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Mechanisms of Olfaction in Insects - ResearchSpace@Auckland ...

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Conclud<strong>in</strong>g Discussion 130<br />

components or test odorants may be toxic to the OR be<strong>in</strong>g tested and an<br />

understand<strong>in</strong>g <strong>of</strong> the roles <strong>of</strong> other olfactory players <strong>in</strong> these <strong>in</strong> vitro systems may<br />

help overcome these limitations.<br />

Functional studies <strong>of</strong> EpOR6, 30, 33 and 34 will enable the determ<strong>in</strong>ation <strong>of</strong> their<br />

roles <strong>in</strong> E. postvittana olfaction. The phylogenetic relatedness <strong>of</strong> EpOR6 to the<br />

pheromone receptors from other moths confers it as a PR candidate, however, tissue<br />

expression analysis and functional characterisation <strong>of</strong> this candidate OR will deduce<br />

its role <strong>in</strong> E. postvittana olfaction. The relatively high expression <strong>of</strong> EpOR30, 33 and<br />

34 <strong>in</strong> male moth antennae, as shown by qRT-PCR is suggestive <strong>of</strong> a plausible role <strong>in</strong><br />

pheromone recognition <strong>of</strong> these ORs. In situ hybridisation <strong>of</strong> these candidates can be<br />

used to test if they are likely PRs. ORs that are expressed at the base <strong>of</strong> pheromone<br />

sensitive trichoid sensilla <strong>of</strong> male moths will likely be PRs. Functional analysis by<br />

clon<strong>in</strong>g, expression and characterisation <strong>in</strong> an assay system aga<strong>in</strong>st E. postvittana<br />

pheromone components will confirm their b<strong>in</strong>d<strong>in</strong>g partners. The functional<br />

characterisation <strong>of</strong> PRs from moths such as B. mori and H. virescens has <strong>in</strong>dicated the<br />

presence <strong>of</strong> multiple PRs with<strong>in</strong> each species which are tuned to recognis<strong>in</strong>g one or<br />

more <strong>of</strong> the sex pheromone components. It is tempt<strong>in</strong>g to postulate the existence <strong>of</strong><br />

multiple PRs <strong>in</strong> E. postvittana also and one or more <strong>of</strong> the four candidates could be<br />

the PRs <strong>of</strong> E. postvittana, however, further functional analysis will have to be done to<br />

test the roles <strong>of</strong> these ORs.<br />

If any <strong>of</strong> these four candidates are found to be the PR for E. postvittana, then further<br />

strategies can be developed <strong>in</strong> deal<strong>in</strong>g with this agricultural pest. Mimics that can act<br />

as irreversible block<strong>in</strong>g agents for the b<strong>in</strong>d<strong>in</strong>g site <strong>of</strong> the PR could be developed. A<br />

mimic that will not be cleared from the receptor after signal attenuation would be<br />

ideal (native pheromones are cleared from the receptor hence large amounts are<br />

needed <strong>in</strong> mat<strong>in</strong>g disruption studies, render<strong>in</strong>g this pest control method expensive). Its<br />

release <strong>in</strong>to E. postvittana <strong>in</strong>fested areas could see a reduction <strong>in</strong> the number <strong>of</strong><br />

successful mat<strong>in</strong>gs as the mimic will flood the PR and confuse the male moth.<br />

Another strategy would be to genetically modify the PR itself so that it no longer<br />

recognises the pheromone components. This can be done by completely shutt<strong>in</strong>g <strong>of</strong>f<br />

the PR by RNAi silenc<strong>in</strong>g. Small <strong>in</strong>terfer<strong>in</strong>g RNA or double-stranded RNA (dsRNA)<br />

could be sprayed on host plants, or genetically modified plants express<strong>in</strong>g dsRNA

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