2.8. Statistical analysesAll treatm

2.8. Statistical analyses
All treatments were repeated once and those showing a variability
coefficient higher than 20% were tested an additional time. Student’st-test
was used for a specific contrast. The statistical package used was SPlus
Version 6.2 (Insightful Corp, Seattle, WA, USA).
3. Results and discussions
3.1. HPP-induced germination ofC. perfringensspores
A negligible extent of germination was observed when pressuretreated (at 100, 150 or 200 MPa for 7 min at 50

C)C. perfringens
spores were incubated at 40

C for 60 min in 25 mM phosphate
buffer (pH 7.0) (Fig. 1). Microscopy analysis was consistent with
negligible germination, as only a small fraction of the pressuretreated spore population (w10%) had become phase dark (data not
shown). This result is in contrast to the result obtained with B.
subtilis spores, where a low pressure (w150 MPa) could induce
spore germination by activating the GerA-type receptors (Black
et al., 2005; Paidhungat et al., 2002). In B. subtilisspores, the
requirements for low-pressure activation of GerA-type receptors
are similar to requirements for nutrient activation of these receptors (Black et al., 2005). AlthoughC. perfringensGerA-type receptors
have not been fully characterized, they have striking differences
with those ofB. subtilis (Paredes-Sabja et al., 2008d). Indeed
C. perfringensGerKA and GerKC proteins are required for nutrient
germination (i.e.,L-asparagine) asB. subtilisGerA-type receptors,
yet they are also required for normal DPA release through chemical
germination (i.e., Ca-DPA and dodecylamine) and spore outgrowth
(Paredes-Sabja et al., 2008d), suggesting differences on the
germination apparatus betweenC. perfringensandB. subtilisspores.
These differences might be related with the lack of low-pressure
induced germination observed in C. perfringensspores.