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Appl. Environ. Microbiol., 11 1995, 3943-3949, Vol 61, No. 11
K Groppe, I Sanders, A Wiemken and T Boller
Randomly amplified polymorphic DNA fingerprinting, which is based on PCR
with arbitrary 10-nucleotide primers, were used to analyze genetic
diversity among isolates of the endophytic ascomycete Epichloe typhina,
which were collected at a single field site from a population of one of its
hosts, the grass Bromus erectus. One of the polymorphic randomly amplified
polymorphic DNA PCR products occurred in all isolates as single bands with
different but closely related sizes. Two of the size variants of this
product were cloned and sequenced, and they were found to represent the
same DNA sequence, except for a stretch of tandem repeats of the
trinucleotide AAG.TTC, which differed in size, consisting of 8 and 18
repeats, respectively. Tandem repeats of this type are called
microsatellites. Oligonucleotides were synthesized corresponding to
portions of the sequence flanking the microsatellite and were used for PCR
amplification of the loci from the genomic DNAs of different Epichloe
isolates. A single PCR product was found for most isolates, indicating that
the sequence represented a single genetic locus. Five alleles that could
clearly be distinguished in size were found in a population of 91 field
isolates. PCR with (AAC)8 and (AAG)8 as primers yielded a number of
amplified bands from genomic DNA of Epichloe isolates, indicating that
these types of microsatellites occur frequently in the genome of this
fungus. A survey of all fungal DNA sequences currently deposited in the DNA
sequence databases of EMBL and GenBank revealed that microsatellites of
different repeating units are widespread in fungi.(ABSTRACT TRUNCATED AT
250 WORDS)
Copyright © 1995, American Society for Microbiology
A microsatellite marker for studying the ecology and diversity of fungal endophytes (Epichloe spp.) in grasses
Botanisches Institut der Universitat Basel, Switzerland.
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