Oil reservoirs in stem, rhizome, and root of Solidago canadensis (Asteraceae, tribe Astereae)

The anatomy of internal secretory spaces in immature and mature aerial stems, rhizomes, and roots of common goldenrod, Solidago canadensis (Asteraceae, tribe Astereae), was studied from resin-embedded samples cut 1–2 μm thick. Oil-filled cavities of different lengths, each lined by a uniseriate epithelium, form in young stems and rhizomes. Epithelial cells enlarge and elongate, and some continue to divide mitotically. The cavities thereby expand and accommodate themselves to the growing stem and rhizome. Septa are sometimes forced open by this enlargement, which merges adjacent cavities. Oil reservoirs in roots are probably also cavities, but their lack of densely cytoplasmic epithelial cells prevented us from locating the end walls. Cavities in stem, root, and the cortex of rhizomes occur only as one median file located just outside of each phloem strand; in the pith of rhizomes, however, several files of cavities of larger diameter seem randomly distributed. This study extends our earlier findings that the oil reservoirs in leaves of this species are cavities; we have therefore verified that cavities, not ducts, permeate the goldenrod plant.     

Anatomy of the vegetative organs and secretory structures of Rhaponticum carthamoides (Asteraceae)

Roots, stems, rhizomes and leaves of Rhaponticum carthamoides (Willd.) Iljin (a Siberian adaptogenic plant, originating from the Altai and Saian Mountains) of different ages were investigated by means of light and electron microscopy. Schizogenous secretory reservoirs occurred in every organ, and were located within the secondary xylem (adventitious roots and rhizome of young plants), at the interface of endodermis/cortical parenchyma (roots and hypocotyl), along phloem and primary xylem (older rhizome), around the vascular bundles (inflorescence stem, petiole and leaf midrib veins) and along phloem (cotyledonary and leaf veins). At the interface of endodermis/inner parenchyma, secretion accumulated in the intercellular spaces prior to the formation of proper epithelial cells. The secretion as observed by transmission electron microscopy comprised three components: soluble (i.e. absent from sections; probably phenolic), insoluble and strongly osmiophilic (probably phenolic) and insoluble, moderately osmiophilic (probably lipidic). Numerous osmiophilic oil droplets, similar to the lipidic secretion inside the reservoirs, local proliferation of rough endoplasmic reticulum and numerous multivesicular bodies characterized epithelial cells in all organs. Leucoplasts (in subterranean organs) with osmiophilic inclusions and peroxisomes with crystalloid inclusions were specific for parenchyma cells. Peltate glandular hairs were formed on leaf blades.  © 2004 The Linnean Society of London, Botanical Journal of the Linnean Society , 2004, 144 , 207–233.     

Occurrence of secretory structures in underground systems of seven Asteraceae species

In contrast with the abundance of anatomical studies of secretory structures on aerial vegetative organs of Asteraceae species, the information about secretory structures on thickened subterranean organs is sparse. The aim of this study was to investigate the occurrence of secretory structures on thickened and nonthickened subterranean organs of seven Asteraceae species from three tribes: Eupatorieae (Chromolaena squalida and Gyptis lanigera), Vernonieae (Chresta sphaerocephala, Lessingianthus bardanoides, L. glabratus and Orthopappus angustifolius), and Plucheeae (Pterocaulon angustifolium). The specimens were collected in areas of cerrado from the State of São Paulo, Brazil. All species of the tribe Vernonieae studied exhibited endodermic cells, other than the epithelial cells of the canal, with secretory activity in the roots. In C. sphaerocephala roots, two types of endodermic cell were found, but only one had secretory activity. Secretory canals were found in the tuberous and nontuberous roots of all studied species. These data agree with the results from the literature for Asteraceae species. Here, we describe for the first time in Asteraceae the presence of secretory idioblasts in C. sphaerocephala. Secretory trichomes are present in the Orthopappus angustifolius rhizophore. Histochemical tests have shown that all types of secretory structure possess substances containing lipids. © 2008 The Linnean Society of London, Botanical Journal of the Linnean Society, 2008, 157 , 789–796.     

CRYPTOCHROME2 in vascular bundles regulates flowering in Arabidopsis

Plants make full use of light signals to determine the timing of flowering. In Arabidopsis thaliana, a blue/UV-A photoreceptor, CRYPTOCHROME 2 (cry2), and a red/far-red photoreceptor, PHYTOCHROME B (phyB), are two major photoreceptors that control flowering. The light stimuli for the regulation of flowering are perceived by leaves. We have recently shown that phyB expression in mesophyll but not in vascular bundles suppresses the expression of a key flowering regulator, FLOWERING LOCUS T (FT), in vascular bundles. In this study, we asked where in the leaf cry2 perceives light stimuli to regulate flowering. To answer this question, we established transgenic Arabidopsis lines in which the cry2-green fluorescent protein (GFP) fusion was expressed under the control of organ/tissue-specific promoters in a cry2-deficient mutant background. Analysis of these lines revealed that expression of cry2-GFP in vascular bundles, but not in epidermis or mesophyll, rescued the late flowering phenotype. We further confirmed that cry2-GFP expressed in vascular bundles increased FT expression only in vascular bundles. Hence, in striking contrast with phyB, cry2 most likely regulates FT expression in a cell-autonomous manner.     

A comprehensive generic-level phylogeny of the sunflower family: Implications for the systematics of Chinese Asteraceae

The sunflower family (Asteraceae) is the largest and the most diverse flowering plant family, comprising 24 000–30 000 species and 1600–1700 genera. In China, Asteraceae are also the largest family, with approximately 2336 indigenous species in 248 genera. In the past two decades, molecular phylogenetic analyses has contributed greatly to our understanding of the systematics of Asteraceae. Nevertheless, the large-scale analyses and knowledge about the relationships of Chinese Asteraceae at the generic level as a whole are far from complete due to difficulties in sampling. In this study, we presented a three-marker (rbcL, ndhF, and matK) phylogeny of Asteraceae, including 506 genera (i.e., approximately one-third of Asteraceae genera). The study sampled 200 Chinese genera (i.e., approximately 80% of Chinese Asteraceae genera). The backbones of the new phylogeny were largely congruent with earlier studies, with 13 subfamilies and 45 tribes recognized. Chinese Asteraceae were distributed in 7 subfamilies (Mutisioideae, Wunderlichioideae, Carduoideae, Pertyoideae, Gymnarrhenoideae, Cichorioideae, and Asteroideae) and 22 tribes (Mutiseae, Hyalideae, Cardueae, Pertyeae, Gymnarrheneae, Vernonieae, Cichorieae, Doroniceae, Senecioneae, Astereae, Anthemideae, Gnaphalieae, Calenduleae, Inuleae, Athroismeae, Helenieae, Coreopsideae, Neurolaeneae, Tageteae, Millieae, Eupatorieae, and Heliantheae). Chinese Asteraceae lacked 6 basal subfamilies and 23 tribes. Several previously ambiguous relationships were clarified. Our analyses also resolved some unplaced genera within Chinese Asteraceae. Finally, our phylogenetic tree was used to revise the classification for all genera of Chinese Asteraceae. In total, 255 genera, 22 tribes, and 7 subfamilies in China are recognized.     

SECRETORY RESERVOIRS (DUCTS) OF TWO KINDS IN GIANT RAGWEED (AMBROSIA TRIFIDA; ASTERACEAE)

Two types of tubular secretory reservoirs occur in Ambrosia trifida, the first such example known in plants. Paraffin and resin sections, and clearings showed that, although each type consists of many separate unbranched tubes, they differ in anatomy, secretory contents, distribution, and length. Reservoirs (PAR) containing a red substance (presumably a polyacetylene) and lined with a biseriate epithelium parallel the largest leaf and stem vascular bundles. One PAR arises near the base of each leaf lobe midrib and extends through the petiole to the node or continues in the stem cortex to the node below. Other PARs start at the cotyledonary node or in cotyledons and extend down into the primary root, where they have only a single layer of unspecialized epithelium. PARs realign themselves, and more form de novo, until the primary root has two to four separate arrays of PARs abutting the endodermis, each with three to six parallel PARs. Branch roots have similar PAR arrays but unconnected to PARs of the parent root. Inflorescence PARs occur only in bracts, and in petals of male flowers. The second type of reservoir (OR) has a uniseriate epithelium and contains an unidentified oil. ORs occur in phloem, and in pith next to xylem, of stem and large leaf bundles. They dwindle in successively smaller veins until the two smallest orders lack them. ORs occur only in phloem in the hypocotyl; none occur in cotyledons, roots, or floral parts.     

买麻藤根的异常次生生长

买麻藤(Cnetum montanum)根的异常次生生长与茎的异常次生生长相似,位于维管束外围的薄壁组织细胞可以形成维管束,以这种方式使根加粗。并且在生长过程中以同样的方式,在维管束的外围不断形成新的维管束。这些新的维管束成环状排列,因此,在老根中呈多圈的维管束。与茎唯一不同的是根的异常次生生长为不均等的,在两个宽大的射线区外侧,没有异常的维管束形成,因此,根主要向着与两条宽大射线相垂直的方向扩展,故外形呈扁圆形。     

Flowering regulation by tissue specific functions of photoreceptors

Flowering is one of the most important steps in a plant life cycle. Plants utilize light as an informational source to determine the timing of flowering. In Arabidopsis, phytochrome A (phyA), phyB and cryptochrome2 (cry2) are major photoreceptors that regulate flowering. These photoreceptors perceive light stimuli by leaves for the regulation of flowering. A leaf is an organ consisting of different tissues such as epidermis, mesophyll and vascular bundles. In the present study, we examined in which tissue the light signals are perceived and how those signals are integrated within a leaf to regulate flowering. For this purpose, we established transgenic Arabidopsis lines that expressed a phyB-green fluorescent protein (GFP) fusion protein or a cry2-GFP fusion protein in organ/tissue-specific manners. Consequently, phyB was shown to perceive light stimuli in mesophyll. By contrast, cry2 functioned only in vascular bundles. We further confirmed that both phyB-GFP and cry2-GFP regulated flowering by altering the expression of a key flowering gene, FT, in vascular bundles. In summary, perception sites for different spectra of light are spatially separated within a leaf and the signals are integrated through the inter-tissue communication.Key words: photoreceptor, light, flowering, phytochrome, cryptochrome, inter-tissue signalThe timing of flowering is strictly regulated by environmental conditions such as light. Two aspects of light, spectral nature and photoperiod, dramatically affect flowering. In Arabidopsis, phyB and phyA/cry2 are the major photoreceptors mediating these responses. Although photoreceptors are expressed in almost all organs,¹ partial irradiation and grafting analyses have demonstrated that plants perceive light signals only in leaves.^2–4 However, roles for different tissues in a leaf remained unknown due to a lack of a proper method. To answer the question, we established Arabidopsis transgenic lines that expressed phyB-GFP or cry2-GFP on the respective mutant backgrounds. The resultant transgenic lines were examined for their flowering phenotype. Consequently, we found that phyB-GFP in mesophyll but not in other tissues regulated flowering.⁵ By contrast, cry2-GFP functioned only in vascular bundles.⁶A strong genetic interaction between phyB and cry2 in the regulation of flowering is known.^7,8 Cry2 regulates the flowering by suppressing the inhibitory effect of phyB on flowering. Hence, cry2 function is observed only in the presence of phyB. Conversely, the effect of phyB is exaggerated in the cry2 mutant, because phyB is not counteracted by cry2 in its absence. Here, we tested how phyB and cry2 in different tissues regulated flowering in the absence of the other photoreceptor. For this purpose, we took a physiological approach. Phenotype of the phyB-GFP lines was examined under monochromatic red light, in which phyB but not cyr2 is activated. As expected, phyB-GFP in mesophyll but not in vascular bundles strongly affected the flowering in this condition (Fig. 1A). We also tested the cry2-GFP function when phyB was not activated. Namely, plants were placed under blue light supplemented with strong far-red light. As expected, cry2-GFP failed to affect the flowering even under this condition regardless of where it was expressed (Fig. 1B).Open in a separate windowFigure 1FT expression under phyB or cry2 inactive conditions. Total RNA was extracted from the seedlings grown under long-day condition for 10 days and subjected to qRT-PCR for FT expression analysis. Data were normalized to the level of FT mRNA in (A) of the wild type, which was set to 1 arbitrary unit (a.u.). Mean ± SE (n = 4). WT, wild type. (A) Long-day red light, (16L 8D; 10 µmol m^-2 s^-1). WT, wild type; phyB, phyB mutant; Bpro, PHYB promoter-PHYB-GFP; PBT56, phyB-GFP in mesophyll; PBT239, phyB-GFP in vascular bundles.⁵ (B) Long-day blue and far-red light (16L 8D; blue light, 3 µmol m^-2 s^-1; far-red light, 10 µmol m^-2 s^-1). WT, wild type; cry2, cry2 mutant; pCRY-C2G, CRY2 promoter-CRY2-GFP; pCAB-C2G, CAB3 promoter-CRY2-GFP; pSUC-C2G, SUC2 promoter-CRY2-GFP.⁶Photoreceptors regulate flowering by altering the expression of a key flowering regulator, FT.^9,10 Interestingly, the FT gene is expressed specifically in vascular bundles.¹¹ Indeed, mesophyll phyB-GFP controlled the expression of FT in vascular bundles. Hence, there must be a mechanism by which the light signal is transduced from mesophyll to vascular bundles to regulate the FT expression in vascular bundles. It should be noted here that FT is not the sole factor involved in the light regulation of flowering. Factors such as CO, SPA, COP1 and PFT1 are known to link the photoreceptors and FT.^12–14 These factors most likely function in leaves. However, their function sites at the tissue level remain totally unknown except for CO. The biological clock is another class of machinery that is tightly related to the light signal transduction pathway.¹⁵ Unfortunately, function sites of the clock components for the regulation of flowering remain unclear. The future work should reveal those sites. Such analyses should finally provide a complete picture illustrating a network of the inter-tissue signaling for the regulation of flowering.The present work urges us to indentify the molecule that mediates the inter-tissue signaling between mesophyll and vascular bundles. Potential candidates include phytohormones, microRNA¹⁶ and peptides.¹⁷ Among phytohormones, gibberellin promotes flowering.¹⁸ However, gibberellin is probably not the answer because gibberellin does not alter the FT expression directly. Except gibberellin, no exogenously added phythromone dramatically affects flowering in Arabidopsis. It is known that microRNA such as miR172, miR159 and miR156 are involved in the regulation of flowering time.¹⁹ However, those microRNA''s neither regulate the FT expression nor are regulated by light. Since most of microRNA''s has not been intensively studied yet, it remains possible that one of them may mediate the above inter-tissue signal. Another potential candidate is a peptide. Although not much is known about peptide hormones in plants yet, peptides such as PSK,²⁰ xylogen²¹ and CLE²² have been shown to regulate cell growth and differentiation. Although none of peptides is known to regulate flowering in plants at present, a future work may reveal a novel peptide that mediates the inter-tissue signals for flowering.     

Morphogenesis of galls induced by Baccharopelma dracunculifoliae (Hemiptera: Psyllidae) on Baccharis dracunculifolia (Asteraceae) leaves.

The commonest insect gall on Baccharis dracunculifolia (Asteraceae) leaves is induced by Baccharopelma dracunculifoliae (Hemiptera, Psyllidae). The gall-inducing insect attacks young leaves in both the unfolded and the fully expanded stages. Four developmental phases were observed in this type of gall: 1) A folding phase, during which the leaf lamina folded upward alongside the midrib and the edges of the upper portion of the leaf approached each other, forming a longitudinal slit. A single chamber was formed on the adaxial surface of the leaf; 2) A swelling phase, in which the folded leaf tissues thickened and the edges of the leaf drew closer together, narrowing the slit. In this phase the gall matured, turning succulent, fusiform and pale green. The single nymphal chamber was lined with white wax and was able to house from one to several nymphs; 3) A dehiscence phase, characterized by the opening of the slit to release inducers; and 4) A senescence phase, when the gall turned dark and dry. The dermal system of the mature gall was composed of a single-layered epidermis. The mesophyll was swollen, and the swelling was due mainly to hyperplasia of the parenchyma. The vascular tissues along the midrib vein were conspicuous and the perivascular fibers resembled parenchymal cells. The hypertrophied secretory cavities contained low lipophylic content. This gall does not form nutritive tissue, but salivary sheaths left by the inducers were observed near the parenchyma, vascular bundles and secretory cavities. This study complements our current knowledge of gall biology and sheds further light on the plasticity of plant tissues stimulated by biotic factors.     

DEVELOPMENTAL CHANGES IN CONTENT OF FOLIAR SECRETORY CAVITIES OF TAGETES ERECTA (ASTERACEAE)

The quantitative and qualitative changes in the contents of foliar secretory cavities during development of Tagetes erecta CV. Moonshot plants were determined. Separation of the secretory components by HPLC yielded three major compounds, subsequently identified by mass spectroscopy, UV spectra, and cochromatography as indole, piperitenone, and piperitone. Comparison of extracts from isolated cavities vs. lamina without cavities showed that in all cases the components were absent from lamina tissues. The quantities of indole and piperitone, in general, increased as the plants developed up to the stage of early flowering, when there was a reduction in total content. At late flowering, the amounts of these components, once again, increased. Concomitantly, the amount of piperitenone decreased during plant development. At all ages studied, indole comprised at least 99% of the total secretion product. This is the first report of the secretory components being restricted to the cavities.     

Phytochrome B in the mesophyll delays flowering by suppressing FLOWERING LOCUS T expression in Arabidopsis vascular bundles

Light is one of the most important environmental factors that determine the timing of a plant's transition from the vegetative to reproductive, or flowering, phase. Not only daylength but also the spectrum of light greatly affect flowering. The shade of nearby vegetation reduces the ratio of red to far-red light and can trigger shade avoidance responses, including stem elongation and the acceleration of flowering. Phytochrome B (phyB) acts as a photoreceptor for this response. Physiological studies have suggested that leaves can perceive and respond to shade. However, little is known about the mechanisms involved in the processing of light signals within leaves. In this study, we used an enhancer-trap system to establish Arabidopsis thaliana transgenic lines that express phyB-green fluorescent protein (GFP) fusion protein in tissue-specific manners. The analysis of these lines demonstrated that phyB-GFP in mesophyll cells affected flowering, whereas phyB-GFP in vascular bundles did not. Furthermore, mesophyll phyB-GFP suppressed the expression of a key flowering regulator, FLOWERING LOCUS T, in the vascular bundles of cotyledons. Hence, a novel intertissue signaling from mesophyll to vascular bundles is revealed as a critical step for the regulation of flowering by phyB.     

Thiophene synthesis and distribution in young developing plants of Tagetes patula and Tagetes erecta

Thiophene synthesis and accumulation were investigated in organsof Tagetes patula and T. erecta. Thiophene accumulation startedrapidly in germinating seedlings of both species. Roots andhypocotyls were the major thiophene accumulating organs and5-(3-buten-1-ynyl)-2, 2-bithienyl (BBT) and 5-(4-acetoxy-1-butynyl)-2,2 -bithienyl (BBTOAc) were the major accumulated compounds.Higher thiophene concentrations were reached in Tagetes patulathan in T. erecta. Accumulation patterns for individual thiopheneswere different within organs, between organs and between bothspecies. Within hypocotyls of Tagetes patula, thiophene concentrationswere high in the epidermis and the vascular tissue and low inthe parenchymatic tissues of cortex and pith. Synthesis of thiopheneswas high in the roots and hypocotyls and very low in the leaves.Transport of thiophenes from the roots into the shoot occurred,but the rate of transport was too low to explain the high concentrationsin the hypocotyl. It is concluded that for the main part thiophenesare accumulated where they are synthesized. Key words: Tagetes, hiophenest, synthesis, accumulation, secondary metabolites     

FLORAL DEVELOPMENT AND VASCULATURE IN HYDROCLEIS NYMPHOIDES (BUTOMACEAE)

The flower of Hydrocleis nymphoides consists of three sepals which arise in spiral succession, three simultaneously arising petals, numerous stamens and staminodia which arise in centrifugal order, and six carpels. A residual apex remains at maturity. The first-formed members of the androecium are stamens and the later-formed members are staminodia which develop below the stamens and which become outwardly displaced during expansion of the receptacle. The androecium is supplied by branching vascular trunk bundles. The carpels are completely open but the ventral margins are slightly conduplicately appressed basally. A single dorsal bundle provides the stigmatic area with vascular tissue, and a network of small placental bundles supplies the numerous laminar ovules. There are no clearly defined ventral bundles. It is suggested that Hydrocleis nymphoides is neither the most primitive nor the most advanced member of the family. A pattern of phylogenetic reduction in the androecium and receptacle is suggested for the entire family.     

The role of phytohormones in tumor formation in radish

Tumor formation was studied in inbred radish lines that produce tumors on plant roots during flowering. In all radish lines under consideration, the sequences homologous to oncogenes tmr/tml of Agrobacterium tumefaciens were revealed by Southern hybridization. No sequences homologous to the tms locus of A. tumefaciens and the oncogenes of A. rhizogenes were determined. It was found that auxin sensitivity and the tumor-producing capacity were coinherited. We suggest that tumor phenotype arise as a result of a combination between agrobacterial "cytokinin" oncogenes and certain alleles of "auxin" radish genes.     

Foliar oil reservoir anatomy and distribution in Solidago canadensis (Asteraceae, tribe Astereae)

In leaves of goldenrod, Solidago canadensis (Asteraceae, tribe Astereae), numerous internal oil reservoirs with a uniseriate epithelium occur as a single file above or below veins or as isolated cavities in the mesophyll. Reservoirs are abaxial to major veins (vein orders 1–3), either above, below, or superimposed in intermediate 4th order veins, but strictly adaxial to 5th and 6th order minor veins. Reservoirs are initiated as discrete cavities, but those below 1st and 2nd order veins are in a single crowded file, each separated only by epithelial cells. Elongation of these cavities, accompanied by stretching and separation of septa, gives a false impression at maturity of an indefinitely long duct instead of a series of tubular cavities. Reservoirs of vein orders 3–6 are mostly more widely separated and less subject to elongation, thus they are shorter and remain discrete at maturity. The overall foliar pattern is one of successively shorter reservoirs, a sequence that is in concert with the successively narrower and progressively less elongated vein orders. The shift from abaxial to adaxial reservoirs in minor veins may be related to different phloem functions: sugar transport in major veins and photosynthate assimilation in minor veins.     

Specialist bees collect Asteraceae pollen by distinctive abdominal drumming (<Emphasis Type="Italic">Osmia</Emphasis>) or tapping (<Emphasis Type="Italic">Melissodes</Emphasis>, <Emphasis Type="Italic">Svastra</Emphasis>)

Four species of western US Osmia (3 Cephalosmia) that are Asteraceae specialists (mesoleges) were observed using a stereotypical means of collecting pollen—abdominal drumming—to gather pollen from 21 flowering species representing nine tribes of Asteraceae. Abdominal drumming is a rapid dorso-ventral motion of the female’s abdomen (467 pats/min) used to directly collect and place pollen in the bee’s ventral scopa. A co-occurring generalist, O. lignaria, never drummed Asteraceae flowers for pollen, but instead used its legs to harvest pollen. Observed drumming by several other osmiines is noted. A different pollen-harvesting behavior, abdominal tapping, is described for two eucerine bees (Melissodes agilis and Svastra obliqua), both oligolectic for the Asteraceae. The behavior also involves a dorso-ventral motion, but they tap their distal abdominal venter against disk flowers at a slower tempo (304 taps/min). These females’ distal sternites have distinctly dense and long hair brushes for acquiring pollen by this behavior. Brief accounts of similar abdominal pollen gathering behaviors by other megachilids are summarized.     

Investigation of P and S Distributions in the Roots of Tagetes patula L. using Micro-PIXE

A proton microprobe for energy-dispersive PIXE-analysis hasbeen used to measure elemental distributions of sulphur andother elements in roots of Tagetes patula L. by making a line-scanalong the diameter of the cross-section. Higher concentrationsof phosphorus and sulphur were found in or near the phloem.In addition the endodermis contained an increased sulphur concentration.The results obtained and future possibilities for this kindof investigation are discussed. Key words: Tagetes patula L., micro-PIXE, sulphur, thiophenes, endodermis, Pratylenchus penctrans (Cobb)     

Systematic and comparative anatomy of Cymbidieae (Orchidaceae)

Cymbideae comprise an assemblage of 28 genera nearly all of which are represented in this study. Their anatomy is relatively homogenous with the exception of Govenia , in which roots lack velamen and pseudobulb vascular bundles lack sclerenchyma, conditions that do not obtain in other genera. Marginal fibre bundles in leaves of Grammatophyllum and Porphyroglottis consist of clusters of thicker-walled, narrower, epidermis-facing fibres as well as thinner-walled, wider, mesophyll-facing fibres. This feature also occurs in some species of Maxillaria . Baculate tilosomes appear in the roots of a majority of genera in Cymbidieae, as they do in species of Maxillaria , confirming DNA analyses showing a close relationship between tribes Cymbidieae and Maxillarieae. Govenia is singled out both on anatomical and molecular grounds as being ill-placed in Cymbidieae. Cladistic analysis produces only a few tentative hypotheses of phylogenetic relationships among the 28 genera, showing that anatomical characters are of limited value in assessing affinities within this tribe. © 2002 The Linnean Society of London, Botanical Journal of the Linnean Society , 2002, 139 , 1–27.