Formation of Specialized Propagules Resistant to Desiccation and Cryopreservation in the Threatened Moss Ditrichum plumbicola (Ditrichales, Bryopsida)

doi:10.1093/aob/mcm141

AOBPreview originally published online on July 30, 2007
Annals of Botany 2007 100(3):483-496; doi:10.1093/aob/mcm141

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Formation of Specialized Propagules Resistant to Desiccation and Cryopreservation in the Threatened Moss Ditrichum plumbicola (Ditrichales, Bryopsida)

J. K. Rowntree¹^,3^,*, J. G. Duckett², C. L. Mortimer¹^,4, M. M. Ramsay¹ and S. Pressel²

¹ Micropropagation Unit, Royal Botanic Gardens Kew, Richmond, Surrey TW9 3AB, UK
² School of Biological and Chemical Sciences, Queen Mary University of London, Mile End Road, London E1 4NS, UK
³ Faculty of Life Sciences, University of Manchester, Stopford Building, Oxford Road, Manchester M13 9PT, UK
⁴ Department of Biology and Biochemistry, University of Bath, Bath BA2 7AY, UK

^* For correspondence. E-mail jkrowntree{at}mac.com

Received: 24 January 2007 Returned for revision: 19 March 2007 Accepted: 25 May 2007 Published electronically: 30 July 2007

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

Background and Aims: Successful cryopreservation of bryophytes is linked to intrinsicdesiccation tolerance and survival can be enhanced by pre-treatmentwith abscisic acid (ABA) and sucrose. The pioneer moss Ditrichumplumbicola is naturally subjected to desiccation in the fieldbut showed unexpectedly low survival of cryopreservation, aswell as a poor response to pre-treatment. The effects of thecryopreservation protocol on protonemata of D. plumbicola wereinvestigated in order to explore possible relationships betweenthe production in vitro of cryopreservation-tolerant asexualpropagules and the reproductive biology of D. plumbicola innature.

Methods: Protonemata were prepared for cryopreservation using a four-stepprotocol involving encapsulation in sodium alginate, pre-treatmentfor 2 weeks with ABA and sucrose, desiccation for 6 h and rapidfreezing in liquid nitrogen. After each stage, protonemata wereprepared for light and electron microscopy and growth on standardmedium was monitored. Further samples were prepared for lightand electron microscopy at intervals over a 24-h period followingremoval from liquid nitrogen and re-hydration.

Key Results: Pre-treatment with ABA and sucrose caused dramatic changes tothe protonemata. Growth was arrested and propagules inducedwith pronounced morphological and cytological changes. Mostcells died, but those that survived were characterized by thick,deeply pigmented walls, numerous small vacuoles and lipid dropletsin their cytoplasm. Desiccation and cryopreservation elicitedno dramatic cytological changes. Cells returned to their pre-dehydrationand cryopreservation state within 2 h of re-hydration and/orremoval from liquid nitrogen. Regeneration was normal once theABA/sucrose stimulus was removed.

Conclusions: The ABA/sucrose pre-treatment induced the formation of highlydesiccation- and cryopreservation-tolerant propagules from theprotonemata of D. plumbicola. This parallels behaviour in thewild, where highly desiccation-tolerant rhizoids function asperennating organs allowing the moss to endure extreme environmentalconditions. An involvement of endogenous ABA in the desiccationtolerance of D. plumbicola is suggested.

Key words: ABA, asexual propagules, cell-biology, cryopreservation, desiccation tolerance, Ditrichum plumbicola, extremophiles, protonemata, sucrose

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

The production of asexual propagules in bryophytes, in particularmosses, is well documented (Whitehouse, 1973, 1980; Side and Whitehouse, 1987;Duckett and Ligrone, 1992; Goode et al., 1993a, b, 1994). Propagulesinclude gemmae, tubers or brood cells and are continually beingdescribed from both tissue cultures and natural populations.Their suggested function is as perennating organs, producedas survival mechanisms in unfavourable circumstances (Duckett and Pressel, 2003;Preston, 2004; Pressel et al., 2005). Previous studies, particularlyon the formation of brood cells, indicate that abscissic acid(ABA) and/or desiccation are stimuli for formation (Goode et al., 1993a).

Specialized propagules with the ability to survive prolongedperiods without water add an extra dimension to the knowledgeof desiccation tolerance in mosses (for an overview, see Oliver et al., 2000a,b; Proctor, 2001). In common with other plant tissues, somemosses when suitably dried, are able to tolerate extreme temperaturestress (Bequerel, 1951; Bewley, 1973; Glime and Carr, 1974;Norr, 1974; Hearnshaw and Proctor, 1982). This is exploitedin cryopreservation protocols for the storage of plant tissues,where material is often first dried before being immersed inliquid nitrogen (LN) at – 196 °C. Indeed there isevidence that post-cryopreservation survival in mosses dependson intrinsic desiccation tolerance (Burch, 2003) and that thiscan be enhanced by pre-treatment with ABA and sucrose (Pence, 1998;Burch and Wilkinson, 2002).

The use of cryopreservation techniques is advocated for thelong-term storage of plant material when conventional methods,such as seed banking, are inappropriate (Benson, 1999). Suchtools are increasingly being used for the ex situ conservationof threatened species (Guerrant et al., 2004). Between 2000and 2006, the Royal Botanic Gardens, Kew supported a projectfor the ex situ conservation of threatened bryophytes in theUK. One aim of the project was to provide a cryopreserved collectionof gametophytic material, to store taxa from which spores werenot necessarily available (Ramsay and Burch, 2001), and methodswere developed accordingly (Burch and Wilkinson, 2002; Burch, 2003).

One of the target species of the project was Ditrichum plumbicola,a moss classified as near threatened on the British red list(Church et al., 2001), the distribution of which in the BritishIsles is restricted to lead mine spoil (Porley and Hodgetts, 2005).Gametangia and sporophytes are unknown for this species, butrhizoidal tubers have been described (Arts, 1994). Ditrichumplumbicola grows exclusively on bare soil subjected to desiccationin the summer and surface cryoturbation after winter frosts.It was therefore reasonable to assume that the moss was bothdesiccation and freezing tolerant. Preliminary cryopreservationtrials on the protonemata, however, showed that this moss respondedto the protocol differently from any other desiccation-tolerantspecies tested (Burch, 2003; J. K. Rowntree, unpubl. res.).In particular, exposure to ABA and sucrose elicited profoundchanges in protonemal morphology, producing cells which initiallyfailed to regenerate following cryopreservation.

Thus, the aims of this study were firstly to determine if ABAor sucrose, or a combination of the two, induced the morphologicalchanges observed in D. plubicola; and whether any other stagesof the protocol played a part in this process. In a wider context,the objectives were (a) to characterize the cytology of thesecells and compare them with brood cells; (b) to report on thecytological changes elicited in these cells by desiccation andcryopreservation; (c) to explore possible relationships betweenthe production in vitro of asexual propagules that survive cryopreservationand the reproductive biology of D. plumbicola in nature.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

Plant material
Gametophytic material of Ditrichum plumbicola Crundw. was collectedfrom a single lead mine spoil site in County Durham for initiationinto tissue culture. Wild protonemata were collected for comparisonfrom the same site and also from two further lead mine spoilsites in North and mid-Wales. The latter were kept in herbariumpackets and observed over a 1-year period from the time of collection.As the species is designated under the UK Biodiversity ActionPlan initiative, collection was only undertaken with permissionof the lead partner (see http://www.ukbap.org.uk/ for more information)and specific site details are undisclosed.

Culture conditions
Protonematal cultures were prepared from surface-sterilizedgametophore fragments. Stock cultures were maintained on sucrose-freequarter strength Murashige and Skoog medium (1/4 MS) with micro-and macro-elements including vitamins (Duchefa Biochemie B.V.,Haarlem, The Netherlands) at pH 5·8, solidified with4·0 g L^–1 Gelrite^TM (standard medium) in Petridishes sealed with Micropore^TM tape to allow for gas exchange.They were maintained in a growth room with a 16 h light/8 hdark regime, under a 1 : 1 mixture of NARVA 58W/077 and GE58W/29fluorescent tubes (15–50 µmol m^–2 s^–1PAR) at 20·5 °C (±3·5).

Cryopreservation experiment
Protonematal material was prepared for cryopreservation in LNaccording to the methods developed by Burch and Wilkinson (2002)and Burch (2003). The protocol was a four-stage process: (1)encapsulation in 3 % sodium alginate, solidified with 100 mMCaCl solution, (2) pre-treatment for 2 weeks with 10 µMABA and 50 g L^–1 sucrose, (3) dried for 6 h followed by(4) rapid immersion and storage in LN.

Ten protonematal plugs (approx. 1 mm diameter) were removedfrom the stock cultures, transferred onto standard medium andtheir growth monitored weekly for a total of 5 weeks by measuringplug diameter along two permanent transects marked on the baseof the dishes with vernier callipers according to Rowntree et al. (2005)(control treatment). Forty protonematal plugs were each encapsulatedin an alginate strip (for methods, see Burch and Wilkinson, 2002).The strips were then placed singly in Petri dishes containingstandard medium and maintained in the growth room for 1 weekto allow for recovery from possible damage incurred during theirpreparation. Protonematal growth from ten strips was monitoredweekly for a total of 5 weeks (encapsulation treatment). Theremaining 30 strips were transferred to Petri dishes containingstandard medium supplemented with 50 g L^–1 sucrose and10 µM ABA. Sucrose was added to the medium prior to autoclavingand ABA was added post-autoclaving from a stock solution (50mM in 96 % ethanol) to cooled, but still liquid, medium. After2 weeks, ten strips were transferred back onto standard mediumand their growth monitored for 5 weeks (ABA/sucrose treatment).The remaining 20 strips were placed in clean, open Petri dishesin a laminar flow hood, under a sterile air flow (0·45m s^–1) for 6 h to dry. Final water content was approx.0·1 g H₂O g^–1 d. wt. Ten of these strips were transferredback onto standard medium and growth was monitored for 5 weeks(dehydration treatment), while the remaining ten strips wereplaced into 2·0-mL cryovials (Nalgene, Rochester, NY,USA) and sealed. The vials were frozen by rapid immersion inLN and stored at –196 °C for 1 week. Vials were thenremoved from the LN, immersed in a water bath at 40 °C for2 min and dried. Strips were removed from the vials in a laminarflow hood, placed onto standard medium and growth was monitoredfor 5 weeks (cryopreservation treatment).

After 5 weeks, five replicates were randomly selected from eachof the treatments. Protonemal material was removed from insidethe alginate strips, transferred onto plates of standard mediumand growth was monitored. Additional strips were prepared fromeach treatment for examination via light and electron microscopy.Cryopreserved material remained frozen in LN until processingand was transported in a dry shipper (IC-4VS, Wessington CryogenicsLtd, Houghton-le-Spring, Tyne and Wear, UK) between facilities.

ABA/sucrose experiment

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

Standard medium was prepared without additional sucrose as aboveor with 50 g L^–1 sucrose added. ABA (10 µM) wasthen added to half of the medium, giving a total of four treatments.Plugs of D. plumbicola protonemata (approx. 2 mm diameter) wereremoved from the stock cultures and transferred onto 5-cm-diameter,shallow Petri dishes (15 mL) containing one of the four media.Fifteen replicates were used per treatment, and there were atotal of 60 plates for the whole experiment. Mean diameter growthwas measured for 5 weeks as above and any structural and colourchanges in the protonemata were monitored. After 5 weeks, fivereplicates were again randomly selected from each treatmentand small protonemal plugs were transferred onto plates of standardmedium. Growth was monitored for a further 5 weeks as above.Protonemata representative of each treatment after 2 weeks growthwere prepared for light microscopy.

Light microscopy
Control, encapsulated and ABA/sucrose-treated specimens weremounted in water and photographed with a digital camera undera Leica DM RXAZ microscope using interference contrast optics.Dehydrated and cryopreserved specimens were mounted in immersionoil to prevent re-hydration, and photographed as above.

Electron microscopy
Protonemata were fixed and embedded for electron microscopyfollowing the methods of Duckett and Ligrone (1992). Cryopreservedprotonemata were either placed immediately in fixative uponremoval from LN or allowed to regenerate for 0·5, 1,2, 4, 12 and 24 h on standard medium. Protonemata were fixedin a mixture of 3 % (v/v) glutaraldehyde, 1 % (v/v) formaldehyde(freshly prepared from paraformaldehyde) and 0·5 % tannicacid (w/v) in 0·05 M Na-cacodylate buffer at pH 6·9for 4 h at room temperature. Material was rinsed in 0·1M Na-cacodylate buffer and post-fixed with 1 % (w/v) osmiumtetroxide in 0·1 M Na-cacodylate buffer overnight at4 °C. It was then dehydrated in ethanol and embedded inSpurr's resin via propylene oxide. Thin sections, cut with adiamond knife and sequentially stained with 5 % (v/v) methanolicuranyl acetate for 15 min and lead citrate for 10 min, wereexamined under a Jeol 1200 EX2 electron microscope. Specimensfor scanning electron microscopy were dehydrated in ethanol,critical point dried and observed in a Hitachi S570 scanningelectron microscope operating at 20 kV.

Sections (0·5 µm thick) stained with 1 % toluidineblue were photographed with a Leica DM RXA2 microscope equippedwith differential interference contrast optics.

Data analysis
Data from week 5 of the cryopreservation experiment were analysedwith a fixed effects (Model I) one-way ANOVA and Bonferronipost hoc tests, with the five treatments as independent categoricalvariables. Data from week 5 and then week 2 of the ABA/sucroseexperiment were analysed with separate fixed effects (ModelI) two-way ANOVAs, with sucrose and ABA as independent categoricalvariables. A Bonferroni correction factor for multiple testswas used where ${alpha}$ _adj = ( ${alpha}$ /k) and k was the number of tests (Sokal and Rohlf, 1995,239–240). One replicate from the control treatment didnot survive the original transfer; no growth was observed forthe duration of the experiment and protonemata were colourless.This was removed from the statistical analysis giving a totaln = 59. Normality was tested using a method for small samplesizes according to Sokal and Rolf (1995). Heteroskedasticitywas not directly tested for, as Zar (1999, 185) and Scheffe (1959)indicate the robustness of ANOVAs from deviations in homoskedasticityif sample sizes are equal or nearly equal. Statistical analyseswere performed using Systat 10 software (Systat Software, 2004)

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

Controls
Growth of D. plumbicola in culture was observed mainly as asteady expansion of the protonematal plug in two dimensionsacross the surface of the medium, although three-dimensionalgrowth was also observed (Figs 1 and 2A). The protonemalsystem produced was typical (Fig. 2A), with well-differentiatedchloronema (Fig. 3A) and caulonema filaments with longitudinallyaligned, starch-filled chloroplasts (Fig. 3B). Rhizoidalfilaments with deeply pigmented walls and minute plastids werealso produced, but only after a prolonged period (>5 weeks)of culture (Fig. 3C). An aerial system of tightly packedchloronema filaments arising vertically from the prostrate systemgave a characteristic ‘bushy’ appearance to thecultures (Fig. 2A).

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FIG. 1. Growth data (mean diameter in mm) at week 5 for control (1), encapsulation (2), ABA/sucrose (3), desiccation (4) and cryopreservation (5) treatments of Ditrichum plumbicola. Error bars = s.e., n = 50. Encapsulation treatment shows significantly reduced growth compared with the control (P < 0·001). ABA/sucrose, desiccation and cryopreservation treatments show significantly reduced growth compared with both the control and encapsulation treatments (P < 0·001), but not each other.

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FIG. 2. Ditrichum plumbicola protonema after 5 weeks of treatment: (A) control, (B) encapsulation, (C) ABA/sucrose, (D) desiccation and (E) cryopreservation treatments.

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FIG. 3. Light micrographs of cultured protonemata of Ditrichum plumbicola – controls and encapsulated material. (A–D) Controls: (A) typical chloronema cell with ovoid peripheral chloroplasts; (B) typical caulonema cell with elongated, longitudinally aligned plastids; (C) typical rhizoid with thick brown-pigmented walls, minute elongated plastids and spindle-shaped nucleus (n); (D) dedifferentiation of aerial chloronemal cells into thin-walled brood cells after 2–3 weeks in culture. (E–H) Encapsulated material: (E, F) typical chloronema (E) and caulonema (F) cells indistinguishable from the controls; (G) thin-walled brood cells on chloronema filaments after 2–3 weeks in culture; (H) 1-µm section of chloronema cell – note the large central vacuole and the peripherally located plastids (p) and nucleus. Scale bars: D, E, G = 50 µm; A–C, F = 20 µm; H = 10 µm.

The control protonemata exhibited a marked tendency towardsbroodiness. In young cultures (2–3 weeks old), numerouschloronema cells, especially those of the aerial system, readilydedifferentiated into spherical, thin-walled brood cells (Fig. 3D).

Encapsulation
Post-encapsulation, initial growth was within the alginate stripsbut, after a few weeks, protonemata grew through the alginatematrix onto the standard medium (Fig. 2B). There was asignificant reduction in growth compared with the controls (week5: P < 0·001; Fig. 1). Encapsulation did notaffect the morphology (Figs 2B and 3E, F) and cytology(Fig. 3H) of protonemata and the cells showed the sametendency towards broodiness as the controls (Fig. 3G).

Combined ABA/sucrose treatment
Pre-treatment with a combination of sucrose and ABA elicitedpronounced changes in the protonemata. Growth was significantlyreduced compared with both the controls and encapsulated treatments(week 5: P < 0·001; Fig. 1) and appeared to havebeen arrested within the alginate strips (Fig. 2C). Themajority of the protonemal system died, including almost allthe main caulonemal axes (Fig. 4A, B). The parts that survivedconsisted of uniseriate rows of three to eight cells with thick,deeply pigmented walls and an apical cell ± subapicalcell with less dense cytoplasm and thinner, non-pigmented walls(Fig. 4C). Incomplete cross walls were often present towardsthe tip of the apical cells (Fig. 4D). Some chloronemalside branches and adjacent cells along the filaments also survived.These were characterized by a dense cytoplasm containing numerouslipid droplets and by thick, but not always pigmented, cellwalls (Fig. 4C, E).

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FIG. 4. Light micrographs of sucrose/ABA-treated protonemata: (A) the majority of the cells are dead; those that survive are characterized by heavily pigmented walls; (B) detail of dead cells showing complete disruption of cell contents; (C) heavily pigmented filament with dense cytoplasm and with non-pigmented apical cell (arrowed); (D) detail of non-pigmented apical cell – the arrow indicates incomplete cross wall; (E) lipid-laden chloronemal cells with non-pigmented thick walls; (F–H) encapsulated, sucrose/ABA-treated cells after 2 weeks from transfer to standard growth medium. The protonemal system remains virtually unchanged except for increased brood cell development (F) and detachment of the same (arrowed) from the parent filament (H). Scale bars: A, F = 200 µm; B, C = 100 µm; E, H = 50 µm; D, G = 20 µm.

The cells remained largely unchanged when the alginate stripscontaining them were transferred intact to standard growth medium(Fig. 4F–H), except for a pronounced dedifferentiationof chloronema side branches into brood cells, which often becamedetached from the parent filament (Fig. 4H).

Transmission electron microscopy confirmed observations fromlight microscopy. The majority of the cells that remained viablehad a highly heterogeneous, thick (>3 µm) cell wall,comprising a densely fibrillar central layer with multiple strataof varying density on each side (Fig. 5A). Prominent projectionsof the loosely fibrillar, innermost layer containing a densercentral core (Fig. 5B) were a frequent feature of mostcells along the filaments except for the apical cells. Theirwalls were relatively thin (>1 µm) and homogeneousand never developed inner projections (Fig. 5C). The presenceof incomplete cross walls in the apical cells was confirmed(Fig. 5C). The cytoplasm was packed with numerous smallvacuoles (ranging from 200 nm to a few micrometres in diameter)often containing small deposits of electron-opaque material(Fig. 5D, E). The apical cells usually contained fewervacuoles (Fig. 5C). The plastids were ovoid to discoidalwith numerous, large starch grains (Fig. 5A, D). The mitochondriawere rounded to elongate, with a dense stroma and saccate cristae(Fig. 5E). Nuclei were rounded with a prominent nucleolus(Fig. 5D).

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FIG. 5. Transmission electron micrographs of sucrose/ABA-treated protonemal cells before and after dehydration. (A–E) Fully hydrated cells: (A) cell with starch-filled plastid and with thick, multi-layered cell wall – note the numerous projections of the cell wall innermost layer; (B) detail of cell wall projection consisting of loosely fibrillar material; (C) incomplete cross wall (arrowed) in apical cell – note the thin, homogeneous cell wall (cw); (D) cell packed with small vacuoles – also note the centrally located round nucleus (n) and the starch-filled plastids; (E) cytoplasm containing mitochondria (m) with dense matrix and saccate cristae and vacuoles (v) with electron-opaque content. (F–H) Dehydrated cells: (F) ovoid plastids with small starch grains (arrowed) and with an intact, undulating thylakoid system; (G) nucleus (n) with conspicuous blocks of condensed chromatin surrounded by small vacuoles; (H) heterogeneous cell wall (cw) with irregular internal projections. Scale bars: D = 5 µm; A–C, E–G = 2 µm; H = 1 µm.

Separate ABA/sucrose treatments
ABA and sucrose applied singly caused changes similar to, butless pronounced than, the combined treatment, with the majorityof the cells remaining alive. Both treatments caused a significantreduction in growth compared with the controls (week 5: P <0·001; Fig. 6) and a significant interaction betweenABA and sucrose was detected (week 5: P < 0·001; Fig. 6).Analysis of data at week 2 did not change the effects or significancevalues determined but R-values were slightly reduced.

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FIG. 6. Mean diameter (mm) of Ditrichum plumbicola protonema grown for 5 weeks on control (open circles, continuous line), 5 % sucrose (open triangles, continuous line), 10 µM ABA (closed circles, dashed line) and 5 % sucrose/10 µM ABA (closed triangle, dashed line) media. Error bars are s.e., n = 59. Significance values from two-way ANOVA at week 5 are shown.

After 2 weeks on medium supplemented solely with 10 µMABA, most of the filaments had become thick-walled and deeplybrown-pigmented (Fig. 7A). The majority of chloronemalcells had dedifferentiated into spherical brood cells (Fig. 7B,C), while caulonemal cells were shorter, with denser contentsthan the controls and bore only very short side branches (Fig. 7D).

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FIG. 7. Light micrographs of ABA- and sucrose-treated protonemal cells. (A–D) Treatment for 2 weeks with 10 µM ABA: (A) most filaments are thick-walled and deeply pigmented; (B) dedifferentiation of chloronema filaments into spherical brood cells; (C) caulonema filament with thick pigmented walls – note the short cells with dense cytoplasm and the very short side branch. (E–H) Treatment for 2 weeks with 5 % sucrose: (E) general aspect showing thick-walled pigmented filaments as in (A) but no brood cells; (F) detail of thick-walled pigmented filament – note the thin-walled non-pigmented apical cells in the side branch; (G, H) caulonema cells with numerous small vacuoles (v) (G) and abundant lipid droplets (L) (H) in their cytoplasm. Scale bars: A, E = 200 µm; B, C, F = 50 µm; D, G, H = 20 µm.

The addition of 50 g L^–1 sucrose only to the medium elicitedsimilar changes to the appearance of protonemal cultures especiallywith regards to an increase in cell wall thickness and pigmentation(Fig. 7E). In contrast, the sucrose treatment affectedmainly the prostrate system, with filaments of the aerial systemappearing largely unaffected (data not shown). The prostratechloronemal filaments did not dedifferentiate into brood cells.With the exception of apical and a few sub-apical cells, whichremained thin-walled (Fig. 7F), the majority of these filamentsbecame thick-walled and deeply brown-pigmented (Fig. 7E,F). Numerous lipid droplets were present in the cytoplasm ofthese cells (Fig. 7G) together with abundant small vacuoles(Fig. 7H).

Dehydration
Dehydration caused few additional cytological changes and althoughgrowth was significantly reduced compared with the controlsand encapsulated treatment (week 5: P <0·001), therewere no statistical differences with the ABA/sucrose treatment(Fig. 1). Numerous small vacuoles were present in the cytoplasmof dehydrated cells (Fig. 5G) and the cell wall remainedhighly heterogeneous and with conspicuous extensions in theirinnermost layers (Fig. 5H). The starch grains in the plastids,however, were less numerous and much smaller than in the hydratedcells (Fig. 5F), and within the nucleus, conspicuous blocksof condensed chromatin surrounded the highly compacted nucleolus(Fig. 5G). Mitochondria were generally rounded and withstraight tubular cristae (Fig. 5F, H).

Cryopreservation and subsequent re-hydration
Light microscopy showed the frozen cells to be flattened withrounded or discoidal plastids distributed throughout the celllumen (Fig. 8A). One hour after removal from LN, the cytoplasmhad expanded but remained packed with numerous small vacuolesand large lipid droplets (Fig. 8B, C). The cytoplasm inthe apical cells was less dense (Fig. 8D) and incompletecross walls, resembling those in the sucrose/ABA-treated hydratedcells, were often present (Fig 8E). The overall appearanceof the cells remained unchanged even after several weeks ofrecovery (Fig. 8F). Growth at 5 weeks was significantlyreduced compared with the control and encapsulated treatments(P < 0·001), but no statistical differences were detectedbetween the three post-ABA/sucrose treatments (Fig. 1).

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FIG. 8. Light micrographs of frozen and thawed protonemal cells. (A) Frozen cells mounted in immersion oil, the cells are flattened and the discoidal plastids are distributed throughout the cell lumen. (B–E) Frozen cells 1 h after thawing: (B, C) elongate plastids (p) in cytoplasm packed with lipid droplets (L) and small vacuoles – note the ovoid nucleus (n) with prominent nucleolus and no evidence of condensed chromatin in (C); (D) apical cells with round nuclei and less dense cytoplasm; (E) apical cell with incomplete cross wall (arrowed). (F) Cells kept in the original alginate strip 2 weeks after thawing – the cytology remains unchanged; (G, H) Production of normal filaments 2 d (G) and 4 d (H) after removing the thawed protonema from the alginate strips. Scale bars: G, H = 200 µm; A–F = 20 µm.

The cytology of the cryopreserved cells resembled that of thedehydrated cells (Fig. 9A–E): cells were packed withsmall vacuoles and numerous lipid droplets; nuclei were roundedwith conspicuous blocks of condensed chromatin (Fig. 9A)and some starch grains remained in the plastids (Fig. 9B),especially those of the apical cells (Fig. 9D, E). In thelatter the cytoplasm was less dense, the vacuoles less numerousthan in the other cells (Fig. 9D and E), and short segmentsof tubular endoplasmic reticulum (ER) were often present inthe proximity of the cell wall (Fig. 9E). As in the driedcells, mitochondria were ovoid with tubular, parallel cristae(Fig. 9C).

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FIG. 9. Transmission electron micrographs of frozen and thawed protonemal cells. (A–E) Frozen cells: (A) elongated plastids and nucleus with condensed chromatin – note the numerous lipid droplets and the small vacuoles in the cell lumen; (B) plastids with intact thylakoids and small starch grains; (C) rounded mitochondria with thin, parallel-sided cristae; (D) ovoid plastids with starch grains in an apical cell. (E) Short segments of ER (arrowed) remaining in the lumen of an apical cell (cw, cell wall). (F–H) Frozen cell 1–4 h after thawing: (F) the cytoplasm is packed with small vacuoles and numerous lipid droplets; (G) profiles of tubular ER (arrowed) are scattered in the cytoplasm amongst the mitochondria and the plastids, which now contain numerous starch grains, especially those of the apical cells (H). cw, Cell wall. Scale bars: A, F = 5 µm; B, D, E, G, H = 2 µm; C = 1 µm.

After 1–4 h following removal from LN, the cytoplasm hadincreased in volume but remained packed with numerous smallvacuoles and large lipid droplets (Fig. 9F). Small pocketsof cytoplasm between the nuclei, plastids and mitochondria containeddictyosomes and profiles of tubular ER (Fig. 9G). The plastids,especially those of the apical cells (Fig. 9H) containednumerous starch grains and were indistinguishable from the controls.Thereafter, the cytology of the protonemata remained unchangedand 24 h after removal from LN, the appearance of the cellswas the same as that after 4 h (data not shown).

When re-hydrated cells were removed from the alginate stripsand then placed onto standard growth medium they promptly regenerated,producing a normal protonemal system within 2–3 d (Fig. 8G,H). The same was also true for sucrose/ABA-treated and dehydratedcells (data not shown).

Ditrichum plumbicola in the wild
Gemmiferous protonemata around the periphery of gametophorecolonies were not detected in the three wild populations ofD. plumbicola examined in the present study. Older coloniesof D. plumbicola, particularly where the soil showed no signsof recent disturbance, were often overgrown by the perennialprotonemata of Pogonatum aloides (Fig. 10A). Analysis ofthe rhizoids revealed a similar absence of asexual propagules.Both freshly collected rhizoids (Fig. 10C) and those keptas herbarium specimens (Fig. 10B) had thick brown-pigmentedwalls and were packed with food reserves mainly in the formof large lipid droplets interspersed with occasional starchdeposits (Fig. 10C). Some had minute longitudinally alignedplastids like those seen in culture (Fig. 10D). When bothfreshly collected and stored rhizoids were placed on culturemedium they produced typical protonemata indistinguishable fromthe cultured controls within 2–3 d (Fig. 10E).

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FIG. 10. Ditrichum plumbicola from the wild: (A) scanning electron micrograph of mature colony showing D. plumbicola gametophores overgrown by the perennial protonemata of Pogonatum aloides; (B–D) light micrographs of herbarium (B) and freshly collected (C and D) material showing thick-walled rhizoids packed with lipid droplets of various sizes and only occasional starch grains (C) – in (D) note the minute plastids (arrowed) aligned along cytoplasmic strands like those seen in culture (see Fig. 4C); (E) normal protonemal system regenerating from > 1-year-old herbarium material. Scale bars: E = 100 µm; B–D = 50 µm; A = 20 µm.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

The results clearly showed that exposure to a combination ofsucrose and ABA inhibited growth and caused marked morphologicaland cytological changes to the protonemal cells of Ditrichumplumbicola. The majority of cells died but those that remainedviable were characterized by thick walls, abundant lipid droplets,and by numerous small vacuoles in their cytoplasm. These cellshad the ability to survive desiccation and cryopreservationin LN largely unperturbed. Once the ABA/sucrose stimulus wasremoved, i.e. following re-hydration and removal from the originalalginate-matrix, the cells quickly regenerated into a normalprotonemal system. Encapsulation in an alginate-matrix alonehad little or no effect, apart from a reduction in protonemalgrowth rate. ABA and sucrose, applied singly, elicited changessimilar to, but less pronounced than, those of the combinedtreatment, with the majority of the cells remaining alive. Theeffects of ABA were more pronounced and extended to all thefilaments, while sucrose affected exclusively the prostratesystem. Cells with morphology typical of brood cells were producedonly in response to ABA but not sucrose.

Cytological considerations
Duckett and Ligrone (1992) and Goode et al. (1993a) describedthe formation of typical brood cells, as spherical or ovatecells ‘derived by re-differentiation from initially cylindricalchloronemal cells by swelling and breakdown of the middle lamellaeof the cross walls’. The cells formed from D. plumbicolaafter pre-treatment with sucrose/ABA were similar to, even ifnot entirely congruent with, this description and will thereforebe referred to as ‘brood bodies’.

The cytology of the brood bodies was remarkably similar to thatdescribed by Goode et al. (1994) for Aloina aloides and by Goode (1992)for a number of other species from ageing cultures or afterexposure to ABA alone. Ultrastructural observations also revealedthe D. plumbicola brood bodies to have characteristics typicalof drought-tolerant propagules, e.g. thick cell walls and densecytoplasm containing numerous small vacuoles and lipid droplets(Goode et al., 1994; Schnepf and Reinhard, 1997).

The presence of abundant food reserves is a common feature ofbryophyte spores (Brown and Lemmon, 1987, 1988), and leaf cellsof desiccation-tolerant mosses often contain small vacuoles(Tucker et al., 1975; Proctor and Tuba, 2002). Vacuolar fragmentationin response to drying has been extensively reported in desiccation-tolerantvascular (resurrection) plants (Gaff et al., 1976; Thomson and Platt, 1997;Vander Willigen et al., 2003) and, recently, in both the leafcells (Proctor et al., 2007) and food-conducting cells (Pressel et al., 2006)of the desiccation-tolerant moss Polytrichum formosum. Nagao et al. (2005)showed that exposure to ABA induced vacuolar fragmentation inprotonemal cells of Physcomitrella patens.

The dehydration treatment caused relatively few cytologicalchanges to the brood bodies of D. plumbicola, and the integrityof the membranes and organelles was retained throughout thedrying process. This supports the assertion that the brood bodiesthemselves are highly desiccation tolerant. Chromatin condensationwas most likely a direct consequence of the withdrawal of waterfrom the cells (Pressel et al., 2006) and is a typical featureof seeds during the dehydration phase of maturation (Klein and Pollock, 1968).Changes in the internal structure of mitochondria have beendescribed previously in dried vegetative tissues in numerousplant systems, and are indicative of metabolic inactivity (Dalla Vecchia et al., 1998;Navari-Izzo et al., 2000; Proctor et al., 2007).

The disappearance of starch from the plastids in the dry statehas been previously reported, e.g. in the mosses Polytrichumformosum (Pressel et al., 2006; Proctor et al., 2007) and Sphagnum(Gerdol et al., 1996), and the resurrection angiosperms Sporobolusstapfianus (Quartacci et al., 1997; Dalla Vecchia et al., 1998),Craterostigma plantagineum (Bianchi et al., 1991; Norwood et al., 2000)and Craterostigma wilmsii (Vicre et al., 2004). Perhaps themost likely explanation for the persistence of a few small starchgrains in the plastids of D. plumbicola after drying, is thatthese cells already contained high levels of soluble carbohydratesfollowing the sucrose pre-treatment. It is also possible thatthe rate of drying in the laminar flow hood did not allow sufficienttime for all the starch to be hydrolysed. Further, death ofthe caulonemal cells may have prevented the translocation ofsoluble carbohydrates.

Once dried, the brood bodies of D. plumbicola survived cryopreservationwithout incurring further cytological changes. Their promptreturn to the pre-drying and pre-cryopreservation state uponremoval from LN and re-hydration was shown by an increase inthe ER network, the reappearance of numerous starch grains inthe plastids, and changes in the internal structure of the plastidsand mitochondria. This confirms previous reports that driedplant tissues can survive extreme cold (Bequerel, 1951; Pence, 2000)and further emphasizes the link between desiccation toleranceand freezing survival (Burch, 2003).

ABA, sugars and desiccation biology
Sugars and ABA have been linked to improved desiccation andfreezing tolerance in a wide range of plant tissues (Pence, 1998;Sreedhar et al., 2002; e.g. Werner et al., 1991; Zhu et al., 2006)with potentially interacting protective effects (Suzuki et al., 2006).They are often incorporated singly or in combination into cryopreservationprotocols (e.g. Burch and Wilkinson, 2002; Fang et al., 2004).

Sugars and specific proteins play important roles during theloss of cellular water, by protecting membranes and macromoleculesvia direct interaction and by immobilizing the cytoplasm intoa highly viscous, glassy state (for a review, see also Buitink and Leprince, 2004;Alpert, 2006). Sugars are also osmotic agents, reducing cellwater content (Benson, 1999; Zhu et al., 2006) and there isevidence that they play a further protective role by scavengingdamaging free radicals (Linders et al., 1997).

Many of the responses elicited by ABA in bryophytes are thesame, or very similar to, those described in higher plants (Beckett, 2001).In bryophytes specifically, besides increasing desiccation andfreezing tolerance (Hartung et al., 1987; Nagao et al., 2005;Pence et al., 2005), exogenous ABA has been shown to inducethe production of specific proteins (Bopp and Werner, 1993;Werner et al., 1991), inhibit cytokinin-stimulated bud induction(Valadon and Mummery, 1971) and reduce protonemal growth rates(Burch and Wilkinson, 2002). Following ABA treatment, the mossFunaria hygrometrica (Werner et al., 1991) and the liverwortsRiccia fluitans and Pallavicinia lyellii (Pence et al., 2005)were able to withstand faster rates of desiccation, while toleranceof the moss Atrichum androgynum to ion leakage during rehydrationwas enhanced (Beckett, 2001; Guschina et al., 2002). ABA hasalso been shown to be an important stimulus in the transitionof the liverwort Riccia fluitans from water to land form (Hellwege et al., 1992).

The failure of protonemal cells of D. plumbicola to regeneratewithin the alginate strips following removal from LN and re-hydrationis attributed to an accumulation and retention of ABA in thealginate strip following pre-treatment. That these cells promptlyregenerated once removed from the alginate strips and placedonto fresh culturing medium, supports this suggestion. Theseresults also agree with studies on brood cell formation (Goode, 1992;Goode et al., 1993a), which showed that once produced, broodcells did not germinate in situ but only after they were transferredto new growth medium. The same has also been demonstrated forprotonemal gemmae (Duckett and Ligrone, 1991).

Extremeophile propagules
The desiccation- and cryopreservation-tolerant brood bodiesof D. plumbicola resemble such ‘extremophile’ propagulesas those produced by microbes in the high arctic and the encystedembryos of the crustacean Artemia franciscana (Clegg, 2005;Mueller et al., 2005). Mueller et al. (2005) suggested thatpigmentation of the microbial propagules provided protectionfrom a range of environmental stresses, whilst Clegg (2005)indicated that the tough shell of Artemia cysts ensured survivalof the embryos within. The Ditrichum brood bodies with theirthick, pigmented walls clearly join the category of ‘extremophile’propagules.

Ecological considerations
Although wild asexual propagules of Ditrichum plumbicola werenot detected in the present study, they have been observed previously.Arts (1994) described the occasional occurrence of rhizoidaltubers comprising uniseriate rows of five to eight swollen thick-walledcells, 50–90 µm in diameter, terminated distallyby smaller (20–30 µm) lenticular apical cells. Thetubers also regenerated into green chloronemata when placedon fresh medium. This description bears a striking resemblanceto the brood bodies reported in the present study and it islikely that they are the same structures.

Analysis of both freshly collected rhizoids (Fig. 10C)and rhizoids kept as herbarium specimens (Fig. 10B) revealedthat these were also packed with lipid and starch reserves similarto those in the ABA/sucrose-induced brood bodies. Again, theyregenerated rapidly when transferred to fresh culture medium(Fig. 10E). The rapid formation of protonemata from structuressuch as rhizoids, tubers and brood bodies would likely giveD. plumbicola a competitive advantage after cryoturbatic disturbanceof the soil over species, such as Pogonatum aloides, the protonemal/rhizoidalsystems of which lack asexual propagules (Duckett et al., 2004).When the ground remains undisturbed, Ditrichum does indeed becomeoverrun by the perennial protonemata of Pogonatum (Fig. 10A)and other slower growing, but ultimately more competitive species.This is further demonstrated by another pioneer moss, Disceliumnudum, which also gains a temporal advantage over ultimatelymore successful competitors, following winter exfoliation ofthe clay banks on which it grows (Duckett and Pressel, 2003).These data support a growing body of evidence that asexual propagulesare potentially very important in the continued survival anddispersal of mosses, including threatened species (Preston, 2004;Mallon et al., 2006).

The role of natural endogenous ABA in the desiccation and freezingtolerance of D. plumbicola merits further consideration. Certainlythe marked tendency to dedifferentiate into brood cells exhibitedby protonemal cultures as young as 2–3 weeks, suggeststhat high levels of endogenous ABA may be present. The productionof brood cells in vitro is usually associated with ageing (presumablyin response to dehydration and/or accumulation of ABA in themedium) or with exposure to exogenous ABA (Goode, 1992; Goode et al., 1993a).While it is well known that exogenous ABA increases the desiccationand freezing tolerance of bryophytes (e.g. Beckett et al., 2000;Nagao et al., 2005; Pence et al., 2005), only a handful of studieshave reported the presence of endogenous ABA (Hartung et al., 1987;Werner et al., 1991; Hellwege et al., 1994), with only two demonstratingan increase in endogenous ABA levels during drying (Werner et al., 1991;Hellwege et al., 1994). Clearly, and as discussed previouslyby Proctor and Tuba (2002), there is now the need for a systematicsearch for endogenous ABA in bryophytes and of a comprehensivestudy to determine whether endogenous ABA levels increase duringdrying.

CONCLUSIONS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

Exposure to a combination of exogenous sucrose and ABA causesthe protonema of the moss D. plumbicola to transform into specializedresting propagules or brood bodies. The cytology of these isconsistent with that of moss brood cells previously described.The brood bodies are able to withstand extreme desiccation andcryopreservation stress, confirming that they are resting cellspre-adapted to withstand desiccative stress. The formation ofsuch cells confers on D. plumbicola an additional survival strategy,and this has been exploited for the conservation of the speciesvia cryopreservation.

ACKNOWLEDGEMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

We thank English Nature (Natural England), Scottish NaturalHeritage and Countryside Council for Wales for funding the exsitu bryophyte project, and the Natural History Museum, leadpartner on the Biodiversity Action Plan for Ditrichum plumbicola,for permission to collect material for the project and thisstudy. Dr R. Preziosi, University of Manchester, gave statisticaladvice. S.P. held a Natural Environment Research Council (UK)/CASEstudentship with the Royal Botanic Gardens, Kew. Thanks alsoto two anonymous reviewers for comments on an earlier draftof this manuscript.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
ABA/sucrose experiment
RESULTS
DISCUSSION
CONCLUSIONS
ACKNOWLEDGEMENTS
LITERATURE CITED

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