Glomus eburneum and Scutellospora fulgida, species of arbuscular 
mycorrhizal fungi (Glomeromycota) new for Europe

Janusz Błaszkowski and Beata Czerniawska 

Department of Plant Pathology, University of Agriculture in Szczecin 
słowackiego 17, PL-71-434 szczecin, jblaszkowski@agro.ar.szczecin.pl

Błaszkowski J., Czerniawska B.: Glomus eburneum and Scutellospora fulgida, species of arbuscular 
mycorrhizal fungi (Glomeromycota) new for Europe. acta Mycol. 43 (1): 57–65, 2008.

Morphological characters of spores and mycorrhizae of Glomus eburneum and spores 
of Scutellospora fulgida, arbuscular mycorrhizal fungi of the phylum Glomeromycota, are 
described and illustrated. additionally, the known distribution of these species in both Poland 
and other regions of the world is presented. Both species were not earlier reported from 
europe.  

Key words: Glomus eburneum, Glomeromycota, Scutellospora fulgida, occurrence

introduCtion

examination of pot trap cultures with mixtures of rhizosphere soils and roots col-
lected in Poland and other regions of the world revealed spores of Glomus eburneum 
L.J. kenn., J.C. stutz et J.B. Morton and Scutellospora fulgida koske et C. walker, 
arbuscular mycorrhizal fungi of the phylum Glomeromycota. Both species were not 
earlier reported from europe.  

the aims of this paper are to describe and illustrate these species and present 
their distribution in both Poland and the world.

MateriaLs and Methods

Establishment and growth of trap and one-species cultures, extraction of spores, 
and staining of mycorrhizae. spores examined in this study came from both pot trap 
and one-species cultures. trap cultures were established to obtain a great number of 
living spores of different developmental stages and to initiate sporulation of species 
that were present but not sporulating in the field collections (stutz, Morton 1996).  
the method used to establish trap cultures, their growing conditions, and the meth-
od of spore extraction were previously described (Błaszkowski et al. 2004, 2006).

 aCta MYCoLoGiCa
 Vol. 43 (1): 57–65
 2008



58 J. Błaszkowski and B. Czerniawska 

one-species cultures were also generally established and grown as given in 
Błaszkowski et al. (2004), with two exceptions. First, instead of marine sand, their 
growing medium was an autoclaved commercially available coarse-grained sand 
(grains 1.0-10.0 mm diam. - 80.50%; grains 0.1-1.0 mm diam. - 17.28%; grains < 
0.1 mm diam. - 2.22%) mixed (5:1, v/v) with clinopthilolite (zeocem, Bystré, slo-
vakia) of grains 2.5-5 mm. Clinopthilolite is a crystaline hydrated alumosilicate of 
alkali metals and alkaline earth metals having, e.g., a high ion exchange capability 
and selectivity, as well as a reversible hydration and dehydration. ph of the sand-
clinopthilolite mixture was 7.3. second, the cultures were kept in transparent plastic 
bags, 15 cm wide and 22 cm high as suggested by walker and Vestberg (1994), rather 
than open pot cultures (Gilmore 1968). to prevent contamination of the cultures 
with other aMF but still to allow exchange of gases, we left an opening, ca. 1 cm 
wide, in the centre of the upper part of each bag, while the edges on both sides 
were closed with small plastic clips. the cultures were watered with tap water once 
a weak, harvested after five months when spores were extracted for study. to reveal 
mycorrhizae, root fragments located ca. 1-5 cm below the upper level of the growing 
medium were cut off with a scalpel. the host plant used in both trap and one-species 
cultures was Plantago lanceolata L. 

Microscopy survey. Morphological properties of spores and their wall structure 
were determined based on examinations of at least 100 spores mounted in polyvinyl 
alcohol/lactic acid/glycerol (PVLG; omar, Bollan and heather 1979) and a mixture 
of PVLG and Melzer’s reagent (1:1, v/v). spores at all developmental stages were 
crushed to varying degrees by applying pressure to the cover slip and then stored at 
65oC for 24 h to clear their contents from oil droplets. these were then examined 
under an olympus BX 50 compound microscope equipped with nomarski differen-
tial interference contrast optics. Microphotographs were recorded on a sony 3Cdd 
color video camera coupled to the microscope.

terminology of spore structure is that suggested by stürmer and Morton (1997) 
and walker (1983). spore colour was examined under a dissecting microscope on 
fresh specimens immersed in water. Colour names are from kornerup and wan-
scher (1983). nomenclature of fungi and plants is that of walker and trappe (1993) 
and Mirek et al. (1995), respectively. the authors of the fungal names are those pre-
sented at the index Fungorum website http://www.indexfungorum.org/authorsof-
Fungalnames.htm. specimens were mounted in PVLG on slides and deposited in 
the department of Plant Pathology, university of agriculture, szczecin, Poland.

Colour microphotographs of spores and mycorrhizae of the fungi presented here 
can be viewed at the urL http://www.agro.ar.szczecin.pl/~jblaszkowski/.

desCriPtions oF the sPeCies

Glomus eburneum L.J. kenn., J.C. stutz et J.B. Morton
Sporocarps unknown. Spores occur singly in the soil (Fig. 1); origin blastically at 

the tip of hyphae continuous with extraradical mycorrhizal hyphae. spores yellow-
ish white (4a2) to butter yellow (4a5); globose to subglobose; (92-)108(-146) μm 
diam; or ovoid; 104-115 x 123-139 μm; with one subtending hypha (Figs 1, 2, 5 and 
6). Subcellular structure of spores consists of a spore wall composed of two tightly 
adherent layers (layers 1 and 2; Figs 2-5). Layer 1, forming the spore surface, semi-



 Glomus eburneum and Scutellospora fulgida 59

permanent, semi-flexible, hyaline, (0.7-)1.0(-1.2) μm thick, frequently intact or only 
slightly deteriorated in mature spores, sometimes associated with granular soil de-
bris. Layer 2 laminate, semi-flexible, smooth, yellowish white (4a2) to butter yellow 
(4a5), (2.5-)3.5(-4.4) μm thick. none of the two layers stains in Melzer’s reagent. 
Subtending hypha yellowish white (4a2) to butter yellow (4a5); straight or recurved; 
cylindrical or slightly flared, sometimes slightly constricted; (7.8-)9.9(-14.0) μm wide 
at the spore base (Figs 1, 5 and 6). Wall of subtending hypha yellowish white (4a2) 
to butter yellow (4a5); (1.0-)1.6(-2.7) μm thick at the spore base; composed of two 
layers continuous with spore wall layers 1 and 2 (Fig. 5). Pore 3.8-5.1 μm diam. open 
or occluded by a straight or recurved septum, (1.0-)1.4(-2.0) μm thick, continuous 
with the innermost laminae of the laminate spore wall layer 2, positioned up to 11.3 
μm below the spore base (Figs 5 and 6). Germination. not observed.

Mycorrhizal associations. the presence of mycorrhizae in field-collected root 
samples was not determined. 

in one-species cultures with P. lanceolata as the host plant, mycorrhizae of G. 
eburneum comprised arbuscules, as well as intra- and extraradical hyphae. arbus-
cules consisted of short trunks branched from parent hyphae and numerous branch-
es with very fine tips (Figs 7 and 8). their distribution along root fragments ranged 
from uniform to patchy, depending on the root fragment examined. intraradical 
hyphae grew along root axis, were (2.0-)4.9(-8.3) μm wide and sometimes formed 
Y- or h-shaped branches and coils (Figs 7 and 8). the coils were ellipsoid, 10.5-
23.3 x 36.8-57.4 μm, when observed in a plane view. extraradical hyphae were (2.7-) 
3.1(3.4) μm wide and occurred very rarely and in low abundances. in 0.1% trypan 
blue, arbuscules stained violet white (15a2) to light lilac (16a5), intraradical hyphae 
violet white (16a2) to pale violet (16a3), coils lilac (16a5) to royal purple (16d8), 
and extraradical hyphae violet white (16a2) or remained unstained.

Phylogenetic Position. kennedy, stutz and Morton (1999) concluded that 
the lack of vesicles and the faintly staining other components of mycorrhizae of 
G. eburneum are untypical of most species of the genus Glomus, but are charac-
teristic for, e. g., Archaeospora trappei (r.n. ames et Linderman) J.B. Morton et 
d. redecker emend. spain, Appendicispora gerdemannii (s.L. rose, B.a. daniels 
et trappe) spain, oehl et sieverd. and Diversispora spurca (C.M. Pfeiff., C. walker 
et Bloss) C. walker et schuessler, of which the former two fungi come from the 
order archaeosporales C. walker et schuessler and the latter one has recently been 
accommodated in the family diversisporaceae C. walker and schuessler of the or-
der diversisporales C. walker et schuessler (schüßler, schwarzott and walker 2001; 
spain, sieverding and oehl 2006; walker and schüßler 2004). Gamber and Leucht-
mann (2007) found the inVaM isolate az420a of G. eburneum to be in a sister po-
sition to G. versiforme (P. karsten) s.M. Berch, being phylogenetically most closely 
related to D. spurca (schwarzott, walker and  schüßler 2001).

Distribution anD habitat. in Poland, spores of G. eburneum were found in only 
one trap culture containing a mixture of rhizosphere soil and root fragments taken 
from under Helichrysum areanarium (L.) Moench growing in maritime sand dunes of 
the słowiński national Park (54o45’n, 17o26’e) on 26 June 2003. the occurrence of 
spores of arbuscular fungi in the field sample was not investigated. the species of ar-
buscular fungi co-occurring with G. eburneum in the trap culture were Archaeospora 



60 J. Błaszkowski and B. Czerniawska 

trappei (r.n. ames et Linderman) J.B. Morton et d. redecker emend. spain and 
G. lamellosum dalpé, koske et tews.     

The holotype of G. eburneum has been selected from spores extracted from the 
inVaM culture az420a established from a mixture of rhizosphere soil and root 
fragments of Sporobolus wrightii Monro ex scribn. growing along the san Pedro riv-
er in arizona, u.s.a. (kennedy, stutz and Morton 1999). Sporobolomyces wrightii 
is a native grass species found only along rivers and streams of the semiarid regions 
of south-western north america. additionally, the same scientists and stutz et al. 
(2000) recorded this fungus among roots of other plants growing in other sites of ar-
izona and Mexico, as well as under different plant species colonizing a dune transect 
in the namibia desert.    

collections exaMineD. Poland: szczecin, under pot-cultured P. lanceolata, 
10.02.2005, J. Błaszkowski 2682-2696 (dPP).

notes. The most distinctive characters of G. eburneum are its light-coloured 
spores filled with dense, opaque oil substance and the semi-flexible, 2-layered spore 
wall with the outermost layer nonreactive in Melzer’s reagent and usually remaining 
more or less intact in mature spores (Figs 1-6). 

when observed at a low magnification, spores of G. eburneum are most remi-
niscent of those of D. spurca, G. albidum C. walker et L.h. rhodes, G. gibbosum 
Błaszk., G. viscosum nicol., and Paraglomus occultum (C. walker) J.B. Morton et d. 
redecker. darker-coloured spores of G. eburneum may also be confused with light-
pigmented spores of G. claroideum n.C. schenck et s.M. sm. and G. versiforme. 

Except for G. versiforme, examination of spores crushed in PVLG and PVLG 
mixed with Melzer’s reagent under a compound microscope readily separates 
G. eburneum from all the other species listed above. Considering the spore wall 
structure, as well as the phenotypic and biochemical properties of its components, 
the fungus most closely related to G. eburneum is D. spurca. although the opinions 
of the number of layers overlaying the laminate spore wall layer of D. spurca are 
contradictory (one layer according to kennedy, stutz and Morton 1999 and Morton 
2002 vs. two layers as Błaszkowski (2003) stated), the laminate layer and the layer 
directly overlaying it are almost identical in both their phenotypic and biochemical 
properties. the main differences between these fungi hide in the persistency of the 
spore wall layers directly covering the structural laminate layer and the degree of 
the association of these layers with the laminate layer. Consequently, the second 
property defines the basic differences in the persistency of the subtending hyphae 
of both fungi. 

although the outer spore wall layer is relatively long-lived and usually retains as 
a more or less deteriorated structure in mature spores of G. eburneum (Figs 2-5), its 
spatially corresponding spore wall layer in D. spurca is more persistent and always 
remains intact in even old spores (Błaszkowski 2003; kennedy, stutz and Morton 
1999).

in G. eburneum, the outer spore wall layer always remains tightly adherent to the 
laminate spore wall layer (Figs 2-5), whereas the semi-flexible layer directly covering 
the laminate spore wall layer of D. spurca easily separates in crushed spores or bal-
loons when immersed in lactic acid-based mountants (Błaszkowski 2003; kennedy, 
stutz and Morton 1999).



 Glomus eburneum and Scutellospora fulgida 61

in G. eburneum, the structural layer of the subtending hyphal wall (shwl2) con-
tinuous with the laminate spore wall layer and being the support of the outer thin 
wall layer of the subtending hypha gradually thins and expands up to 25 μm below 
the spore base (Fig. 5). in contrast, in D. spurca spores, the laminate spore wall layer 
abruptly thins and stops to grow at their base and, thereby, it does not create a suf-
ficient support to stabilize the outer subtending hyphal wall layer continuous with 
the spore wall layer 2 sensu Błaszkowski (2003). therefore, almost all crushed spores 
of D. spurca usually lack the subtending hypha, which detaches along with the outer 
wall layer of these spores.  

Finally, in contrast to the opaque, frequently yellow-coloured contents of G. ebur-
neum spores, the spore contents of D. spurca consists of transparent oil droplets.  

Compared with G. albidum described to also form a 2-layered spore wall of simi-
lar phenotypic characters (walker, rhodes 1981) to those of the wall layers of spores 
of G. eburneum, spores of the latter species do not react in Melzer’s reagent (vs. 
become pink to orange red in G. albidum; walker, rhodes 1981). 

two characters of spores of G. gibbosum readily separate this fungus from 
G. eburneum. First, while spores of the former species occur in the soil singly, in loose 
aggregates and conglomerations enclosed by a common hyphal mantle (Błaszkowski 
1997, 2003), the latter fungus produces only single spores (Fig. 1). second, the spore 
wall of G. eburneum comprises only two layers (Figs 2-5), and that of G. gibbosum 
consists of four layers (Błaszkowski 2003). the spore wall of G. eburneum lacks the 
wall layers 2 and 4 of spores of G. gibbosum.

Spores of G. viscosum are also frequently formed in loose aggregates (Morton 
2002; vs. only single spores in G. eburneum; Fig. 1) and have a more complex wall 
structure (3-layered) than those of G. eburneum (2-layered; Figs 2-5). the spore wall 
layer of G. viscosum not synthesized by G. eburneum is the permanent, semi-flexible, 
thin layer positioned between a semi-flexible layer forming the spore surface and a 
laminate layer, both phenotypically similar to the spore wall layers 1 and 2, respec-
tively, of G. eburneum. 

As far as the species compared here are concerned, the fungus most diverged 
morphologically from G. eburneum is Paraglomus occultum. these species share only 
their outermost spore wall layer (Morton 2002; Morton, redecker 2001). although 
these layers in both fungi are of the type of impermanent layers, the longevity of the 
layer in G. eburneum is much higher than in P. occultum, in which it usually highly de-
teriorates with age to form a granular structure (Morton 2002), a phenomenon not 
found in G. eburneum (Figs 2-6). the two other spore wall layers of P. occultum are 
uniform and much thinner (both <0.5-1.2 μm thick) than the inner laminate spore 
wall layer of G. eburneum [(2.5-)3.5(-4.4) μm thick]. 

as mentioned above, darker-coloured spores of G. eburneum may also overlap 
in colour and appearance with light-coloured spores of G. claroideum and G. ver-
siforme. however, the former two fungi differ fundamentally in the construction 
of their spore wall, as well as in the phenotypic and biochemical properties of its 
components. Compared with the simple, 2-layered spore wall of G. eburneum (Figs 
2-6), that of G. claroideum comprises four layers with the innermost layer staining 
in Melzer’s reagent (Błaszkowski 2003; Morton 2002; stürmer, Morton 1997; vs. 
none of the spore wall layers of G. eburneum reacts in this reagent; Fig. 4). the only 
layers of the spore wall of G. claroideum sharing the phenotypic and biochemical 



62 J. Błaszkowski and B. Czerniawska 

properties of layers 1 and 2 of the G. eburneum spore wall are its layers 2 and 3, 
respectively. the distinctive component of the spore wall of G. claroideum is the in-
nermost flexible layer, which is lacking in G. eburneum.

Light-coloured spores of G. versiforme may be indistinguishable from mature 
spores of G. eburneum when observed under both a dissecting and a compound 
microscope. apart from colour, spores of the two species are almost identical in 
size, as well as in the construction and the phenotypic and biochemical properties of 
the components of their wall. Moreover, mycorrhizae of both species stain faintly in 
0.1% trypan blue (Figs 7 and 8; Błaszkowski, pers. observ.; Morton 2002). the only 
property distinguishing G. eburneum and G. versiforme is the formation of sporo-
carps by the latter fungus (Morton 2002).

apart from the morphological differences characterized above, the species 
compared here also differ in the phylogenetic position within the phylum Glomer-
omycota determined based on results of their molecular analyses. For example, 
G. claroideum and G. viscosum represent Glomus group B in the family Glomeraceae 
Piroz. et dalpé of the order Glomerales J.B. Morton et Benny, and Par. occultum, 
originally described as G. occultum C. walker, presently is a member of the fam-
ily Paraglomaceae J.B. Morton et d. redecker in the Paraglomerales C. walker 
et schuessler (schüßler, schwarzott and walker 2001). as presented in the section 
“Phylogenetic position”, G. eburneum should be a member of the family diversispo-
raceae, as Gamber and Leuchtmann (2007) found. unfortunately, the phylogenetic 
positions of G. albidum and G. gibbosum are unknown to date.    

Scutellospora fulgida koske et C. walker
Spores formed singly in the soil; origin blastically at the tip of a bulbous sporog-

enous cell; yellowish white (4a2) to cream (4a3); globose to subglobose; (165-)229 
(-280) µm diam (Fig. 9). Subcellular structure of spores consists of a spore wall and 
one inner germination wall (Figs 10-13). spore wall composed of two layers (lay-
ers 1 and 2; Figs 10, 11, 13 and 14). Layer 1, forming the spore surface, permanent, 
smooth, pale yellow (3a3) to light orange (5a5), (1.2-)2.0(-3.2) µm thick, usually 
tightly adherent to layer 2, sometimes slightly separated from it in vigorously crushed 
spores. Layer 2 laminate, smooth, yellowish white (4a2) to cream (4a3), (7.6-)9.7 
(-13.0) µm thick. Germination wall comprises two flexible, smooth layers (layers 
1 and 2; Figs 10-13). Layer 1 ca. 0.5 µm thick, adherent to layer 2, but frequently 
wrinkled in crushed spores and, thereby, giving the inner wall a rugose or blistered 
appearance and making this layer more visible. Layer 2 0.8-1.5 µm thick. in Melzer’s 
reagent, the spore wall layers 1 and 2 stain orange white (5a2) to copper (7C8) 
and pale yellow (3a3) to reddish orange (7B7), respectively, and both germination 
wall layers remain nonreactive (Figs 11-14). Sporogenous cell formed terminally on a 
sparsely septate hypha continuous with an extraradical mycorrhizal hypha; ovoid to 
clavate; (38.7-)44.6(-53.2) µm wide; cream (4a3) to light orange (5a5), usually with 
a hyphal peg (Figs 9 and 14). Wall of sporogenous cell composed of two permanent 
layers (layers 1 and 2) continuous with spore wall layers 1 and 2 (Fig. 14). Layer 1 
pale yellow (3a3) to light orange (5a5), (1.7-)2.4(-3.2) µm thick. Layer 2 cream 
(4a3) to light yellow (4a4), (1.5-)2.6(-3.9) µm thick at the spore base. Both layers 
always tightly adherent to one another and difficult to observe. Germination shield 
cardioid; pale yellow (3a3); 60-120 x 110-190 µm, of a more or less incised border; 



 Glomus eburneum and Scutellospora fulgida 63

ornamented with widely usually unequally dispersed warts, 1.5-2.5 x 0.5-1.5 µm; po-
sitioned on the upper surface of the inner germination wall (Fig. 15). one to three 
germ tubes or germ tube initials emerge from the germination shield. Auxiliary cells 
borne in the soil, in clusters of 6-10; hyaline to cream (4a3); globose to irregular; 
18-28 x 23-39 µm; with knobby projections; produced on straight or coiled hyphae; 
2.5-8.0 µm diam; concolorous with auxiliary cells (Fig. 16).

Mycorrhizal associations. the presence of mycorrhizae in field-collected root 
samples was not determined. Many attempts to growth this fungus in one-species 
cultures failed. according to Morton (2002), S. fulgida formed mycorrhizae with 
arbuscules and intraradical hyphae staining intensively in trypan blue.

Distribution anD habitat. The spores of S. fulgida showed here were extracted 
from six trap cultures with rhizosphere soils and root fragments collected under 
plants colonizing maritime dunes of Portugal (four samples), italy and oman (one 
sample each). the occurrence of arbuscular fungi in the field soil-root mixtures was 
not determined. the field samples from italy came from under Ammophila arenaria 
(L.) Link and were collected on 11 october 2002. the exact sites and dates of col-
lections of the soil and root samples, as well as the host plants sampled in Portugal 
and oman are unknown. the trap cultures with these samples were established on 
8 March 2004 and 30 June 2003, respectively, i. e., some days after they arrived to the 
laboratory of the author of this paper. the arbuscular fungi accompanying S. fulgida 
in the cultures representing italy were Acaulospora scrobiculata Trappe, Intraspora 
schenckii (sieverd. et s. toro) oehl et sieverd., Glomus aurantium Błaszk., V. Blanke, 
C. renker et F. Buscot, G. constrictum Trappe, G. versiforme (P. karsten) s.M. Berch, 
an undescribed Glomus 169, and S. persica (koske et C. walker) C. walker et F.e. 
sanders. the only arbuscular fungus co-occurring with S. fulgida in the Portugal 
culture was an undescribed Glomus 172, and the culture with the rhizosphere soil 
and root mixture of oman still contained spores of G. fasciculatum (thaxt.) Gerd. 
et trappe emend. C. walker et koske and S. persica. 

The type of S. fulgida comes from field-collected spores isolated from under 
A. breviligulata Fern. colonizing maritime dunes of the seashore state Park in Vir-
ginia, u.s.a. (koske and walker 1986). this fungus has also been found in other 
soil samples taken from under A. breviligulata, Solidago sempervirens L., and Uniola 
paniculata L. growing in dunes extending from new Jersey to Virginia (koske 1987). 
sylvia and will (1988) found spores of S. fulgida associated with U. paniculata and 
Panicum sp. growing in soils of a beach replenishment site in Florida. additionally, 
S. fulgida has been reported to occur under Triticum aestivum L. cultivated in argen-
tina (schalamuk et al. 2006) and in soils of China (Gai et al. 2006).    

collections exaMineD. Poland: szczecin, all from trap cultures with P. lanceolata 
as the host plant and rhizosphere soils and root fragments of A. arenaria sampled (1) 
near Calambrone (italy; 43o35’n, 10o18’n) on 11 october 2002 and harvested on 21 
June 2006, Błaszkowski J. 2697-2701 (dPP); (2) in oman, harvested on 15 March 
2003, Błaszkowski J. 2702-2708 (dPP); and (3) in Portugal, harvested on 22 July 
2006, Błaszkowski J. 2709-2716 (dPP). 

notes. The distinctive characters of S. fulgida are its light-coloured spores of 
a smooth surface and the sinthesization of only one inner germination wall (Figs 
9-13). the last property keys this fungus into a monophyletic group still comprising 
S. castanea C. walker, S. coralloidea (trappe, Gerd. et h.h. ho) C. walker et F.e. 



64 J. Błaszkowski and B. Czerniawska 

Sanders, S. gregaria (n.C. schenck et nicol.) C. walker et F.e. sanders, S. persica 
(koske et C. walker) C. walker et F.e. sanders, and S. verrucosa (koske et C. wal-
ker) C. walker et F.e. sanders.

Four spore characters readily separate the species listed above. First, spores of 
S. fulgida are much lighter-coloured than those of the other species compared here 
(cream to light orange in S. fulgida (Figs 9 and 10) vs. from pale straw to orange 
brown in S. verrucosa to red brown to dark brown in S. gregaria; Morton 1995, 2002). 
Second, in contrast to the smooth spores of S. castanea (walker, Gianinazzi-Pear-
son and Marion-espinasse 1993) and S. fulgida (Figs 9-14), the spore surface of the 
other species is ornamented with warts (Morton 1995, 2002). however, S. fulgida 
and S. castanea markedly differ in colour and size of spores. the darkest spores of 
the former fungus are of a yellow shade, and mature spores of the latter species are 
brown (walker, Gianinazzi-Pearson and Marion-espinasse 1993). third, although 
the lower size range of globose spores of S. fulgida and S. castanea overlaps, the larg-
est spores of S. fulgida (280 µm diam) are much smaller than the greatest spores of 
S. castanea (up to 372 µm diam; walker, Gianinazzi-Pearson and Marion-espinasse 
1993). spores of the other species discussed here may also attain a much higher size 
than those of S. fulgida (384 µm diam in S. persica to 480 µm diam in S. gregaria; 
Morton 1995). Fourth, similarly as in S. castanea, the warts ornamenting the germi-
nation shield of S. fulgida spores are much lower and less densely dispersed on its 
surface (Fig. 15) compared with those ornamenting the germination shield of the 
other species. this also causes the germination shields of the former two species to 
be relatively more flexible, as Morton (1995) concluded. 

Acknowledgements.  this study was supported in part by the Committee of scientific researches, a grant 
no. 2 P04C 041 28.

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Glomus eburneum i Scutellospora fulgida, nowe dla europy gatunki mikoryzowych 
grzybów arbuskularnych (Glomeromycota)

S t r e s z c z e n i e

opisano i zilustrowano cechy morfologiczne zarodników i mikoryz Glomus eburneum oraz 
zarodników Scutellospora fulgida, mikoryzowych grzybów arbuskularnych z gromady Glome-
romycota. Ponadto przedstawiono poznane rozmieszczenie tych gatunków zarówno w Polsce, 
jak i innych regionach świata. oba te gatunki nie były wcześniej podawane z europy.



Figs 1-8. Glomus eburneum. 1. Intact spores. 2. Spore wall layers 1 (swl1) and 2 (swl2) and 
subtending hypha. 3 and 4. Spore wall layers 1 (swl1) and 2 (swl2). 5. Spore wall layers 1 (swl1) 
and 2 (swl2), subtending hyphal wall layers 1 (shwl1) and 2 (shwl2), and curved septum. 6. Sub-
tending hypha occluded by curved septum. 7 and 8. Arbuscules, trunk, intraradical hyphae, 
and coil of mycorrhizae stained in 0.1% trypan blue. Fig. 1, spores in lactic acid. Figs 2, 3, 5-8, 
spores crushed in PVLG. Fig. 4, spore crushed in PVLG+Melzer’s reagent. Fig. 1, bright field 
microscopy. Figs 2-8, differential interference contrast. 



Figs 9-16. Scutellospora fulgida. 9. Intact spores with bulbous sporogenous cells. 10-13. 
Spore wall layers 1 (swl1) and 2 (swl2) and inner germination wall layers 1 (gwl1) and 2 
(gwl2). 14. Spore wall layers 1 (swl1) and 2 (swl2) and sporogenous cell wall layers 1 (scwl1) 
and 2 (scwl2). 15. Germination shield with germ tube and two germ tube initials. Fig. 9, 
spores in lactic acid. Figs 10 and 16, spores crushed in PVLG. Figs 11-15, spores crushed in 
PVLG+Melzer’s reagent. Fig. 9, bright field microscopy. Figs 10-16, differential interfer-
ence contrast. 


		2014-01-01T11:47:14+0100
	Polish Botanical Society