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Appl. Environ. Microbiol., Feb 1995, 556-560, Vol 61, No. 2
MJ Bidochka, SR Walsh, ME Ramos, RJ Leger, JC Silver and DW Roberts
The zygomycetous fungus Entomophaga grylli is a pathogen that shows
host-specific variance to grasshopper subfamilies. Three pathotypes of the
E. grylli species complex were differentiated by three molecular
techniques. In the first method, the three pathotypes showed different
fragment patterns generated by random amplification of polymorphic DNA
(RAPD). There was little or no interisolate variability in RAPD fragment
patterns within each pathotype. Passage of an isolate of pathotype 3,
originally from an Australian grasshopper (Praxibulus sp.), through a North
America grasshopper resulted in no differences in the resultant RAPD
fragment patterns. In the second method, polymorphic RAPD fragments were
used to probe the genomic DNA from the three pathotypes, and
pathotype-specific fragments were found. In the third method, restriction
fragments from genomic DNA of the three pathotypes were cloned and screened
for pathotype specificity. A genomic probe specific for each pathotype was
isolated. These probes did not hybridize to DNA from Entomophaga aulicae or
from grasshoppers. To facilitate the use of RAPD analysis and other
molecular tools to identify pathotypes, a method for extracting DNA from
resting spores from infected grasshoppers was developed. The DNA from the
fractured resting spores was of sufficient integrity to be blotted and
probed with the pathotype-specific DNA probes, thus validating the use of
these probes for pathotype identification in field-collected grasshoppers.
Copyright © 1995, American Society for Microbiology
Pathotypes in the Entomophaga grylli species complex of grasshopper pathogens differentiated with random amplification of polymorphic DNA and cloned-DNA probes
Boyce Thompson Institute for Plant Research, Cornell University, Ithaca, NY 14853, USA.
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