et al. 2011).P. chrysogenum demonst

et al. 2011).
P. chrysogenum demonstrates that fungal species identification
based on morphological and phenotypic characteristics
can be challenging, often leading to contradictory
findings and the grouping of more than one species (Taylor
et al. 2000). As P. chrysogenum exhibits few distinguishing
features, which additionally may vary depending on growth
conditions and culture media (Henk et al. 2011). Using the
genealogical concordance phylogenetic species recognition
(GCPSR) for fungi has proven to be fruitful, by utilising
multiple genealogies to detect and distinguish species by
diagnosing breaks in concordance amongst gene phylogenies
(Taylor et al. 2000). Phylogenetic studies have shown that there
are multiple distinct lineages within what was previously
considered P. chrysogenum (Scott et al. 2004; Henk et al. 2011).
The analysis of 81 NRRL strains and 125 collected samples
demonstrated the ‘Fleming species’, including the original
Fleming isolate (NRRL-824) and the industrial penicillin producing
strain (NRRL-1951, the isolate found on a mouldy
cantaloupe), diverged from P. chrysogenum sensu stricto (NRRL-
810) circa 0.8 million yr ago (MYA) (Henk et al. 2011). Furthermore,
the authors described two additional species within
the Chrysogenum species complex, provisionally named
Species A and Species B, which are likely to have diverged
even more recently from within the group (Henk et al. 2011).
Species-specific diagnostic tools enabling discrimination
between the four species are required as each species elicits
minimal phenotypic features (Henk et al. 2011) which are
likely to be unstable between different isolates. In this paper
the term ‘Chrysogenum complex’ is applied rather than
‘Chrysogenum series’ as we are specifically referring to the
four species recently described by Henk et al. (2011). The official
‘series Chrysogena’ additionally includes Penicillium