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Chapter 2<br />

time) and a dried bi<strong>of</strong>ilm (cell suspension and organic substances were<br />

dried onto the surface to simulate organic soil). The comparative work also<br />

incorporated a dehydrated bi<strong>of</strong>ilm model where the coupons were<br />

released from the CBR and dried in a petri-dish over a 2 hour period. The<br />

SD for the mean log 10 density <strong>of</strong> cells on the two glass coupons was 0.211<br />

and 0.224 for P. aeruginosa and S. pneumoniae bi<strong>of</strong>ilm respectively [117].<br />

When examining P. aeruginosa bi<strong>of</strong>ilm density, the CBR model had a lower<br />

SD than the drip-flow (SD <strong>of</strong> 0.788), the dehydrated bi<strong>of</strong>ilm (0.548) and<br />

dried surface bi<strong>of</strong>ilm (0.435), but a slightly higher SD than the static bi<strong>of</strong>ilm<br />

(0.208). The S. pneumoniae bi<strong>of</strong>ilm density assessed in the CBR had a lower<br />

SD than the drip flow (SD <strong>of</strong> 0.586), the static bi<strong>of</strong>ilm (0.330) and the<br />

dehydrated bi<strong>of</strong>ilm (0.322). The dried surface bi<strong>of</strong>ilm had a lower SD<br />

(0.157) [117].<br />

Donlan et al. described the assessment <strong>of</strong> S. pneumoniae bi<strong>of</strong>ilm density in<br />

situ and in real time using the CBR model [124]. The bi<strong>of</strong>ilm was developed<br />

on germanium coupons and bi<strong>of</strong>ilm cell density was measured using the<br />

plate count technique after 21, 45, 69, 141 and 189 hours development.<br />

The mean log 10 density and SD was calculated from 3 replicate coupons,<br />

with 2 coupons used to calculate the SD <strong>of</strong> the 141 hours incubation time.<br />

There was no indication if the replicate coupons were taken from the single<br />

or multiple runs using the CBR. The SD for bi<strong>of</strong>ilm density was between<br />

0.06-0.34 for the five time points [124]. Hadi et al. used X-ray diffraction,<br />

spectroscopy and SEM to examine the density <strong>of</strong> P. aeruginosa bi<strong>of</strong>ilm<br />

formed on plastic (polytetrafluoroethylene) coupons using the CBR [123].<br />

Hadi et al. reported an SD <strong>of</strong> 0.655 through crystal violet staining and<br />

measurement <strong>of</strong> the bi<strong>of</strong>ilm through a commercial assay used to quantify<br />

the volume <strong>of</strong> proteins remaining on the surface. The SD was calculated on<br />

9 coupons from each run, performed in triplicate (n=27) [123].<br />

Page<br />

46

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