The SZN sampling and analysis strategy was as follows (samples were taken at N1,N2,N3,N4, S1,S2,S3,S4, E1,E2,E3,E4 and SE01,SE02,SE03 SE04 stations):
m mesh size); at each station, 10
Calanus helgolandicus females were sorted from samples and incubated in 50 ml bottles with natural
sea water phytoplankton; after 24 h females were removed and eggs counted, after another 24 h the number of
hatched eggs was determined; at each station, 30 females were incubated in filtered sea water for 24 h and
then fixed with Trizol (Invitrogen) and stored in liquid nitrogen;
m net ( 40 cm diameter)by towing at the
surface for ten minutes; samples were centrifuged at 3500 rpm for 3 minutes and pellets were stored
in liquid nitrogen; each pellet will be analyzed for chemical costituents such as polyunsaturated aldehydes,
epoxyalcohols, hydroxyacids and other oxylipins.
The 200 m Nansen net sample was used to
quantify the number of Calanus helgolandicus females, males and juveniles
in order to estimate secondary production rates at the time for this
important copepod species in the Adriatic Sea. Egg production and egg
hatching success data will further allow the estimation of recruitment
rates at each station in this period which generally coincides with the
period of maximum population numbers for this species. To verify the
possibility of using fluorescent markers to quantify live/dead eggs thereby
avoiding cumbersome egg hatching success experiments that require 48h
onboard ship incubations, 100 Calanus eggs were also collected at several
stations and fixed in 4% formaldehyde for further Comet-assay analysis
in the laboratory. This is a sensitive technique for the detection of DNA
damage at the level of the individual cell and is a standard technique for
evaluation of DNA damage/repair, biomonitoring and genotoxicity testing.
The test has rarely been used for copepods before and SZN is currently
developing this method in the laboratory, together with
new methods for stress gene analyses in copepods, particularly in C.
helgolandicus. Frozen samples (adult females and males) collected at
different stations during the cruise will be evaluated for up- or
down-regulation of the following genes: Cytochrome P450, Glutathione
S-transferase, Glutathione Synthase, Aldehyde Dehydrogenases, Catalase,
Superoxide Dismutase, Alpha and Beta Tubulins, Inhibitor of Apoptosis
Protein (IAP), Cell Cycle and Apoptosis Regulatory Protein (CARP), Cellular
Apoptosis Susceptibility Protein (CAS). These results will allow to
determine whether copepods were more "stressed" at some stations rather
than others, and to identify the possible causes leading to reduced fitness
in C. helgolandicus. Previous studies in SZN laboratory have shown that
diatoms produce a number of toxic oxylipins deriving from the oxidation of
polyunsaturated fatty acids which reduce copepod egg hatching success and
later larval recruitment (reviewed by IANORA2010). Since the
period of the cruise coincided with the end of a Skeletonema marinoi diatom
bloom the objective of the studies was to evaluate oxylipin production at
different stations and possible impacts on the C. helgolandicus population
(e.g. reduced egg hatching success and population recruitment rates,
down-regulation of specific stress genes).
![\includegraphics[width=\linewidth]{IMG/SW104_LUNGO_01.eps}](img34.gif)
![\includegraphics[width=\linewidth]{IMG/SW104_CORTO_01.eps}](img35.gif)