Abstract:
Cylindrocladium quinqueseptatum Boedijn & Reitsma causes seedling blight and
extensive defoliation on a wide variety of plants and the fungus is widely distributed in
the humid tropics. In Sri Lanka, C. quinqueseptatum is a serious pathogen of Eugenia
caryophyllata and is identified as a potential pathogen of Hevea brasiliensis.
Cultural characteristics and reproductive morphology of the clove isolate of C.
quinqueseptatum (IMI 342173) were shown to be similar to C. quinqueseptatum isolates
studied in different parts of the world. Dimensions and photomicrographs on
morphology of IMI 342173 (Rt) are also provided.
Some isolates collected from different clove growing localities in Sri Lanka
showed a great deal of variation in their morphology. Subsequent studies showed that
a distinct variation exists among C. quinqueseptatum isolates and differences in (a)
morphology, (b) sporulation on CDA and (c) growth at room temperature are significant
and provide a very useful characters to separate them.
Lesions produced on E. caryophyllata as well as on twenty one H. brasiliensis
clones by the different isolates following inoculation varied in size significantly showing
differences in virulence among the isolates. Isolate, Aw was the most virulent while Rw
isolate caused the smallest lesions consistently on Hevea clones indicating it's mild
nature. A considerable variation in susceptibility existed among the Hevea clones grown
in the Eastern Hemisphere. Clones PB 28/59, HP 74-181, Tjir 1, RRIC 121, RRIC 45,
RRIC 36, RRIC 130, RRIC 110, RRIM 712, RRIM 600 were the most susceptible and
IAN 873, AV 1373, RRIC 102 and [AN 717 were among the least susceptible clones.
The fungus sporulated freely when grown on artificial media viz. Czapek Dox
Agar and Lima Bean Agar, both under the normal light and dark regime and under
continuous dark. Spore production occurred between 20°C and 35°C with an optimum
at 30°C. Spore productivity was highest in the Aw isolate.
The maximum spore germination observed was around 90% after 5 h incubation
as wet smears on Hevea leaves. A period of 10 min exposure of spores as wet smears to
UV (253.7nm) inactivated the spores significantly and 40 min exposure was detrimental.
The most critical factor which influenced the spore viability and germination was the
humidity. Free water or a film of water (resulted as dew formation at 100% RH) was
found to be essential for spore germination. With regard to the lesion production on
leaves, lesions with a reasonable size were produced only at 100% humidity. Size of the
lesions at 96% humidity was negligible and no lesions were produced at 91% RH. The
temperature also greatly influenced the spore viability and germination. Spore
germination occurred above 10°C and below 35°C. Thus it was shown that the optimum
conditions for germination of spores are those conditions present in the rubber growing
districts of Sri Lanka during the South-West monsoon period.
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All isolates were found to be capable of secreting toxic substances to the growing
medium and this toxin was proved to be thermostable (up to 100°C) and host specific.
A technique was also developed to partially purify the toxin secreted by C.
quinqueseptatum. The type and the size of the lesions produced on Eugenia and different
Hevea clones by the crude toxin of different isolates varied markedly. Isolate Rt
produced the largest lesions overall on Hevea indicating its aggressive nature in toxin
production. Isolate Kp was also found to be very active while Aw and Rw showed only
a mild reaction. Three main clusters of clones were distinguished through cluster
analysis indicating the marked variation of Hevea clones grown in the Eastern
Hemisphere in sensitivity to the crude toxin.
None of the C. quinqueseptatum isolates secreted polygalacturonase (PG)
(except Kp isolate) or pectin lyase (PL) in culture. Isolate Kp showed mild PG activity.
The extracts of the clove and rubber leaf tissues inoculated even with Kp isolate did not
reveal any PG or PL activity. Our investigations, however, failed to show the
involvement of an inhibitor of PG. All isolates of C. quinqueseptatum secreted
cellulases viz. cellobiase and B-glucosidase in culture. A marked increase in activity of
cellobiase was detected on rubber leaf on third day following the infection and activity
of B-glucosidase, an inherent enzyme of Hevea leaves increased markedly following
infection. Considering the above observations and available literature it is proposed that
toxins play a vital role in initial stages of infection and development of symptoms while
latter stages of interaction may be due to the activity of cellulolytic enzymes.
A total of sixteen fungicides were screened against C. quinqueseptatum
employing three screening techniques; conidial germination test (CGT), poisoned food
technique (PFT), and soil fungicide screening test (SFST). Though there were eleven
fungicides effective in CGT, this number was reduced to five in SFST. However, only
four viz. benomyl, mancozeb, metalaxyl 8% + mancozeb 64% and oxadixyl 10% +
mancozeb 56% were identified as potential fungicides in the management of C.
quinqueseptatum. It was shown that, for a pathogen producing microsclerotia, SFST is
the most appropriate test. Further, the incubation period after treatment was of vital
importance in CGT as low incubation periods provide misleading information on the
efficacy of fungicides. In addition to chemical control, possibility of the development
of a successful breeding programme to produce disease resistant Hevea clones, using
observations reported on clonal susceptibility, is discussed