BIOTROPIA No


BIOTROPIA No. 12, 1999 : 59 - 77 

THE EFFECTIVENESS OF SOME ECTOMYCORRHIZAL FUNGI IN 
ALGINATE BEADS IN PROMOTING THE GROWTH OF SEVERAL 

DIPTEROCARP SEEDLINGS 

SUPRIYANTO  

SEAMEO B1OTROP, P.O Box 116, Bogor 16001, Indonesia 

ABSTRACT 

The effectiveness of six species of ectomycorrhizal fungi (Scleroderma columnare, S.dictyosporum, 
Laccaria toccata, Rhizopogon luteolus, Amanita umbronata and Descomyces sp.) in alginate beads in 
promoting the growth of four species of dipterocarp seedlings (Shorea pinanga, S.leprosula, S.ovalis and 
Hopea odorata) were studied. Different sodium alginate concentrations of 5 g, 10 g, 15 g and 20 g/L were 
tested to find out the best bead's elasticity and spore germination. 

Seedling height, Relative Field Mycorrhizal Dependency, percentage of mycorrhizal colonization, 
nutrient absorption, and the formation of Hartig's net and mantle structure of dipterocarp seedlings were 
observed 4 months after inoculation. 

The best elasticity of alginate beads was found in the concentration of sodium alginate of 15 g/L. 
The best growth increment was found in Hopea odorata inoculated with Amanita umbronata (126.60 %) 
followed by Shorea pinanga inoculated with Descomyces sp. (27.10%), Shorea ovalis inoculated with 
Amanita umbronata (26.90 %) and Shorea leprosula inoculated with Descomyces sp. (24.20 %) over the 
control. The highest Relative Field Mycorrhizal Dependency was found in Hopea odorata followed by 
Shorea ovalis, S. pinanga and S. leprosula. 

The highest mycorrhizal colonization was obtained in Shorea pinanga inoculated with Descomyces 
sp. (75%), while inoculation with Amanita umbronata on S.leprosula, S.ovalis and Hopea odorata 
increased mycorrhizal colonization i.e. 64.5 %, 52.5%, and 46.2 %, respectively. 

Hartig's net and mantle structures were well formed in Shorea leprosula as well as S.ovalis seedlings 
with all mycorrhizal fungi tested, while in S.pinanga seedlings these structures were only well formed with 
Descomyces sp. 

There is no clear difference in P levels in the leaves following inoculation as compared to the controls. 

Key words: Mycorrhizas/Alginate beads/Scleroderma columnare/Scleroderma dictyosporumlLaccaria 
laccatalRhizopogon luteoluslAmanita umbronatalDescomyces sp./Growth/Dipterocarpace-
ae/Seedlings. 

INTRODUCTION 

Background 

Industrial Forest Plantation (IFF) is one of the Government Programs to 
improve the reduced forest productivity due to logging activities (logged-over areas) 
and deforestation (critical lands). During the period of the Fourth to Sixth Five-year 
Development Plan of the Government of Indonesia, the area of IFP was projected to 
be 4.6 million hectares (Departemen Kehutanan 1994). High quality seedlings to 
replant these areas are needed. Dipterocarp species make up one of the recommended 
species for sawn-timber production. Dipterocarp is an important timber species in 
Southeast Asian Countries (PROSEA 1994). Seventy five percent of Indonesian 

59 



BIOTROPIA No. 12, 1999 

wood trading comes from dipterocarp species. Currently, the rate of logging is 
higher than the rate of replanting. There are some problems in planting dipterocarp 
species. Among these are the irregular flowering season, recalcitrant seeds, and the 
need of mycorrhizae for promoting their growth during the seedling stage. 

Mycorrhizal research in Indonesia has been promoted by the Government, 
because of its beneficial contribution to increase the quality of seedlings via growth 
acceleration (Marx 1973; Supriyanto et al. 1992), to control root pathogenic 
microorganisms (Marx 1973), to improve soil structure (De la Cruz 1982), to 
improve rooting system due to hormone production (Gay and Debaud 1987), to 
increase nutrient and water uptake (Boyle et al. 1987), to increase drought resistance 
(Boyle et al. 1987; Supriyanto et al. 1992), and to increase the survival rate and 
accelerate the xylem formation of seedlings obtained by tissue culture techniques 
(Supriyanto 1989; and Chang 1993). 

Inoculum improvements of the potential ectomycorrhizal fungi have been 
achieved in some species by single spore culture, cell fusion (mating type) and 
protoplast culture. These techniques can be used for mass production of vegetative 
inoculum (Fortin et al. 1988). 

The inoculum can be packed in several ways such as tablet, capsule, spore 
powder or mycelium suspension (Supriyanto et al. 1992) and in alginate beads 
(Supriyanto et al. 1994; Supriyanto 1996). There are some advantages and 
disadvantages for each type of packaging system. Alginate beads are simple, easily 
stored, free from climatic influences, inexpensive and are available at any time. 

Recent technological improvements of the vegetative inoculum production 
promote the use of the inoculum packaging system. It is important to evaluate the 
effectiveness of selected tropical mycorrhizal fungi packed in alginate beads to 
promote the growth of dipterocarp species recommended for the Industrial Forest 
Plantation Program. 

Objective 

The objective of the research was to compare the effectiveness of alginate 
inoculum of six species of ectomycorrhizal fungi on the growth of four species of 
dipterocarp seedlings. 

MATERIALS AND METHODS 

Seed Germination 

Dipterocarp seeds (S.pinanga, S.leprosula, S.ovalis, H.odoratd) were collected 
from Dipterocarp Experimental Areas, Jasinga, Forest Research Institute and were 
dipped in Dithane M-45 at 1% concentration for 10 minutes to eliminate the 
pathogenic fungi. Seeds were germinated in sterilized sand medium. Germination 
and transplanting media were autoclaved at 1.5 bar, 120°C for 30 minutes. 
Dipterocarp seedlings, two weeks old, were transplanted into poly-bags containing 
sterilized sand: soil: compost (1:1:1). 

 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

Aiginate Bead Elasticity 

Ectomycorrhizal fungi of Scleroderma columnare, Laccaria laccata, Amanita 
umbronata, Descomyces sp. were collected from dipterocarp plantation. Sclero-
derma dictyosporum was collected from Pinus merkusii plantation, while Rhizo-
pogon luteolus was collected from Eucalyptus urophylla plantation. 

The spores of ectomycorrhizal fungi were packed in alginate beads based on Le 
Tacon et al. method (1985) modified by Supriyanto et al. (1994). The elasticity tests 
of alginate beads were done in different concentrations of sodium alginate (5, 10, 15, 
20 g/L). An amount of 2 g of ectomycorrhizal fungi spores were extracted from 
mature fruit bodies and diluted in each different concentration of sodium alginate (an 
algal extract). Spore suspension was trapped in sodium alginate to form beads in 
0.7M calcium chlorite solution. The alginate bead elasticity was classified into very 
soft, soft, elastic and hard by pressing the beads in between two fingers. To evaluate 
the spore viability in different concentrations of sodium alginate, 10 beads were 
placed in a petri dish containing Modified Melin-Nokran medium. Five replicates 
were used for the evaluation of each sodium alginate concentration. Germination 
percentage of the spores in alginate beads was recorded. 

Inoculation Technique 

Three-week old dipterocarp seedlings (one week after transplanting) were then 
inoculated with 5 alginate beads at a concentration of 15g/L sodium alginate. A 
pipette was used to aspire the alginate beads. The alginate beads were then injected 
into transplanting media close to the rooting system (at a depth of 2 cm). Eight 
replicates were used for each treatment. 

Parameters 

Mycorrhizal seedlings were evaluated 4 months after inoculation on the basis of 
several parameters to determine the effectiveness of selected mycorrhizal fungi as 
follows: 
                                                               Ht- He 
High growth increment (HGI, %) = —————  x 100 %, where: 
He 
Ht = Height of mycorrhizal seedlings, He = Height of non-mycorrhizal seedlings 
(control) 

Relative Field Mycorrhizal Dependency / RFMD (Plenchette et al. 1983 in Bagyaraj 
1994). 

                     DWt-DWc 
RFMD (%) = ———————— x 100 %, where : DWc 

 

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BlOTROPlA No. 12,1999 

DWt = Dry weight of inoculated seedlings (treatment),  DWc : Dry weight of non-
inoculated seedlings (control) 

Seedlings were dried in an oven at 70°C for 48 hours and their dry weights were 
determined. The leaf dry weights were separated for nutrient content analysis. 

                                                                             Number of colonized roots 
Percentage of colonization (Fortinef a/. 1982)= ——————————————xlOO% 
                                                                           Total number of root samples 

The colonized roots were determined by the presence of hyphae enveloping the 
roots (external hyphae). 

Structural analysis of mycorrhizal and non-mycorrhizal roots was done to 
observe the presence of Mantle and Hartig's net formation based on the SASS 
microtechniques method (1958) in Berlyn and Miksche (1976). Toluedine blue 0 of 
0.1% was used for root staining. Toluedine blue 0 stains specifically the mycorrhizal 
hyphae either mantle or Hartig's net in blue - pinkish color. The presence of Mantle 
(M), Hartig's Net (HN) or none in the rooting system were used to determine the 
compatibility of inoculated mycorrhizal fungi and host plant. It was classified into 
semi-compatible (Mantle only), compatible (Hartig's net and Mantle) or incompatible 
(no Mantle and no Hartig's net). Good formation of Mantle and Hartig's net will 
influence the effectiveness of mycorrhizal fungi in nutrient and water absorption. The 
criteria of mantle formation are as follows: - (negative) for no mantle formation, + 
(positive) for one layer or poor formation, ++ for two layers or good formation and +-
H- for three layers or best formation. The criteria of Hartig's net formation are as 
follows: - (negative) for no Hartig's-net formation, + (positive) for one series or poor 
formation, ++ for two series or good formation, +++ for three series or best formation. 

Leaf content of N, P, K, Ca, Fe, Mg were used as a nutrient parameter. All of the 
seedlings were dried at 70 ° C for 48 hours for nutrient analysis. Dried leaves were 
powdered and 250 mg leaf powder was digested with concentrated H2SO4 and 30% 
H2O2. The leaf nutrient content was analyzed as follows: 

Nitrogen 

Nitrogen content was analyzed using the titration method. To 20 ml of filtered 
solution in the nitrogen distillate apparatus was added 15 ml of 30% NaOH. Nitrogen 
distillation was done for 10 minutes. An amount of 20 ml of 1% boric acid added to 
the distillate solution were combined with 3 drops of BCRM (brom cresol green and 
red methyl) indicator. Titration of the ammonium solution was done using 0.05N 
H2SO4. 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanlo 

Phosphate 

Phosphate content was determined spectrophotometrically at X 693 nm. Phos-
phate solutions of 0, 0.5, 1.0, 2.0, 3.0, 4.0, 5.0 ppm were used as standards from 
which the phosphate content was determined. 

Iron 

The wet destruction method of powdered leaf was done using HNO3 + HC1O4 + 
HjSC^. The iron was analyzed spectrophotometrically at A. 508 nm. An amount of 0.25 
ml of metal reduction solution was added to the destructed solution thoroughly to 
homogenize the solution. An amount of 0.5 ml of orthophenontroline and 7 ml of 
sodium citrate were combined. Standardized iron solutions of 0, 1.0, 2.0, 4.0, 6.0 and 
8.0 ppm using (NH4)2Fe(SO4)2 . 6 H2O were used. 

Potassium, Calcium and Magnesium 

Atomic absorption spectrophotometry was used to determine the potassium, 
calcium and magnesium content. Standardized solutions of potassium and calcium each 
of 0, 2.5, 5.0, 10.0, 15.0, 20.0 and 25 ppm were prepared and used to determine 
potassium and calcium content. To determine magnesium content, standardized 
solutions of 5 ml magnesium were made from MgSO4 .7 H2O, i.e. 0, 2.5, 5.0 ppm to 
which 5 ml LaCl3 containing 4000 ppm La were added. 

R E S U L T S  

Alginate Bead Elasticity 

The spore suspension was trapped using sodium alginate and formed to beads in 
calcium chloride solution. Bead elasticity depended on the concentration of sodium 
alginate used. The best concentration is determined by the criteria for bead elasticity 
and germination percentage of trapped spores. This was 15g/L sodium alginate with 
the average spore germination percentage of 77% (Table 1). The concentration of 
sodium alginate of 20 g/L produced harder beads but the germination percentage of 
spores trapped in alginate beads decreased. Concentrations of sodium alginate lower 
than 15 g/L produced soft or very soft beads and can easily be dried by airflow even 
when its spore germination was higher. The concentration of sodium alginate at 15 
g/L will be used for inoculum packaging system at SEAMEO BIOTROP. This 
packaging system is easily handled, with high productivity and high inoculum 
viability. Although Le Tacon et al. (1985) used the sodium alginate at the 
concentration of 10 g/L, vegetative mycelia were used instead of spores. 

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BIOTROPIA No. 12, 1999 

Table 1. Degree of Bead Elasticity and Germination Percentage of Scleroderma columnare Ecto-
mycorrhizal Fungi at Different Concentrations of Sodium Alginate. 

No. 5g/LS.A. 
VS        %G

l O g / L S.A 
S            %G 

15 g/L S.A. 
ELS           % G

20 g/L S.A.  
H            %G 

1 
2 
3 
4 
5 

VS
VS 
VS 
VS 
VS

70
85 
80 

75 8 
0

S
S 
S 
S 
S

75 
75 
80 
90 
80 

ELS
ELS 
ELS 
ELS 
ELS

80
75 
80 
75 
75

H
H 
H 
H 
H 

60 
65 
60 
50 
60 

Average VS 78 S 80 ELS 77 H 59 

Note:   VS: Very Soft, S: Soft, ELS: Elastic, H: Harder, % C: Germination Percentage, S.A.: Sodium 
Alginate. 

High Growth Increment (HGI) 

The percentage of high growth increment (HGI) of mycorrhizal seedlings over 
the control (not inoculated) is presented in Table 2. The best HGI was obtained at 
Hopea odorata seedlings inoculated with Amanita umbronata (126.60%). All of the 
mycorrhizal fungi stimulated the growth of Hopea odorata seedlings, ranging from 
40.6 % to 126.60 % and the growth of Shorea pinanga ranging from 5.70 % to 
27.10 %. The HGI of Shorea pinanga and S. leprosula was promoted by inoculation 
with Descomyces sp., whereas the HGI of Shorea ovalis and Hopea odorata 
was promoted best by Amanita umbronata. Scleroderma columnare, Rhizopogon 
luteolus and Laccaria laccata were not able to stimulate the HGI of Shorea 
leprosula, and Laccaria laccata was not able to stimulate the HGI of Shorea ovalis. 
Scleroderma dictyosporum consistently stimulated the HGI of four dipterocarp 
seedlings tested, ranging from 10.30 % to 75.00 %. 

Table 2. Percentage of High Growth Increment Over the Control of 4-Month Old Dipterocarp Seedlings 
Inoculated with Different Species of Ectomycorrhizal Fungi. 

Species of Ectomycorrhizal FungiDipterocarp 
Species Sd Sc R LL AM DE 

Shorea pinanga 10.30 5.70 12.90 13.60 15.50 27.10 
Shorea leprosula 11.10 -3.00 -13.70 -18.00 23.80 24.20 
Shorea ovalis 18.30 11.60 14.10 -10.80 26.90 24.10 
Hopea odorata 75.00 54.70 49.60 40.60 126.60 84.40 
Note : Sd: Scleroderma dictyosporum, Sc: Scleroderma columnare, R: Rhizopogon luteolus, LL: Laccaria 

laccata, AM: Amanita umbronata, DE: Descomyces sp. 

The growth response of each dipterocarp seedling inoculated with different 
mycorrhizal fungi can be seen in Figure 1 (S. pinanga), Figures 4 and 6 (S. 
leprosula). 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

 

 

 

 

 

 

 

 

 

 

 

 

Figure 1: Shorea pinanga seeds (A, x 0.1), alginate beads (B, x 0.18), mycorrhizal seedlings (Sc, Sd, R, 
LL, AM, DE) and non- mycorrhizal seedlings (c) (C, x 0.06) and the colonization of 
Scleroderma columnare mycorrhizal fungi at the rooting system of Shorea pinanga seedling 
(D, x 0.2). 

Relative Field Mycorrhizal Dependency (RFMD) 

The influence of mycorrhizal inoculation can also be determined from their 
Relative Field Mycorrhizal Dependency (RFMD). RFMD is the dependency of a 
plant species on the mycorrhizal fungi at a given soil fertility. RFMD is determined on 
the dry weight of mycorrhizal seedlings. It is important because dry weights may 
reflect the efficiency of physiological processes due to the mycorrhizal inoculation 
and photosynthetic activity. 

Regarding the RFMD value (Table 3), Hopea odorata was very dependent on 
the inoculated mycorrhizal fungi, ranging from 82.45% to 416.10%. Shorea pinanga 
was dependent on Scleroderma dictyosporum (17.87%), Rhizopogon luteolus (8.6%), 
Laccaria laccata (27.82%), Amanita umbronata (16.82%) and Descomyces sp. 
(34.89%). Shorea leprosula was dependent on Descomyces sp. (34.32%) and on 
Amanita umbronata (27.86%), while Shorea ovalis was dependent on all of 

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BIOTROPIA No. 12, 1999 

inoculated mycorrhizal fungi ranging from 32.10 % to 88.20 %. Since some values 
are negative, it is possible that in this stage of colonization, mycorrhizal fungi 
consumed a high amount of carbohydrate for their energy and development. 
Generally, those carbohydrates are translocated for plant organ development. 

Table 3. Percent Relative Field Mycorrhizal Dependency Over the Controls (not Inoculated) of 4-Month 
Old Dipterocarp Seedlings Inoculated with Different Species of Ectomycorrhizal Fungi. 

Ectomycorrhizal FungiDipterocarp 
Species Sd Sc R LL AM DE 

Shorea pinanga 
Shorea leprosula 
Shorea ovalis Hopea 
odorata 

17.87
-25.10 
43.50 
394.20 

-12.28 
-15.30 
32.10 
221.10 

8.60
-33.90 
32.50 
128.10 

27.82
-225.30 7 

3.20 
82.45 

16.82
27.86 
88.20 
416.10 

34.89 
34.32 
63.20 

321.40 

Note : Sd : Scleroderma dictyosporum, Sc: Scleroderma columnare, R: Rhizopogon luteolus, LL: Laccaria 
laccata, AM: Amanita umbronata, DE: Descomyces sp. 

Percentage of Mycorrhizal Colonization 

Percentage of mycorrhizal colonization is defined as the ability of inoculated 
mycorrhizal fungi to form a mantle sheet and Hartig's net in the rooting system of 
certain host-plants. The presence of the mantle sheet can be observed by macroscopic or 
microscopic observation (external hyphae), while the presence of Hartig's net can be 
observed by a microscope (internal hyphae). The presence of mantle and Hartig's net 
in the rooting system explains the compatibility status between host plant and 
inoculated mycorrhizal fungi. Technically, the percentage of mycorrhizal 
colonization is obtained from the hyphal extension that can be observed visually, 
while the Hartig's net structure must be observed using microscopic magnification. 

The extent of mycorrhizal colonization of inoculated mycorrhizal fungi on four 
species of dipterocarp seedlings is shown in Table 4. The extent of mycorrhizal 
colonization is classified in five categories: excellent (75 - 100%), good (50 - 74%), 
moderate (24 - 40%), poor. (1 - 24%) (Marx and Bryan 1969). Based on this 
classification, the colonization by Scleroderma dictyosporum, S. columnare, 
Rhizopogon luteolus, Laccaria laccata, Amanita umbronata and Descomyces sp. are 

Table 4. Percentage of Mycorrhizal Colonization in the Root System of 4-Month Old Seedlings of Shorea 
pinanga, Shorea leprosula, Shorea ovalis and Hopea odorata. 

Mycorrhizal colonization for each mycorrhizal fungus Dipterocarp
Seedlings Sd. Sc. R LL AM DE 

Shorea pinanga 
Shorea leprosula 
Shorea ovalis Hopea 
odorata 

51.87 
63.00 
43.10 
37.50 

,54.37 
41.50 
49.40 
45.00 

64.37
39.00 
50.00 
46.20 

66.26 
42.50 
52.70 
30.70 

67.50 
64.50 

52.50 46.20 
 

75.00  . 
55.50 
44.00 
37.50 

Note : C: Control, Sd : Scleroderma dictyopsorum, Sc: Scleroderma columnare, R: Rhizopogon luteolus, 
LL: Laccaria laccata, AM: Amanita umbronata, DE: Descomyces sp. 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

moderate and good (30.70% to 75.00 %). Excellent mycorrhizal colonization was 
found in Shorea pinanga inoculated with Descomyces sp. 

The ability of Scleroderma dictyopsorum, S. columnare, Rhizopogon luteolus, 
Laccaha laccata, Amanita umbronata and Descomyces sp. to form the Hartig's net 
and mantle structure is shown in Table 5. Mycorrhizal colonization in Shorea 
pinanga and S. leprosula seedlings were generally classified in term of good and best 
formation, while S. ovalis and Hopea odorata were classified as poor. 

Table 5. The Presence of Mantle and Hartig's net in the Root System of Mycorrhizal and Non-mycorrhizal 
Seedlings of 4-Month Old Seedlings of Shorea pinanga, S. leprosula, S. ovalis and Hopea 
odorata. 

 

 

 

 

 

 

 

 

 

 

Note: - : no formation, + : poor formation, -H-: good formation, +++ : best formation. 
C: Control, Sd : Scleroderma dictyosporum, Sc: Scleroderma columnare, R: Rhizopogon luteolus, 
LL: Laccaria laccata, AM: Amanita umbronata, DE: Descomyces sp. 

The extent of mycorrhizal colonization of the inoculated mycorrhizal fungi in 
dipterocarp seedlings is shown in Figure 2 (S. pinanga), Figures 5 and 6 (S. 
leprosula), Figure 7a, 7b (S. ovalis). The transversal section showing the mantle and 
Hartig's net formation in each host plant is shown in Figure 3 (S. pinanga), Figure 8 (S. 
ovalis). 

Leaf Nutrient Content 

Nutrient concentration in the leaves of S.pinanga, S. leprosula, S. ovalis and 
H. odorata is presented in Table 6. Effect of mycorrhizal inoculation on the leaf 
nutrient content was obtained by comparing the nutrient content of mycorrhizal and 
non-mycorrhizal seedlings. Table 6 shows that the increment of leaf nutrient content 
varied depending on the host plant species and the inoculated mycorrhizal fungi. 

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BIOTROPIA No. 12, 1999 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Figure 2: Non-mycorrhizal and mycorrhizal root system of Shorea pinanga. 
A: Non-mycorrhizal root system (x 10), B: Root system inoculated with S.columnare (x4), C: 
Root system inoculated with S.dictyosporum (x 5), D: Root system inoculated with L laccata (x 5), 
E: Root system inoculated with A. .umbronata (x 5), F: Root system inoculated with Descomyces 
sp. (x 5). 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads- Supriyanto 

 
Figure 3 : Transversal section of Shorea pinanga mycorrhizal roots inoculated with S.columnare (B, x  

400), A. umbronata (C, x 400), Rhizopogon luteolus (D, x 400), Descomyces sp. (E, x 400) and 
Non-mycorrhizal roots (A, x 400). CC = Cortical cells, REEC= Radially elongated epidermis cells, 
M= Mantle, HN= Hartig's net. 

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BIOTROPIA No. 12, 1999 

 
Figure 4 : The growth of non-mycorrhizal seedling (A,c) and mycorrhizal seedlings (Sd: S.dictyosporum, 

Sc: S.columnare, R: R. luteolus, LL: L.laccata, AM: A.umbronata, DE: Descomyces sp.) of 4- 
month old Shorea leprosula (A, x 0.07) and the colonization of Rhizopogon luteolus (B x 0 3 
C,xl5). ' ' ' 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

 
Figure 5 : The development and colonization of mycorrhizal fungi hyphae at the root system of 4-month 

old Shorea leprosula seedlings. 
A (x 0.1) and H (x 10): Non-myconrhizal roots (Control), B: Inoculated with S. dictyosporum (x 
0.1) and 5". columnare (C, x 0.1), L .laccata (D, x 0.1), Descomyces sp. (E, x 0.1), Rhizopogon 
luteolus(f,\Q.l),A. umbronata(G,xQ.l;l,x 15). 

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BIOTROPIA No. 12,   1999 

 

 

 

 

 

 

 

 

 

 

Figure 6:  Root system of 4-month old Shorea leprosula seedlings inoculated with Amanita umbronata (A, 
x 0.2 , B, X 0.5). 

 
Figure 7a: Degree of mycorrhizal colonization of S.dictyosporum (C, \ 0.4; D, x 8), S. columnare (E, x 0.4; 

F, x 10), Rhizopogon luteolus (G, x 0.4; H, x 10), at root system of 4-month old Shorea ovalis. 
A, B: non-mycorrhizal roots. 

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The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

 
Figure 7b : Degree of mycorrhizal colonization of I .laccata (I, x 0.4; J, x 10), A.umbronata (K, x 0.4; L, x 

10), and Descomyces sp. (M, x 0.4; N, x 10). 

 
Figure 8 : Transversal section of non-mycorrhizal and mycorrhizal roots of 4-month old Shorea ovalis 

seedlings. 
A. Structure of non-mycorrhizal roots (x 400), and inoculated with S.columnare (B, x 200), 5. 
dictyosporum (C, x 400), A.umbronata (D, x 400), Descomyces sp. (E, x 400) and Rhizopogon 
luleolus(F,x 1000). 

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BIOTROPIA No. 12, 1999 
 
Table 6. Leaf nutrient content of Shorea pinanga, Shorea leprosula, Shorea ovalis and Hopea odorata 

mycorrhizal and non-mycorrhizal seedlings. 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Note : Values in bold means nutrient content increment and the values not in bold means no nutrient 
increment. C: Control, Sc: Scleroderma columnare, Sd.: Scleroderma dictyosporum, R: Rhizopogon 
luteolus, LL: Laccaria laccata, AM: Amanita umbronata, DE: Descomyces sp. 

In S. pinanga seedlings, calcium concentration in the leaves was increased by 
the inoculation of Laccaria laccata (1.085%) and Descomyces sp. (1.111%), while 
the concentration of iron (Fe) was increased by the inoculation of Amanita 
umbronata ( 511.2 ppm) and Rhizopogon luteolus (410.6 ppm). The concentration of 
N, P, K and Mg was not significantly influenced by mycorrhizal inoculation. 

In Shorea leprosula, the concentration of nitrogen in the leaves was increased 
by the inoculation of Scleroderma columnare (1.737%), Laccaria laccata (1.659%) 
and Amanita umbronata (1.708%) and the concentration of calcium and magnesium 
was increased by the inoculation of Scleroderma columnare (0.904%) and Laccaria 

74 



The Effectiveness of some Ectomycorrhizal Fungi in Alginate Beads - Supriyanto 

laccata (0.204%). The concentration of P, K and Fe in the leaves was not influenced 
by the mycorrhizal inoculation. 

In Shorea avails, the nitrogen concentration in the leaves was increased by the 
inoculation of Scleroderma dictyasporum (1.317%), Amanita umbronata (1.356%), 
Rhizopogon luteolus (1.756%) and Descomyces sp. (1.542%). The concentration of P, 
K, Ca, Fe, Mg in the leaves of Shorea ovalis was not influenced by the inoculation of 
mycorrhizal fungi. 

In Hopea odorata, the nitrogen levels increased with inoculation of Rhizopogon 
luteolus (2.049%) and the level of calcium in the leaves was increased by 
Scleroderma columnare (0.903%), Laccaria laccata (0.909%) and Amanita 
umbronata (0.934%). Magnesium level increased with inoculation of Laccaria 
laccata (0.207%), Amanita umbronata (0.201%) and Descomyces sp. (0.200 %). Iron 
levels in the leaves of Hopea odorata was increased by the inoculation of 
Scleroderma dictyosporum (1154.7 ppm), Laccaria laccata (825.1 ppm) and 
Rhizopogon luteolus (661.2 %). 

There is no clear pattern of correlation between inoculation with mycorrhizal 
fungi and leaf nutrient content. There is also no clear difference in P concentration in 
the leaves following inoculation as compared to the controls. 

DISCUSSION 

Method of inoculum production of ectomycorrhizal fungi should be easily 
handled, cheap and effective to increase the seedling quality. Alginate beads, as a 
carrier of inoculum of ectomycorrhizal fungi, produces an inoculum of high quality 
and large scale (9,000 - 100,000 beads/hour/machine). 

Feldman and Idczak (1994) specified two characteristics of high quality 
inoculum. High quality means firstly that the inoculum is able to colonize rapidly the 
plant root system. This is guaranteed by an inoculum of high infection. It does not 
necessarily mean large number of spores. Secondly, the characteristic of a high 
quality inoculum is that it should be aseptic or contaminated with only small 
quantities of plant pathogenic microorganisms. Low level of contamination can be 
ignored, for example for planting stock production in the nursery. 

Regarding the percentage of germination of ectomycorrhizal fungi packed in 
alginate beads, the concentration of sodium alginate of 5 - 20 g/L does not prevent 
the spore germination, but its elasticity was different. Based on our results, a 
concentration of sodium alginate of 15 g/L was selected because of the high spore 
germination percentage and good bead elasticity associated with this. 

S. columnare, S. dictyosporum, Rhizopogon luteolus, Laccaria laccata, A. 
umbronata, Descomyces sp. that were packed in alginate beads, were able to colonize 
the root system of Shorea pinanga, S. leprosula, S. ovalis and Hopea odorata. Their 
colonization is shown to be moderate to good. The mycorrhizal fungi formed mantle 
and Hartig's net structures in the root system of the plant. It means that the alginate 
bead as a carrier of inoculum does not prevent the spore germination. Their degree of 

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BIOTROPIA No. 12, 1999 

compatibility can be evaluated on their capability to form the mantle and Hartig's net 
structure. A mycorrhizal species able to form mantle and Hartig's net structures in 
several plant species means that this mycorrhizal species has high compatibility. 
Likely, it is reflected on its natural distribution. Descomyces sp. and A. umbronata 
were the most possible to form those structures in the root system of dipterocarp 
species tested. Their degree of compatibility should be followed further on their 
growth effect and their mycorrhizal dependency value. 

Plants differ greatly in their need for, and response to, mycorrhizal infection. 
Relative Mycorrhizal Dependency (RMD) as degree to which a plant is dependent on 
the mycorrhizal condition at a given level of soil fertility had been defined 
(Gerdeman et al. 1975 in Bagyaraj 1994). The RMD concept was also improved to 
define the mycorrhizal dependency of crops on the mycorrhizal fungi in field 
conditions, called Relative Field Mycorrhizal Dependency (Plenchette et al. 1983 in 
Bagyaraj 1994). Based on the first and second rank of RFMD value, the dipterocarp 
mycorrhizal dependencies are as follows: 5. pinanga to Descomyces sp. and L. 
lacata, S. leprosula to Descomyces sp. and A. umbronata, S. ovalis to A. umbronata 
and L. laccata, H. odorata to A. umbronata and S. dictyosporum, respectively. Those 
mycorrhizal fungi are important for improving the growth of dipterocarp seedlings. 

Mycorrhizae have long been known to affect the nutrient cycling especially of P 
nutrition of the host plant. Phosphate is the major form of P available in the soil 
solution and, therefore, it is not readily transported by mass flow. Thus, as 
mycorrhizal hyphae explore the bulk soil beyond the root hairs, additionally P is 
taken up by hyphae and transported to the host (Alien 1996). Mycorrhizal fungi can 
also increase the uptake of mineralized P by occupying the microsites of active 
decomposition 'and, possibly, by being involved in the degradation of litter. 
Mycorrhizal hyphae on a decomposing leaf and rapid transport of32 P from that leaf to 
a host plant via mycorrhizal hyphae had been observed (Herrera et al. 1978 in 
Alien 1996). 

By their role in the acquisition of nutrient resources, mycorrhizae are critical 
components of nutrient cycling. Nutrient levels in the leaves of dipterocarp tested 
showed that mycorrhizal fungi could increase the nutrient concentration of some of 
the elements tested in the host plant. Based on our results, there is no clear difference in 
P levels in leaves following inoculation as compared to the controls. 

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