, Posada D (2012) jModelTest 2: more models, new heuristics and parallel computing. Nat Methods 9: 772–772. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 53.Guindon S, Gascuel O (2003) A simple, fast, and accurate algorithm to estimate large phylogenies by maximum likelihood. Syst Biol 52: 696–704. [DOI] [PubMed] [Google Scholar]
  • 54.Stamatakis A (2014) RAxML version 8: a tool for phylogenetic analysis and post-analysis of large phylogenies. Bioinformatics 30: 1312–1313. doi: 10.1093/bioinformatics/btu033 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 55.Swofford D (2002) PAUP*. Phylogenetic Analysis Using Parsimony (* and Other Methods). 4 ed: Sinauer Associates, Sunderland, Massachusetts. [Google Scholar]
  • 56.Rambaut A (2016) FigTree Tree Figure Drawing Tool version 1.4.3. http://tree.bio.ed.ac.uk/software/figtree/.
  • 57.Gibbs AK, Udovicic F, Drinnan AN, Ladiges PY (2009) Phylogeny and classification of Eucalyptus subgenus Eudesmia (Myrtaceae) based on nuclear ribosomal DNA, chloroplast DNA and morphology. Aust Syst Bot 22: 158–179. [Google Scholar]
  • 58.Ladiges PY, Bayly M, Nelson G (2010) East-west continental vicariance in Eucalyptus subgenus Eucalyptus In: Williams D, Knapp S, editors. Beyond Cladistics. The Branching of a Paradigm. Berkeley: University of California Press; pp. 267–302. [Google Scholar]
  • 59.Bayly MJ, Ladiges PY (2007) Divergent paralogues of ribosomal DNA in eucalypts (Myrtaceae). Mol Phyl Evol 44: 346–356. [DOI] [PubMed] [Google Scholar]
  • 60.Bayly MJ, Udovicic F, Gibbs AK, Ladiges PY (2008) Ribosomal DNA pseudogenes are widespread in the eucalypt group (Myrtaceae): implications for phylogenetic analysis. Cladistics 24: 131–146. [Google Scholar]
  • 61.Burke JM, Bayly MJ, Adams PB, Ladiges PY (2008) Molecular phylogenetic analysis of Dendrobium (Orchidaceae), with emphasis on the Australian section Dendrocoryne, and implications for generic classification. Aust Syst Bot 21: 1–14. [Google Scholar]
  • 62.Holmes GD, Downing TL, James EA, Blacket MJ, Hoffmann AA, et al. (2014) Phylogeny of the holly grevilleas (Proteaceae) based on nuclear ribosomal and chloroplast DNA. Aust Syst Bot 27: 56–77. [Google Scholar]
  • 63.Kearse M, Moir R, Wilson A, Stones-Havas S, Cheung M, et al. (2012) Geneious Basic: an integrated and extendable desktop software platform for the organization and analysis of sequence data. Bioinformatics 28: 1647–1649. doi: 10.1093/bioinformatics/bts199 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 64.Bailey CD, Carr TG, Harris SA, Hughes CE (2003) Characterization of angiosperm nrDNA polymorphism, paralogy, and pseudogenes. Mol Phyl Evol 29: 435–455. [DOI] [PubMed] [Google Scholar]
  • 65.Mayol M, Rosselló JA (2001) Why nuclear ribosomal DNA spacers (ITS) tell different stories in Quercus. Mol Phyl Evol 19: 167–176. [DOI] [PubMed] [Google Scholar]
  • 66.Baum DA, Smith SD (2013) Tree thinking: an introduction to phylogenetic biology. Greenwood Village, Colarado: Roberts and Company. [Google Scholar]
  • 67.Doyle JJ (1992) Gene trees and species trees: molecular systematics as one-character taxonomy. Syst Bot: 144–163. [Google Scholar]
  • 68.Maddison WP (1997) Gene trees in species trees. Syst Biol 46: 523–536. [Google Scholar]
  • 69.Tsitrone A, Kirkpatrick M, Levin DA, Morgan M (2003) A model for chloroplast capture. Evolution 57: 1776–1782. [DOI] [PubMed] [Google Scholar]
  • 70.Rieseberg LH, Soltis D (1991) Phylogenetic consequences of cytoplasmic gene flow in plants. Evol Trends Pl 5: 65–84. [Google Scholar]
  • 71.McKinnon GE, Jordan GJ, Vaillancourt RE, Steane DA, Potts BM (2004) Glacial refugia and reticulate evolution: the case of the Tasmanian eucalypts. Philos Trans R Soc Lond, B, Biol Sci 359: 275–284. doi: 10.1098/rstb.2003.1391 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 72.Meudt HM, Bayly MJ (2008) Phylogeographic patterns in the Australasian genus Chionohebe (Veronica s.l., Plantaginaceae) based on AFLP and chloroplast DNA sequences. Mol Phyl Evol 47: 319–338. [DOI] [PubMed] [Google Scholar]
  • 73.Dickinson GR, Lee DJ, Wallace HM (2012) The influence of pre-and post-zygotic barriers on interspecific Corymbia hybridization. Ann Bot 109: 1215–1226. doi: 10.1093/aob/mcs050 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 74.Grattapaglia D, Vaillancourt RE, Shepherd M, Thumma BR, Foley W, et al. (2012) Progress in Myrtaceae genetics and genomics: Eucalyptus as the pivotal genus. Tree Genetics & Genomes 8: 463–508. [Google Scholar]
  • 75.Oudjehih B, Abdellah B (2006) Chromosome numbers of the 59 species of Eucalyptus L'Herit. (Myrtaceae). Caryologia 59: 207–212. [Google Scholar]
  • 76.Barbour R, Crawford AC, Henson M, Lee DJ, Potts B, et al. (2008) The risk of pollen-mediated gene flow from exotic Corymbia plantations into native Corymbia populations in Australia. For Ecol Manage 256: 1–19. [Google Scholar]
  • 77.Griffin A, Burgess I, Wolf L (1988) Patterns of natural and manipulated hybridisation in the genus Eucalyptus L’Hér.–a review. Aust J Bot 36: 41–66. [Google Scholar]
  • 78.Jackson H, Steane D, Potts B, Vaillancourt R (1999) Chloroplast DNA evidence for reticulate evolution in Eucalyptus (Myrtaceae). Mol Ecol 8: 739–751. [Google Scholar]
  • 79.McKinnon G, Smith J, Potts B (2010) Recurrent nuclear DNA introgression accompanies chloroplast DNA exchange between two eucalypt species. Mol Ecol 19: 1367–1380. doi: 10.1111/j.1365-294X.2010.04579.x [DOI] [PubMed] [Google Scholar]
  • 80.McKinnon GE, Steane DA, Potts BM, Vaillancourt RE (1999) Incongruence between chloroplast and species phylogenies in Eucalyptus subgenus Monocalyptus (Myrtaceae). Am J Bot 86: 1038–1046. [PubMed] [Google Scholar]
  • 81.McKinnon GE, Vaillancourt RE, Jackson HD, Potts BM (2001) Chloroplast sharing in the Tasmanian eucalypts. Evolution 55: 703–711. [DOI] [PubMed] [Google Scholar]
  • 82.Steane D, Byrne M, Vaillancourt R, Potts B (1998) Chloroplast DNA polymorphism signals complex interspecific interactions in Eucalyptus (Myrtaceae). Aust Syst Bot 11: 25–40. [Google Scholar]
  • 83.Nevill PG, Després T, Bayly MJ, Bossinger G, Ades PK (2014) Shared phylogeographic patterns and widespread chloroplast haplotype sharing in Eucalyptus species with different ecological tolerances. Tree Genetics & Genomes 10: 1079–1092. [Google Scholar]
  • 84.Pollock LJ, Bayly MJ, Nevill PG, Vesk PA (2013) Chloroplast DNA diversity associated with protected slopes and valleys for hybridizing Eucalyptus species on isolated ranges in south-eastern Australia. J Biogeogr 40: 155–167. [Google Scholar]
  • 85.Pollock LJ, Bayly MJ, Vesk PA (2015) The roles of ecological and evolutionary processes in plant community assembly: the environment, hybridization, and introgression influence co-occurrence of Eucalyptus. Am Nat 185: 784–796. doi: 10.1086/680983 [DOI] [PubMed] [Google Scholar]
  • 86.Leach GJ (1986) A revision of the genus Angophora (Myrtaceae). Telopea 2: 749–779. [Google Scholar]
  • 87.Thiele K, Ladiges PY (1988) A cladistic analysis of Angophora Cav. (Myrtaceae). Cladistics 4: 23–42. [DOI] [PubMed] [Google Scholar]

Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Supplementary Materials

S1 File. Workflow used in CLC Genomics Workbench v. 9.5.1 and 9.5.2 (Qiagen).

Quality control and assembly of HTS chloroplast DNA sequences (Excel file).

(XLSX)

S2 File. Alignment of chloroplast data.

Alignment (121,016 base pairs) of chloroplast sequences for 123 accessions of eucalypts (phylip file format).

(PHY)

S3 File. Alignment of nuclear ribosomal data.

Alignment (663 base pairs) of nrITS sequences for 119 accessions of eucalypts (phylip file format).

(PHY)

Data Availability Statement

DNA sequences are available in GenBank (https://www.ncbi.nlm.nih.gov/genbank/), with accession numbers as listed in Table 1. DNA alignments and other files are provided as Supplementary Material.


Articles from PLoS ONE are provided here courtesy of PLOS

RESOURCES