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First published online May 18, 2006
Journal of Experimental Biology 209, 2165-2169 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02252
Evidence that blue petrel, Halobaena caerulea, fledglings can detect and orient to dimethyl sulfide
1 Behavioural Ecology Group, CNRS-CEFE, 1919 route de Mende, F-34293
Montpellier, Cedex 5, France
2 Centre for Animal Behaviour, Section of Neurobiology, Physiology and
Behaviour, University of California, Davis, CA 95616, USA
* Author for correspondence (e-mail: francesco.bonadonna{at}cefe.cnrs.fr)
Accepted 3 April 2006
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Key words: Procellariiform seabird, dimethyl sulphide, orientation, Antarctic, petrel, Halobaena caerulea, olfaction.
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) and partner
recognition (Bonadonna and Nevitt,
2004). One of the early ideas to explain the function of the sense
of smell in petrels was that these seabirds use odours as foraging cues
(Grubb, 1972). For many petrel
species, prey includes small crustaceans, fish and krill, and consequently
early investigation mainly focused on attraction to fishy smelling compounds
(reviewed in Warham,
1996).
More recently, controlled behavioural experiments have shown that different
species of procellariiform seabirds are attracted to a variety of natural
scented compounds associated with their prey
(Nevitt et al., 2004). One
such compound, dimethyl sulphide (DMS), is an odour produced by photoplankton
that is associated with areas of high primary productivity where prey are
likely to be found (Nevitt et al.,
1995). Local emissions of marine DMS can be predictable features
in the environment, reflecting bathymetric features such as shelf breaks and
seamounts (Berresheim, 1987).
Moreover, DMS emissions have been shown to increase during grazing by
zooplankton (Dacey and Wakeham,
1986). Together, these features suggest an odour landscape that
may provide birds with orientation cues for foraging at sea
(Nevitt et al., 1995;
Bonadonna et al., 2003).
Recently, we have shown that at least one species of burrowing petrel,
Antarctic prions (Pachyptila desolata), can detect DMS at biogenic
levels, and that these birds can use DMS as an orientation cue in a
non-foraging context (Nevitt and
Bonadonna, 2005b). These results suggest that prions have the
ability to detect DMS and potentially use a DMS odour landscape as a
navigational aid at sea [harbour seals (see
Kowalewsky et al., 2005)].
The blue petrel (Halobaena caerulea) is another sub-Antarctic
burrow-species that is phylogenetically closely related to Antarctic prions
(Warham, 1996;
Penhallurick and Wink, 2004).
Both experimental and at-sea observational data suggest that both blue petrels
and prions use DMS as a foraging cue at sea
(Nevitt, 2000). Since DMS is
not necessarily produced by prey, birds most likely need to learn to associate
DMS with foraging opportunities soon after fledging. It is possible that this
association is learned even before chicks fledge, since returning parents
bring back scents on their feathers and in the regurgitations that are fed to
chicks. Such early learning would be particularly advantageous for petrels
since, unlike other pelagic species, parents abandon the chicks up to 10 days
before they fledge, leaving them to leave their underground burrows and forage
independently in a thoroughly unfamiliar environment
(Warham, 1996). While it is
possible that naïve fledglings find productive areas through information
transfer, i.e. by way of watching or following other birds coming and going
from the colony (Ward and Zahavi,
1973), it would be most efficient if chicks were able to recognize
foraging opportunities on their own as soon as they leave the nest. Thus, the
possibility we have been exploring is whether chicks leave their underground
burrow with a sense of smell that is already finely tuned to the ocean
environment (see also Cunningham et al., in press).
An initial study using the `Porter method' showed that blue petrel chicks
are able to detect both DMS at micromolar concentrations and a second,
presumably unfamiliar, rose-scented odour, phenyl ethyl alcohol
(Cunningham et al., 2003).
While the DMS concentration tested was considerably higher than ambient levels
that adults would encounter at sea (discussed in
Nevitt and Bonadonna, 2005b),
these results demonstrated that petrel chicks have a well developed olfactory
sense and may be responsive to odours. Since we know that olfactory
sensitivities may be shaped by early experience in many vertebrate species,
such as rabbits (Semke et al.,
1995), ferrets (Vargas and
Anderson, 1996), salmon
(Nevitt and Dittman, 1998) and
chickens (Sneddon et al.,
1998), we have since hypothesized that blue petrel chicks may be
able to learn biologically important odours before they leave the nest
(Nevitt and Bonadonna, 2005b;
Cunningham et al., in press; G. A. Nevitt, R. W. Van Buskirk, G. B. Cunningham
and H. Weimerskirch, manuscript submitted for publication). If this were the
case, then chicks would be predisposed to use odours they have associated with
food in the nest as foraging or orientation cues at sea. Inspired by this
idea, we wanted to test whether blue petrel chicks can detect DMS at biogenic
levels, and whether they are predisposed to use DMS as an orientation cue
before fledging.
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Materials and methods |
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1 km diameter) in the gulf of Morbihan in the
Kerguelen Archipelago. We chose blue petrels, Halobaena caerulea
Gmelin 1789 for this investigation because at-sea studies indicate that these
species naturally associate with DMS
(Nevitt, 2000), suggesting
that they can smell it, and potentially use it as an orientation cue.
Experiments were performed between 24 December 2003 and 15 January 2004, and
from 18 January and 12 March 2005. Birds were banded prior to the study to
identify individuals. For each experiment, birds were used only once. Since
blue petrels lay a single egg, only one chick per nest was tested.
We tested the olfactory responses of 22 blue petrel Halobaena
caerulea chicks using the Porter method (see
Porter et al., 1999;
Cunningham et al., 2003).
Briefly, chicks enter a sleep-like state, and the chick's responses are scored
in response to odour stimuli. This technique is non-invasive, does not affect
fledging success, and has been successfully applied to blue petrel chicks for
other studies (Cunningham et al.,
2003). Chicks were tested at approximately 15-20 days post hatch
(24 Dec-15 Jan; wing chord, 33.4±1.7 mm; tarsus, 24.8±0.6 mm;
mass, 135.3±6.6 g).
For each test, a chick was removed from its burrow and transported in a cotton bag to a well ventilated field hut (4 mx6 m) about 0.5 km from the colony. The chick was then positioned in a freshly lined holding chamber (approximately 10 cmx5 cmx5 cm) opened at both ends. The chick's head protruded from one end while the chamber walls provided contact around the bird's body. Once in the chamber, the chick quickly (within 3 min) entered a sleep-like state in which the head drooped slightly and the eyes closed. As in earlier studies, chicks were considered to be `asleep' when the eyes were closed, the head drooped, and the legs and wings relaxed. We let chicks sleep for at least 3 min before initiating a trial.
Stimuli (DMS or Control, see below) were presented by puffing odour above
the tube nose using a 500 ml Nalgene® squeeze bottle. The tip of the
bottle was positioned 3 cm from the opening of the tube nose. The bottle
was then squeezed 1-2 times in a 5 s period, producing brief puffs of
odorant-saturated air near the bird's nostrils. Responses to odorant
presentations were recorded for 1 min and scored categorically as one
(indicated by biting movements, vocalizations, distinct head or body
movements) or zero (typically no reaction) for each bird (modified from
Porter et al., 1999). Scoring
was done blind in that the solutions were prepared and coded by one
experimenter prior to the start of a trial. The second experimenter delivering
the stimulus and recording the response did not know the identity or
concentration of the stimulus being delivered. If the chick woke up during a
test, the chick was given up to 3 min for it to return to a sleep-like state.
The bird was then allowed to sleep before continuing the experiment. If the
bird did not fall asleep within 3 min, it was immediately returned to its
burrow.
DMS solution (10 pmol l-1, 100 ml) was prepared daily from stock
solution (1 mmol l-1; Sigma-Aldrich, St Louis, MO, USA) and bottled
spring water (Evian®) using sterile glassware. Control solution contained
100 ml water only. Test solutions were transferred to clean Nalgene®
squeeze bottles. Bottles were allowed to sit for at least 3 h at ambient
temperature (9-13°C) to equilibrate the headspace. We calculated the
headspace to be 18-21% of solution concentration using established methods
[(Dacey et al., 1984), assuming
an equilibrium coefficient K=15-20 at a temperature range of 10-14°C, or
approximately 2 pmol l-1]. This concentration falls well within the
biogenic concentrations that adults encounter while foraging (see
Nevitt and Bonadonna,
2005b).
Tests were conducted during daylight hours within a narrow temperature
range (9-13°C) during daylight hours when parents were at sea. Chicks were
transported and tested one at a time and spent approximately 15 min away from
the nest. Each chick was weighed after testing. We checked burrows again prior
to fledging to monitor any adverse affects to fledging success; weight gain
and wing chord growth were within normal parameters
(Jouventin et al., 1985) and
no mortality was noted.
Behavioural experiments
To determine whether blue petrel chicks would orient to DMS before
fledging, we presented birds with DMS in a Y-maze. We have previously
established that other burrow nesting species orient to unfamiliar odours in
Y-mazes. We have previously shown that adult prions prefer DMS to an
unfamiliar odour (Nevitt and Bonadonna,
2005b). In this experiment, adults had previously experienced DMS
at sea, and thus we assumed it was a familiar odour to them. Therefore, in the
present experiment, we predicted that if chicks were also already familiar
with DMS (i.e. through contact with their parents or food), then they would
also orient to this compound in a Y-maze.
The Y-maze was constructed from opaque PVC wire housing and had three 60 cm
symmetrical arms (for details, see
Bonadonna and Nevitt, 2004;
Nevitt and Bonadonna, 2005b).
One arm was used as the starting point and was fitted with two trapdoors that
formed a temporary holding compartment for the bird. Since chicks are
negatively phototactic, odour choice arms were darkened. The end of each odour
choice arm was equipped with a CPU cooling fan (Globe Fan Technology Co. Ltd.,
product number S05010, Taiwan) mounted on a partition to provide a low-noise,
controlled airflow (9 CFM; 243 l min-1). In the compartment behind
the fan, a Petri® dish (5.5 cm diameter) containing either DMS (1 µmol
ml-1, 4 ml) or control solution provided the stimuli. Odour stimuli
were alternated between arms for each trial and frequently exchanged with
fresh solutions. After each trial, the maze was washed thoroughly with
methanol (70%) to remove any odour residue.
DMS solution was prepared in propylene glycol (4 ml; 1 µmol
l-1); control solution contained propylene glycol only (4 ml). DMS
is much more soluble in propylene glycol than in water. To humans, this
compound is lightly scented, suggesting that birds had to discriminate between
two scented compounds rather than the presence or absence of odour. We have
previously estimated the evaporation rate to be 0.1 ml h-1 or
1.7 nmol l-1 min-1
(Nevitt and Bonadonna, 2005b).
This concentration, diluted by air flow in the maze (240 l min-1),
suggests that blue petrels were presented with an average stimulus
concentration of <10 pmol l-1 during experimental trials. This
concentration is below the detection threshold for humans
(Kowalewsky et al., 2005), but
falls well within estimates of biogenic emissions that birds are likely to
encounter at frontal zones in the Kerguelen plateau where adults are known to
forage (Berresheim, 1987;
Sciare et al., 1999;
Nevitt, 2000).
Chicks were tested one at a time. Each chick was away from its nest for a maximum of 30 min and we noted no deleterious effects to fledging success. For each experimental trial, a bird was removed from its burrow, transported to the maze and then placed in the temporary holding compartment for a 1 min acclimation period. An inner trapdoor was then lifted, which allowed the bird to make a choice. We assessed the bird's choice without disturbing the bird by the sounds of it walking in the particular arm of the maze. We scored a positive choice if the bird travelled halfway down an arm and stopped for at least 1 min. Most birds stopped at the end of the arm and remained there. No-choice birds tended to sit quietly in the entryway, and were removed from the maze after 15 min. The choice time was considered to be the time that a chick took to walk halfway up each maze's arm.
The chicks used for Y-maze experiments all had adult plumage and
successfully fledged 1-6 days after testing (mean ± s.e.m.:
3.6±1.6 days) at about 44 days after hatching (43±2 days)
(Jouventin et al., 1985).
Fledglings were tested after parental abandonment, and thus had not been
recently fed.
Statistical analyses
Statistical analyses were performed using SYSTAT. For Porter method
studies, DMS and control scores were compared using a Wilcoxin sign-rank test
for paired data. Y-maze data were analyzed using a Binomial test
(Zar, 1996). Values are
expressed as mean ± s.e.m.
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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2 pmol l-1 headspace concentration
(Dacey et al., 1984)] using the
Porter method (Porter et al.,
1999). Average scores were significantly higher for DMS than for
the control stimulus (P<0.03, W=-63.0, Wilcoxon
matched-pair sign ranks test, N=22;
Fig. 1).
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Discussion |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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),
and at least five orders of magnitude below olfactory detection thresholds
typically reported for other avian species
(Roper, 1999). One of the
improvements made to our experimental design in the present study is that we
confirmed detection ability at picomolar concentrations using a second method,
the Porter method. This method is non-invasive and allowed us to test
responses of an adequate sample size of chicks to DMS under conditions in
which odorant delivery and concentration were well controlled.
Although the Y-maze we used here was similar to the one we used in previous
experiments that tested attraction to DMS in Antarctic prions
(Nevitt and Bonadonna, 2005b),
the motivation of the subjects we tested was probably different. With prions,
we tested adults who had recently returned from sea and were subsequently well
fed in preparation for a 10-15 day incubation shift on the nest. Because these
test subjects were not motivated to look for food, we assumed that DMS in the
Y-maze indicated an avenue of escape to ocean. By contrast, the blue petrel
chicks that were tested in the present experiment had not been recently fed,
and were within a few days of fledging. These birds had also never experienced
DMS in the context of the pelagic environment. Moreover, because chicks were
given a choice between two different odours (DMS in propylene glycol
vs propylene glycol alone), the attraction seemed to be specific to
DMS rather than to the presence of any scented cue. Based on these results, we
conclude that the scent of DMS may already be associated with food before the
chick leaves the nest.
Why would an ability to smell DMS be advantageous for a fledgling? At sea,
DMS emissions become elevated in areas where zooplankton is grazed by
phytoplankton (Dacey and Wakeham,
1986; Daly and DiTullio,
1996). Consequently, DMS characterises areas rich in zooplankton,
in what is presumed to be a visually uniform environment, at least to humans.
Using changes in an odour landscape would seem to be an efficient mechanism
for localising patchily distributed prey
(Nevitt, 2000), but how or
when birds learn to associate prey-related odours with food or foraging
opportunities is unclear. One possibility is that young petrels learn to
associate feeding areas with DMS in their first months or years at sea.
However, our results, complemented by those of other studies, indicate that
chicks already may recognize DMS [or food odours (Cunningham et al., in
press)] even before they leave the nest. Alternatively, it is commonly assumed
that young petrels learn how to forage primarily by watching other birds [the
`information center' hypothesis (Ward and
Zahavi, 1973)]. While monitoring the activity of conspecifics
probably contributes to learning how to forage, this hypothesis ignores the
critical role olfaction plays in the foraging behaviour of certain species,
and particularly, burrow-nesting species
(Nevitt et al., 2004).
Thus, with respect to sensitivity to DMS, two additional possibilities may
be considered: (a) DMS may stimulate an innate attraction; (b) chicks reared
in burrows learn odour cues before leaving the nest. It could be argued that
hard-wired olfactory sensitivities usually function for highly constrained
uses [i.e. pheromone attraction, for example
(Shaal et al., 2003)].
However, olfactory behaviours that have evolved to contend with variability in
the environment tend to be shaped by learning (reviewed by
Hudson, 1999). Moreover,
behaviours that can be learned are more flexible to adapt to environmental
change or to differences that may exist between different populations living
in different areas. For example, among the Antarctic procellariiforms, species
show a great deal of variation in their foraging strategies, particularly with
respect to their attraction to different scented compounds linked either to
their prey or to the ecological characteristics of the species on which they
forage (Nevitt, 1999;
Nevitt et al., 2004;
Nevitt and Bonadonna, 2005a).
It follows that, in the context of foraging in a highly variable environment,
an inflexible, innate sensitivity to a specific suite of prey odours is not
likely to be adaptive.
Furthermore, data from a variety of systems support the hypothesis that
procellariiform chicks might learn to associate relevant foraging odours to
food during the rearing period. For example, it is now well established that
olfactory sensitivity is physiologically tuned after birth in a variety of
animals. In some cases, this tuning has been linked to behaviour, life history
and ecology. For example, salmon home to the scent of the stream of their
birth (reviewed by Nevitt and Dittmann, 2002), and rabbit pups imprint on the
scent of food-related odours expressed in the milk of their mother
(Altbacker et al., 1995;
Semke et al., 1995). When we
consider how and where a petrel chick develops (alone in a dark burrow), smell
is probably a major sensory stimulus during the first few months of life.
Odours brought back on the feathers of parents might provide chicks with the
opportunity to learn scents associated with productive areas. Moreover, DMS is
probably not the only odour they learn since chicks are exposed to a variety
of compounds through interactions with their parents, including scented
compounds in stomach oils with which they are nourished. These compounds are
derived, in part, from prey species and thus are linked to foraging
opportunities in the open ocean. We have recently shown that blue petrel
chicks are sensitive to at least some of these compounds (see Cunningham et
al., in press).
Linking these ideas together, our current hypothesis is that odour cues in
the nest may condition chicks to be able to find food rapidly once they have
fledged (see also G. A. Nevitt, R. W. Van Buskirk, G. B. Cunningham and H.
Weimerskirch, manuscript submitted for publication). For example, in chicken
chicks (Gallus domesticus), exposure to strawberry odour 5 days
before hatching influenced the chick's preference for this odour afterwards
(Sneddon et al., 1998). Our
results suggest that olfactory learning or imprinting in birds may have
important consequences to foraging success. These questions should be explored
further in procellariiform species that rely heavily on olfaction to
forage.
To summarize, while it is commonly assumed that young fledglings follow other birds to feeding areas, or simply wander over the ocean to locate a suitable feeding zone, our results suggest instead that chicks leave the nest already tuned to potential foraging opportunities in their environment. Chicks are thus equipped to adopt the same olfactory strategy used by adults from the beginning of their life at sea.
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