Detection and differentiation of Colletotrichum gloeosporioides isolates using PCR
- Peter R. Mills,
- S. Sreenivasaprasad,
- Averil E. Brown
- Plant Pathology Research Division,
- Queen's University Belfast
Research Output: Contribution to journal Article Peer-review
Abstract
An oligonucleotide primer (CgInt), synthesised from the variable internally transcribed spacer (ITS) 1 region of ribosomal DNA (rDNA) of Colletotrichum gloeosporioides was used for PCR with primer ITS4 (from a conserved sequence of the rDNA) to amplify a 450-bp fragment from the 25 C. gloeosporioides isolates tested. This specific fragment was amplified from as little as 10 fg of fungal DNA. A similar sized fragment was amplified from DNA extracted from C. gloeosporioides-infected tomato tissue. RAPD analysis divided 39 C. gloeosporioides isolates into more than 12 groups linked to host source and geographic origin. Based on the results obtained, the potential of PCR for detection and differentiation of C. gloeosporioides is discussed.
Publication Information
Output type
Research Output: Contribution to journal Article Peer-review
Original language
EnglishPages from-to (Number of pages)
Pages 137-143 (7 pages)Journal (Volume, Issue Number)
FEMS Microbiology Letters (Volume 98, Issue 1-3)Publication milestones
- Published - 01/11/1992
Publication status
Published - 01/11/1992
ISSN
0378-1097External Publication IDs
- Scopus: 0026446703
- PubMed: 1459401
