Ambispora gerdemannii and Glomus badium,  
two species of arbuscular fungi (Glomeromycota)  

new for Europe and Poland, respectively

1Janusz Błaszkowski, 1Beata Czerniawska, 1sławomir kowalCzyk, 
2katarzyna turnau and 3szymon zuBek

1Department of Plant Protection, west Pomeranian university of technology 
słowackiego 17, Pl-71-434 szczecin, janusz.blaszkowski@zut.edu.pl 

2Department of ecological microbiology, institute of environmental sciences 
Jagiellonian university, Gronostajowa 7, Pl-30-387 kraków, katarzyna.turnau@uj.edu.pl 

3laboratory of mycology, institute of Botany, Jagiellonian university 
lubicz 46, Pl-31-512 kraków, szymon.zubek@uj.edu.pl

Błaszkowski J., Czerniawska B., kowalczyk s., turnau k., zubek s.: Ambispora gerdemannii 
and Glomus badium, two species of arbuscular fungi (Glomeromycota) new for Europe and 
Poland, respectively. acta mycol. 45 (1): 17–25, 2010.

morphological characters of spores, as well as sporocarps and spores of Ambispora 
gerdemannii and Glomus badium, respectively, arbuscular fungi of the phylum Glomeromycota, 
are described and illustrated. additionally, the known distribution of these species in both 
Poland and the other regions of the world is presented.  Ambispora gerdemannii was not 
earlier reported from europe, and G. badium is a new fungus for Poland. 
Key words: Glomeromycota, occurrence, distribution

introDuCtion

analysis of collections of arbuscular-mycorrhizal fungi made over the last 27 years 
in Poland and other regions of the world included two unrecorded species, i. e., 
Ambispora gerdemannii (s.l. rose, B.a. Daniels et trappe) spain, oehl et sieverd. 
and Glomus badium oehl, redecker et sieverd. the former fungus has not so far 
been reported from europe, and the latter species has not been reported to occur 
in Poland to date.

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

 aCta myColoGiCa
 Vol. 45 (1): 17–25
 2010

Dedicated to Professor Barbara Gumińska 
on the occasion of her eighty-fifth birthday



18 J. Błaszkowski et al. 

materials anD methoDs

the methods of collection of soil samples, establishment of trap and one-species cul-
tures, growth conditions, isolation and preparation of spores and the determination 
of properties of their subcellular structure, as well as the terminology of spore struc-
ture and colours, the nomenclature of plants and fungi, and the authors of the fun-
gal names used are as those presented previously (Błaszkowski, Czerniawska 2005). 
microphotographs were recorded on a sony 3CDD color video camera coupled to 
an olympus BX 50 compound microscope equipped with nomarski differential in-
terference contrast optics.

Voucher specimens were 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) on slides and deposited in the Department of Plant Pathology (DPP).

Colour microphotographs of spores of Am. gerdemannii and G. badium can be 
viewed at the url http://www.agro.ar.szczecin.pl/~jblaszkowski/.

DesCriPtions of the sPeCies

Ambispora gerdemannii (s.l. rose, B.a. Daniels et trappe) C. walker, Vestberg et 
schuessler

spores formed singly in the soil; arise blastically at the tip of a hyphal branch 
(pedicel) on the neck of a sporiferous saccule (figs 1 and 8). Spores pale yellow (4a3) 
to maize yellow (4a6), globose to subglobose, (150-)210(-250) μm diam, sometimes 
ovoid, 150-190 × 210-250 μm. Subcellular structure of spores consists of a spore wall 
and two inner germination walls (figs 3-6 and 8). Spore wall composed of three lay-
ers (layers 1-3). layer 1, forming the spore surface, evanescent, pale yellow (4a3) to 
maize yellow (4a6), (1.7-)3.3(-5.6) μm thick when intact, usually with deep fissures 
due to sloughing with age (figs 1 and 2). layer 2 semi-flexible, smooth, hyaline 
(1.2-)2.5(-3.7) μm thick, continuous with the wall of the pedicel (figs 3-6 and 8). 
layer 3 flexible to semi-flexible, hyaline, 0.5-1.0 μm thick, usually tightly adherent to 
the lower surface of layer 2 and, hence, difficult to see (figs 3-5 and 8). Germination 
wall 1 comprises two fragile, smooth, hyaline layers (layers 1 and 2), (0.5-)1.1(-1.6) 
μm and (0.6-)1.4(-2.1) μm thick, respectively, usually tightly adherent to one another 
and readily cracking to form line slits or polygonal pieces in crushed spores (figs 
3-8). Germination wall 2 consists of three smooth, hyaline layers (layers 1-3; figs 3-5 
and 8). layer 1 flexible to semi-flexible, 0.5-0.8 μm thick, always tightly adherent to 
layer 2 and, thereby, very difficult to observe (figs 3-5). layer 2 semi-flexible, finely 
laminate, hyaline, (1.7-)2.8(-4.1) μm thick (figs 3-5 and 8). layer 3 flexible to semi-
flexible, 0.5-0.8 μm thick (figs 3-5), rarely separating from layer 2. in melzer’s rea-
gent, only spore wall layer 1 stains orange (6a6) to pastel red (8C5; fig. 5). Pedicel 
10-15 μm long, 15-27 μm wide at the spore base, positioned 80-120 μm from the base 
of the sporiferous saccule, consisting of a hyaline wall continuous with the wall of the 
saccule neck, the spore wall, and layer 1 of germination wall 1 (fig. 8). Spori ferous 
saccule hyaline to yellowish white (4a2), globose to subglobose, (185-)200(-275) μm 



Figs 1-8. Ambispora gerdemannii. 1. Spore (sp) associated with the neck (n) of sporiferous 
saccule (ss). 2. Partly deteriorated spore wall layer 1 (swl1). 3-5. Spore wall layers 1-3 (swl1-3), 
layers 1 and 2 of germination wall 1 (gw1l1+2), and layers 1-3 of germination wall 2 (gw2l1-3). 
6. Spore wall layers 1-3 (swl1-3) and layers 1 and 2 of germination wall 1 (gw1l1+2) with line 
splits in slightly crushed spore. 7. Disintegrated layers 1 and 2 of germination wall 1 (gw1l1+2) 
in vigorously crushed spore. 8. Spore wall layers 1-3 (swl1-3), layers 1 and 2 of germination 
wall 1 (gw1l1+2), layers 1-3 of germination wall 2 (gw2l1-3), and pedicel (p) with a wall con-
tinuous with spore wall layer 2. Fig. 1, spore in lactic acid. Figs 2-4 and 6-8, spores crushed in 
PVLG. Fig. 5, spore crushed in PVLG+Melzer’s reagent. Fig. 1, bright field microscopy; Figs 
2-8, differential interference contrast. Scale bars for Fig. 1=50 μm, for Figs 2-8=10 μm.



Figs 9-16. Glomus badium. 9. Sporocarp. 10. Hyphal plexus (hp). 11. Interspore mycelium 
(im). 12. Cystidium-like structure (cs). 13. Spore wall layers 1-3 (swl1-3). 14. Spore wall lay-
ers 1-3 and interspore mycelium (im); septum (s) of the subtending hypha formed by spore 
wall layer 3 is indicated. 15. Subtending hyphal wall layers 1 and 2 (shwl-2). 16. Plug (p) in 
the lumen of subtending hypha. Figs 9 and 11-16, spores crushed in PVLG. Fig. 10, spore 
crushed in PVLG+Melzer’s reagent. Figs 9-16, differential interference contrast. Scale bars 
for Fig. 9=20 μm, for Figs 10-16=10 μm.



 Ambispora gerdemannii and Glomus badium 19

diam, occasionally ovoid, 160-200 × 210-260 μm, formed at the end of a funnel-
shaped neck (fig. 1). Wall of sporiferous saccule semi-flexible, semi-permanent, hya-
line to yellowish white (4a2), 3.5-8.8 μm thick, smooth in young specimens, rough-
ened because of a patchy sloughing of its outer surface, composed of two to three 
tightly adherent layers, usually difficult to observe. Saccule neck hyaline to yellowish 
white (4a2), 200-250 μm long, 30-45 μm wide at the base of the saccule, 20-25 μm 
wide at the spore base, then gradually tapering up to 8-10 μm wide. 

ColleCtions examined. Poland. Przelewice (53o06’n, 15o05’e), under Thuja occidentalis l., 29 sept. 
1989, Błaszkowski J. 1722 and 1783-1801 (DPP); truskaw (52°18’n, 20°46’e), from the root zone of Juni-
perus communis l., 9 aug. 1990, Błaszkowski J. 1802-1804 (DPP); trzciel (52°22’n, 15°52’e), among roots 
of Equisetum arvense l., 13 aug. 2004, Błaszkowski J. 1805-1806 (DPP); romanówek (52°17’n, 15°22’e), 
from under Achillea millefolium l. and Hypericum perforatum l., 13 aug. 2004, Błaszk. J., s.n. (DPP); 
lubrza (52°18’n, 15°27’e), under H. perforatum, 13 aug. 2004, Błaszk. J. s.n. (DPP); tatra mountains, 
among roots of Campanula polymorpha witasek, Cardaminopsis neglecta (schul.) hayek, Cerastium tatrae 
Borbás, Knautia kitaibelii (schult.) Borbás, Leucanthemum waldsteinii (sch. Bip.) Pouzar, Melampyrum 
herbichii woł., Sesleria tatrae (Degen) Deyl, and Thymus sp., Błaszkowski J. 2634-2643 (DPP). 

distribution and habitat. in Poland, spores of Ambispora gerdemannii were 
found in 19 samples of roots and rhizosphere soils of 14 species of uncultivated 
plants. none of the almost 1500 root and soil mixtures coming from cultivated sites 
of Poland contained spores of this fungus. 

the average abundance of Am. gerdemannii spores in the samples examined was 
4.7 and ranged from 1 to 29 in 100 g dry soil. the proportion of spores of this species 
in spore populations of all the arbuscular fungi recovered averaged 11.8% in a range 
of 2.1-66.7%. the average abundance of species of arbuscular fungi in samples in 
which spores of Am. gerdemannii occurred was 2.7 and ranged from 1 to 6 in 100 g 
dry soil.

the arbuscular fungi accompanying Am. gerdemannii in the field were Acau-
lospora bireticulata f.m. rothwell et trappe, A. capsicula Błaszk., A. koskei Błaszk., 
A. lacunosa J.B. morton, A. paulinae Błaszk., Ar. trappei (r.n. ames et linderman) 
J.B. morton et D. redecker, Entrophospora infrequens (i.r. hall) r.n. ames et 
r.w. schneid., G. caledonium (nicol. et Gerd.) trappe et Gerd., G. claroideum n.C. 
schenck et s.m. sm., G. constrictum trappe, G. deserticola trappe, Bloss et J.a. 
menge, G. ? etunicatum w.n. Becker et Gerd., G. fasciculatum (thaxt.) Gerd. et 
trappe emend. C. walker et koske, G. geosporum (nicol. et Gerd.) C. walker, G. 
macrocarpum tul. et C. tul., G. mosseae (nicol. et Gerd.) Gerd. et trappe, G. pan-
sihalos s.m. Berch et koske, an unrecognized Glomus sp., Pacispora scintillans (s.l. 
rose et trappe) sieverd. et oehl, Scutellospora dipurpurescens J.B. morton et ko-
ske, and S. pellucida (nicol. et n.C. schenck) C. walker et f.e. sanders.

although Am. gerdemannii probably has a worldwide distribution, this species 
has been infrequently reported. most reports of Am. gerdemannii come from the 
united states of america (allen, macmahon 1985; an et al. 1990, 1993; an, Guo 
and hendrix 1993a; an, Quo and hendrix 1993b; Bever et al. 1996; koske, Gemma 
and Jackson 1977; nicolson, schenck 1979; rose, Daniels and trappe 1979). ad-
ditionally, spores of this fungus have been isolated in Brazil (moreira-souza et al. 
2003), Colombia (Dodd et al. 1990), and australia (morton, redecker 2001). in 
southern Poland, turnau et al. (2001) recovered spores of a morphotype named 
Glomus sp. hm-Cl4 of molecular properties close (71%) to those of G. gerdeman-
nii, the basionym of Am. gerdemannii (walker et al. 2007). however, the authors did 



20 J. Błaszkowski et al. 

not show any morphological characters of the spores isolated and did not determine 
which of the two morphotypes of this fungus was found. 

myCorrhizal assoCiations. spores of Am. gerdemannii occurred among vesicu-
lar-arbuscular mycorrhizal roots of the plant species listed in the section “Collection 
examined”. additionally, they were recovered from some trap cultures established 
from mixtures of roots and rhizosphere soils of these plants and with P. lanceolata 
as the plant host. unfortunately, many attempts to produce one-species cultures of 
Am. gerdemannii failed. 

according to morton (2002) and morton & redecker (2001), mycorrhizae of 
Am. gerdemannii consisted of only arbuscules and intraradical hyphae; no vesicles 
were found. all the structures were patchily distributed along roots and stained 
weakly or not at all in trypan blue. Percentage mycorrhizal colonization always was 
very low, below 10%. 

notes. Ambispora gerdemannii has originally been described as Glomus gerde-
manii s.l. rose, B.a. Daniels et trappe from spores isolated from soils of Cascade 
range and siskiyou mountains of oregon, usa (rose et al. 1979). spain et al. 
(2006) transferred G. gerdemannii to the genus Appendicispora spain, oehl et siev-
erd. gen. nov., and walker et al. (2007) to the genus Ambispora C. walker, Vestberg 
et schuessler gen. nov. in the newly erected family Ambisporaceae C. walker, Vest-
berg et schuessler. the genus Appendicispora has been excluded because a nomen-
clatural error (walker et al. 2007). 

the distinctive morphological properties of Am. gerdemannii are the fragile bi-
layered inner wall 1 and the mode of differentiation of spores of this fungus. addi-
tionally, Am. gerdemannii is a dimorphic fungus producing two morphotypes, acau-
losporioid (as in Acaulospora spp.) and glomoid (as in Glomus spp.), a phenomenon 
rarely occurring in other species of arbuscular fungi. 

inner wall 1 of Am. gerdemannii resembles a hardened glass. in slightly crushed 
spores, linear cracks appear on the surface of this wall. however, in spores vigorously 
crushed, this wall almost always breaks into small pieces. another characteristic of 
this wall is its glittering when seen in a polarized light. 

when observed under a dissecting microscope, Am. gerdemannii spores may eas-
ily be confused with those of A. spinosa, A. thomii, Am. appendicula and Am. fennica. 
all the fungi form yellow brown and dull spores of a similar size range. 

spores of Am. appendicula, Am. fennica, and Am. gerdemannii differ mainly in 
the properties of layers of inner wall 1. in the latter two species, both layers of this 
wall are smooth on both sides (spain et al. 2006; walker et al. 2007). in contrast, in 
the former fungus, the lower surface of layer 1 is ornamented with hemispherical 
protuberances, which impress hemispherical concave depressions on the upper sur-
face of layer 2 during its differentiation (morton, redecker 2001; spain et al. 2006). 
additionally, in vigorously crushed spores, inner wall 1 of Am. fennica and Am. ger-
demannii usually disintegrates, and that of Am. appendicula remains its integrity. as 
concluded above (see comments on Am. fennica), Am. fennica and Am. gerdemannii 
probably are congeneric. 

the subcellular structure readily separating Am. gerdemannii from A. spinosa 
and A. thomii is the beaded outer layer and the flexible to plastic, dextrinoid in-
ner layer present in the innermost wall of spores of the latter two species (vs. no 
such structures have been found in spores of Ambispora spp.). additionally, in Am. 



 Ambispora gerdemannii and Glomus badium 21

gerdemannii the sporiferous saccule wall is continuous with spore wall layers 1–3 and 
layer 1 of inner wall 1, whereas in all known Acaulospora spp. the sporiferous sac-
cule wall is continuous with only spore wall layer 1. finally, only Am. gerdemannii is 
a dimorphic fungus, forming both acaulosporioid and glomoid spores. the glomoid 
morphotype of Am. gerdemannii has not so far been found in Poland and the only 
report of its existence is that of morton and redecker (2001).
Glomus badium oehl, redecker et sieverd.

spores occur in dense sporocarps in the soil (fig. 9) and on the surface of 
vesicular-arbuscular mycorrhizal roots. Sporocarps brownish orange (6C8) to red-
dish brown (8e8), mainly ovoid to irregular, 200-500 × 290-680 μm (fig. 9), some-
times globose to subglobose, (250-)298(-320) μm diam, with 4-43 spores, radially 
originating from a hyphal plexus (fig. 10) and separated by an interspore mycelium 
(figs 11 and 14) and occasionally by cystidium-like structures (fig. 12). Interspore 
mycelium consists of tightly interwoven, straight or branched, hyaline to pale orange 
(5a3) hyphae, (2.2-)5.8(-12.3) μm wide, with a wall (0.5-)1.1(-1.5) μm thick (figs 11 
and 14). Cystidium-like structures icicle-like, hyaline, 32.1-39.5 μm long, 9.6-12.0 μm 
wide at the base, with a wall (1.8-)2.0(-2.3) μm thick (fig. 12). Both the interspore 
mycelium and the cystidium-like structures branch out from the hyphal plexus. in-
side sporocarps frequently with sand grains and soil debris. 

spores formed blastically at the tip of hyphae developing from a hyphal plexus 
positioned in the centre of sporocarps (fig. 10). Hyphal plexus composed of thick-
walled, 6.9-10.3 μm thick, two-layered hyphae: a hyaline, evanescent, 0.5-0.8 μm 
thick outer layer, usually highly deteriorated and difficult to see in mature spores 
and pale orange (5a3) to brownish orange (6C8), permanent, (1.2-)2.3(-3.4) μm 
thick inner layer (fig. 12). 

Spores brownish orange (6C8) to reddish brown (8e8), usually ovoid, 35-55 × 
60-70 μm, rarely globose to subglobose, (35-)55(-65) μm, usually with one subtend-
ing hypha (figs 9, 10 and 14-16), occasionally with two. Subcellular spore structure 
consists of a spore wall comprising three layers (layers 1-3; figs 13 and 14). layer 1 
evanescent, hyaline to pale orange (5a3), (0.7-)2.0(-3.4) μm thick, frequently highly 
or completely sloughed in mature spores (figs 13 and 14). layer 2 laminate, brown-
ish orange (6C8) to reddish brown (8e8), (3.7-)4.5(-6.9) μm thick (figs 13 and 14). 
layer 3 flexible, pale yellow (4a3) to light brown (6D8), (0.5)1.7(-2.0) μm thick, 
usually tightly adherent to the lower surface of layer 2 (figs 13 and 14). Subtending 
hypha brownish orange (6C8) to reddish brown (8e8), straight or recurved, cylindri-
cal or slightly flared, rarely slightly constricted, (8.1-)9.5(-10.0) μm wide at the spore 
base (figs 10, 15 and 16). wall of subtending hypha brownish orange (6C8) to red-
dish brown (8e8), (2.9-)4.4(-7.4) μm thick at the spore base, continuous with spore 
wall layers 1 and 2 (fig. 15). Pore 1.0-1.7 μm wide at the spore base, occluded by 
spore wall layer 3 inserted in the lumen of the subtending hypha up to 14.0 μm below 
the spore base (fig. 14) or/and by thickening of spore wall layer 2 and wall layer 2 of 
subtending hypha, in which a hyphal plug occasionally forms (fig. 16). 

ColleCtions examined. Poland. szczecin (53°26’n, 14°35’e), under Glycine max (l.) merr., 5 sept. 
1985, Błaszkowski J. 2644-2646 (DPP); Przelewice, among roots of Malus × purpurea rehder, 16 July 1985, 
Błaszkowski J. 2647-2649 (DPP); Pomierzyn (53°20’n, 15°51’e), in the roots zone of Lupinus luteus l., 9 
aug. 1985, Błaszkowski J. 2650-2652 (DPP); szczecin, in the rhizosphere soil of Anthriscus sylvestris (l.) 
hoffm., 18 oct. 1985, Błaszkowski J. 2653 (DPP); kołbacz (53o18’n, 14o49’e), under Trifolium pratense 



22 J. Błaszkowski et al. 

l., 4 aug. 1985, Błaszkowski J. 2654-2655 (DPP); szczecin, from under Allium schoenoprasum l., 3 sept. 
1985, Błaszk. J. s.n. (DPP); międzyzdroje (53°56’n, 14°26’e), among roots of Avena sativa l., 14 July 1985, 
Błaszk. J. s.n. (DPP); Przelewice, in the roots zone of Acer palamatum thunb., 15 may 1985, Błaszk. J. s.n. 
(DPP); Żelistrzewo (54°41’n, 18°27’e), under Triticum aestivum l., 24 aug. 1985, Błaszk. J. s.n. (DPP); 
hel (54o36’n, 18o49’e), in the rhizosphere soil of Thuja occidentalis, 21 aug. 1985, Błaszk. J. s.n. (DPP); 
Jarosławki (53°32’n, 15°01’e), under Zea mays l., 25 July 1985, Błaszk. J. s.n. (DPP); Żelistrzewo, among 
roots of Ficaria verna huds., 3 april 1989, Błaszk. J. s.n. (DPP); hel, in the root zone of T. occidentalis, 
28 sept. 1988, Błaszk. J. s.n. (DPP); szczecin, under T. occidentalis, 18 oct. 1985, Błaszk. J. s.n. (DPP); 
Żelistrzewo, near roots of Festuca ovina l., 25 June 1986, Błaszk. J. s.n. (DPP); Jastrzębia Góra (54o50’n, 
18o18’e), under Crataegus monogyna Jacq., 30 oct. 1987, Błaszk. J. s.n. (DPP); Żelistrzewo, from under 
Rubus idaeus l., 22 aug. 1987, Błaszk. J. s.n. (DPP); Płoty (53°48’n, 15°16’e), among roots of Agrostis 
stolonifera l., 22 sept. 1987, Błaszk. J. s.n. (DPP); Jastrzębia Góra, in the rhizosphere soil of J. communis 
l., Błaszk. J. s.n. (DPP); szczecin, under Heracleum sphondylium l., 22 oct. 1987, Błaszk. J. s.n. (DPP); 
osłonino (54°42’n, 18°28’e), in the root zone of Helictotrichon pubescens (huds.) Pilg., 22 June 1988, 
Błaszk. J. s.n. (DPP); Chałupy, among roots of Festuca arundinacea schreb., 28 sept. 1988, Błaszk. J. 
s.n. (DPP); kuźnica (54°41’n, 18°34’e), associated with roots of Ammophila arenaria (l.) link, 28 sept. 
1988, Błaszk. J. s.n. (DPP); władysławowo (54°47’n, 18°26’e), on roots of Rosa rugosa thunb., 7 July 
1989, Błaszk. J. s.n. (DPP); Bolesław (50°00’n, 18°12’e), under an unrecognized grass, 17 sept. 1989, 
Błaszk. J. s.n. (DPP); nowy ujków (50°18’n, 19°26’e), among roots of Agropyron repens (l.) P. Beauv., 17 
sept. 1989, Błaszk. J. s.n. (DPP); leszna Góra (49°42’n, 18°43’e), associated with roots of C. monogyna, 
8 sept. 1989, Błaszk. J. s.n. (DPP); Pieski (52°25’n, 15°26’e), under Hordeum vulgare l., 12 aug. 2004, 
Błaszk. J. s.n. (DPP); Połupin (52°03’n, 15°06’e), from under Rumex acetosella l., 12 aug. 2004, Błaszk. 
J. s.n. (DPP); Jemiołów (52°21’n, 15°16’e), in the root zone of Cirsium arvense (l.) scop., 13 aug. 2004, 
Błaszk. J. s.n. (DPP); trzciel (52°22’n, 15°52’e), among roots of Corynephorus canescens (l.) P. Beauv., 
15 aug. 2004, Błaszk. J. s.n. (DPP); łagów (51°59’n, 15°16’e), under Silene latifolia Poir. ssp. alba (mill.) 
Greuter et Burdet, 13 aug. 2004, Błaszk. J. s.n. (DPP); Jemiołów, among roots of H. perforatum, 13 aug. 
2004, Błaszk. J. s.n. (DPP); zarzyń (52°23’n, 15°25’e), from under E. arvense, 13 aug. 2004, Błaszk. J. s.n. 
(DPP); trzciel, in the rhizosphere soil of Juncus effusus l., 15 aug. 2004, Błaszk. J. s.n. (DPP). 

distribution and habitat. in Poland, G. badium was recovered from 39 field-
collected mixtures of roots and rhizosphere soils. of them, 15 came from under nine 
species of cultivated plants, and the others represented 20 species of wild plants.

the spore abundance of G. badium was much higher among roots of wild plants 
(av. 126.3; range 1-850 in 100 g dry soil) than cultivated plants (av. 5.2; range 1-20 
in 100 g dry soil). the proportion of spores of this fungus in spore populations of all 
arbuscular fungi isolated also was higher in the root zone of wild plants (av. 45.2%; 
range 0.9-100%) than cultivated ones (av. 10.8%; range 0.9-40.7%). the species 
abundance in the root and soil samples taken from under cultivated plants averaged 
5.0 with a range of 4-7 in 100 g dry soil, and that under wild plants averaged 3.7 and 
ranged from 1 to 9 in 100 g dry soil. 

the arbuscular fungi co-occurring with G. badium were A. polonica Błaszk., A. 
capsicula, A. cavernata Błaszk., A. gedanensis Błaszk., A. lacunosa, A. mellea Spain 
et n.C. schenck, A. paulinae, an unrecognized Acaulospora sp., G. aggregatum n.C. 
schenck et s.m. sm. emend. koske, G. caledonium, G. constrictum, G. deserticola, 
G. ? etunicatum, G. fasciculatum, G. fuegianum, G. geosporum, G. microcarpum tul. 
et C. tul., G. macrocarpum, G. mosseae, unrecognized Glomus spp., Paraglomus 
occultum (C. walker) J.B. morton et D. redecker, Scutellospora armeniaca Błaszk., 
and Scutellospora dipurpurescens.

apart from Poland, G. badium has been found among roots of grasses and grass-
land plants growing in soils of ph 6-8 and located in Germany, france, switzerland, 
and italy (oehl et al. 2005). 



 Ambispora gerdemannii and Glomus badium 23

myCorrhizal assoCiations. the sporocarps of G. badium found by the authors 
of this paper were formed among and occasionally on vesicular-arbuscular mycor-
rhizal roots of the plant species listed in the section “Collection examined”. in trap 
cultures with root and rhizosphere soil mixtures of the plant species sampled, G. 
badium rarely produced spores. all one-species cultures of this fungus established 
were unsuccessful. oehl et al. (2005) also failed to obtain G. badium in one-species 
cultures and, hence, properties of mycorrhizae of this fungus remain unknown. how-
ever, phylogenetic molecular analyses showed G. badium to be a member of Glomus 
Group a (oehl et al. 2005) sensu schwarzott, walker and schüßler (2001), compris-
ing fungi known to form vesicular-arbuscular mycorrhizae (Błaszkowski 2003).

the most distinguishing characters of G. badium are its small sporocarps lacking 
a peridium and composed of many, brownish orange to reddish brown, relatively small 
spores (fig. 9). the innermost flexible to semi-flexible and coloured layer of the three-
layered spore wall also is a diagnostic property of this species (figs 13 and 14). 

Glomus badium probably forms spores only in multispored sporocarps, and sin-
gle spores occasionally recovered from field-collected soil samples represented their 
fragments. examination of the ontogenesis of this species is needed to confirm this 
supposition. unfortunately, all attempts to produce one-species cultures of G. ba-
dium made by the authors of this paper and by oehl et al. (2005) failed.

the interspore mycelium of the specimens of G. badium found by the authors of 
this paper morphologically corresponds to that characterized by oehl et al. (2005). 
however, the original description of this fungus does not inform of the cystidium-
like structures occurring between spores of the Polish sporocarps of this fungus. the 
function of the cystidia-like structures in sporocarps of G. badium probably is similar 
to that of cystida of agaricales, in which they appear to serve as spacers between 
basidia (ulloa, hanlin 2000). 

of the three wall layers of spores of G. badium, the two outer ones are typical 
of most species of the genus Glomus, in which the outermost layer sloughs with age 
and adheres to a laminate structural layer (figs 13 and 14). spore wall layer 3 of G. 
badium is thin, pale yellow (4a3) to light brown (6D8), and usually tightly adheres 
to the lower surface of the brownish orange (6C8) to reddish brown (8e8) layer 2 in 
even vigorously crushed spores (figs 13 and 14). hence, it is difficult to see, especial-
ly in young and freshly matured spores. in older spores, this layer usually is slightly 
thicker and more frequently separates from the middle laminate layer. additionally, 
this layer is most visible at the spore base where it forms a straight or curved septum 
of the subtending hypha continuous with its part adherent to the laminate spore wall 
layer 2 (fig. 14).

Apart from G. badium, species of the genus Glomus forming small and compact 
sporocarps with small, brownish orange to reddish brown spores are G. cuneatum 
mcGee et Cooper, G. fuegianum (speg.) trappe et Gerd., G. invermaium i.r. hall, 
and G. rubiforme (Gerd. et trappe) r.t. almeida et n.C. schenck. Compared with 
G. badium, sporocarps of G. cuneatum are much larger (2-12 mm vs. 200-500 × 290-
680 μm in G. badium) and have a peridium (fig. 9; vs. no peridium in G. badium; 
mcGee and trappe 2002). additionally, the spore wall of the latter species consists 
of only one laminate layer lightening from black to hyaline towards their inside, 
whereas the spore wall of the former fungus comprises three layers, of which the 
laminate layer is dark- and uniform-coloured (figs 10, 12 and 16).



24 J. Błaszkowski et al. 

according to thaxter (1922), G. fuegianum spores coming from spegazzini’s origi-
nal collection were reddish brown as are those of G. badium. in contrast, all G. fue-
gianum spores found by one of the authors (J. B.) of this paper in Poland, those loaned 
from kew, united kingdom (Błaszkowski, madej and tadych 1998), and those re-
vealed in australia by mcGee and trappe (2002) were pale yellow to yellow brown. 
moreover, the spores were frequently surrounded by branched and convoluted hy-
phae (Błaszkowski 2003) that never occur on G. badium spores (Błaszkowski, pers. 
observ.; oehl et al. 2005). finally, the radial arrangement of spores in sporocarps of 
G. fuegianum is regular, and irregular in G. badium sporocarps.

Glomus badium differs from G. invermaium in the formation of smaller 
(200-500 × 290-680 μm vs. up to 1 mm across) and more compact sporocarps with 
regularly distributed spores (fig. 9; vs. loose sporocarps with randomly distributed 
spores in G. invermaium; Błaszkowski, pers. observ.; hall 1977). other differences 
are the number and the phenotypic properties of the spore wall layers of these fungi. 
the spore wall of G. badium comprises three layers, of which the outermost one 
sloughs with age (figs 13 and 14). in contrast, the outermost spore wall layer of 
G. invermaium spores is persistent and the spore wall of this species lacks spore wall 
layer 3 of G. badium.

the main difference between G. badium and G. rubiforme resides in the wall 
structure of their spores. the spore wall of G. rubiforme comprises only two layers 
similar in colour and phenotypic properties to layers 1 and 2 of the spore wall of 
G. badium (Błaszkowski 2003; Gerdemann, trappe 1974).

Acknowledgment. this study was supported in part by the Committee of scientific researches, a grant 
no. 2 Po4C 041 28 and 164/n-Cost/2008/0.

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Ambispora gerdemannii and Glomus badium, dwa gatunki grzybów arbuskularnych 
(Glomeromycota) nowe odpowiednio dla europy i Polski

streszczenie

opisano i zilustrowano cechy morfologiczne zarodników oraz sporokarpów i zarodników 
odpowiednio Ambispora gerdemannii i Glomus badium, grzybów arbuskularnych z gromady 
Glomeromycota. Ponadto przedstawiono poznane rozmieszczenie tych gatunków zarówno 
w Polsce, jak i innych regionach świata. Ambispora gerdemannii nie była dotychczas notowana 
w europie, a G. badium jest nowym grzybem dla Polski.


		2014-01-01T11:50:07+0100
	Polish Botanical Society