Studies on cultural, morphological, pathogenic and molecular variability of Alternaria brassicae, the causal agent of blight disease of rapeseed-mustard

Prateeksha Mehra, AK Tewari and GoharTaj

Abstract


In the present studies A. brassicae isolates (20 nos.) showed the existence of genetic diversity. Significant
variation in cultural, morphological, pathogenic and molecular variability was observed in A. brassiace isolates
irrespective to geographical locations and Brassica spp. Maximum radial growth (82.0 mm) was in AB-B.
juncea Pantnagar isolate, while minimum in AB- B. caulorapa (49.7 mm) on PDA. Variations were also
observed in colony colour, appearance, margin and zonation number. Substantial variations were found in spore
morphology in respect to conidial length, width and number of septa. Average conidial length and width were
varied from 29.0-6.6 x 185.3-28.2μm. Maximum spore length and width was in AB-B. carinata isolate (185.3
x 25.6 μm), while minimum in AB-B. caulorapa (29.0 x 6.6μm). Number of horizontal and vertical septa ranged
between 3.50-14.75 and 0.75-5.0 respectively. All the isolates were pathogenic to Brassica spp. AB-B. juncea
Pantnagar isolate was most virulent, while AB-S. alba least virulent. RAPD (18 no.) and ISSR (4 no.) primers
generated a total of 310 reproducible and scorable polymorphic bands ranged from 100 to 1350 bp which
displayed genetic polymorphisms among the A. brassicae isolates. On the basis of cultural, morphological,
pathogenic and molecular variability, the A. brassiace isolates has been categorized into 5 major groups. Group
I: AB-R. sativus, AB-B. pekinensis, AB-B. oleracea, AB-B. botrytis and AB-B. caulorapa; Group II: ABB.
juncea Pantnagar, AB-Yellow sarson, AB-Toria, AB-B. nigra, AB-R. oleifera, AB-B. juncea Karnal, ABB.
juncea Punjab and AB-B. juncea Bihar; Group III: AB-B. napus, AB-B. carinata, AB-E. sativa , AB-S.
alba; Group IV: AB-B. juncea Kangara and AB-B. juncea Jammu; Group V: AB-B. rugosa. The different
Brassica spp. (08 nos.) used in the present investigation to differentiate different A. brassicae isolates (09 nos.)
as host differentials has been categorized into 4 major groups on the basis of differential phenotypic disease
reactions. Group I: Varuna, PT-303, PYS-6 and B. nigra; Group II: PBN-9501 and Kiran; Group III: E.
sativa; Group IV: S. alba. Among different methods of culture preservation of A. brassicae isolates, 10 per
cent glycerol at -20ºC was best in terms of sporulation (66.7%) followed by PDA at 4ºC (65.7%) and could be
used for the preservation of A. brassicae isolates at least two years.


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