M13-microsatellite PCR and rDNA sequence markers for identification of Trichoderma (Hypocreaceae) species in Saudi Arabian soil

K.A. Abd-Elsalam, I. Almohimeed, M.A. Moslem and A.H. Bahkali
Published October 13, 2010
Genet. Mol. Res. 9 (4): 2016-2024 (2010)
DOI 10.4238/vol9-4gmr908

About the Authors
K.A. Abd-Elsalam, I. Almohimeed, M.A. Moslem and A.H. Bahkali

Corresponding author:
K.A. Abd-Elsalam
E-mail: kamel200@ksu.edu.sa

ABSTRACT

Seven fungal isolates were identified as pan-global Hypocrea/Trichoderma species, from section Trichoderma, on the basis of their morphology. These species were H. lixii/T. harzianum and H. orientalis/T. longibrachiatum. PCR-based markers with primer M13 (core sequence of phage M13) and internal-transcribed spacer sequences of ribosomal DNA were used to confirm the identity of the two Trichoderma species. Sequence identification was performed using the TrichOKEY version 2.0 barcode program and the multilocus similarity search database TrichoBLAST. Sequences from the ribosomal DNA internal-transcribed spacer regions showed limited variation among the Trichoderma species. This analysis divided the isolates into two main groups. Grouping the isolates based on cluster analysis of their DNA profiles matched the grouping based on morphological taxonomy. Molecular data obtained from analyses of gene sequences are essential to distinguish phonetically cryptic species in this group and to establish phylogenetic relationships.

Key words: Trichoderma; Phytopathogenic fungi; PCR; Biological control.

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