A comparison of the discriminatory ability and sensitivity of the trigeminal and olfactory systems to chemical stimuli in the tiger salamander

Summary Trigeminal receptors can respond to a wide variety of chemical stimuli, but it is unknown whether these receptors mediate discrimination between chemical stimuli matched for equal perceptual intensity. The present electrophysiological and behavioral experiments address this issue using tiger salamanders, Ambystoma tigrinum, and four compounds (amyl acetate, cyclohexanone, butanol, and d-limonene). In addition, the relative sensitivities of the trigeminaland olfactory systems to these compounds are compared. In electrophysiological cross-adaptation experiments (amyl acetate vs cyclohexanone; butanol vs d-limonene), there was complete cross adaptation such that only concentrations above the background (crossa-dapting) stimulus concentration elicited responses, suggesting that chemical stimuli may stimulate trigeminal receptors nonspecifically. In behavioral experiments (amyl acetate vs cyclohexanone; butanol vs d-limonene), only animals with intact olfactory nerves could discriminate between perceptually equivalent concentrations, that is concentrations that elicited the same level of responding. Both electrophysiologically and behaviorally, the trigeminal system exhibited higher thresholds than the olfactory system. We conclude that trigeminal chemoreceptors, at least in salamanders, are unable to discriminate between these two pairs of compounds when matched for equal perceptual intensity, and that trigeminal chemoreceptors are less sensitive than olfactory receptors.Abbreviations AA amyl acetate - CH cyclohexanone - LI d-limonene - BU butanol - EOG electro-olfactogram - ISI interstim-ulus interval - ONX olfactory nerve cut - ppm parts per million (1 l of compound in vapor phase/1l of air=1 ppm)     

Physical Variables in the Olfactory Stimulation Process

Electrical recording from small twigs of nerve in a tortoise showed that olfactory, vomeronasal, and trigeminal receptors in the nose are responsive to various odorants. No one kind of receptor was most sensitive to all odorants. For controlled stimulation, odorant was caused to appear in a stream of gas already flowing through the nose. Of the parameters definable at the naris, temperature, relative humidity, and nature of inert gas had little effect on olfactory responses to amyl acetate, whereas odorant species, odorant concentration, and volume flow rate effectively determined the responses of all nasal chemoreceptors. An intrinsic variable of accessibility to the receptors, particularly olfactory, was demonstrated. Flow dependence of chemoreceptor responses is thought to reflect the necessity for delivery of odorant molecules to receptor sites. Since the olfactory receptors are relatively exposed, plateauing of the response with flow rate for slightly soluble odorants suggests an approach to concentration equilibrium in the overlying mucus with that in the air entering the naris. Accordingly, data for responses to amyl acetate were fitted with Beidler's (1954) taste equation for two kinds of sites being active. The requirement for finite aqueous solubility, if true, suggests substitution of aqueous solutions for gaseous solutions. A suitable medium was found and results conformed to expectations. Olfactory receptors were insensitive to variation of ionic strength, pH, and osmotic pressure.     

Olfactory performance of rats after selective deafferentation of the olfactory bulb by 3-methyl indole

Rats trained to detect propyl acetate and valeric acid and to discriminate between propyl acetate and amyl acetate and between valeric acid and butyric acid were injected with a low dose of 3-methyl indole, a treatment that produces well-defined and selective deafferentation of the olfactory bulbs. Treatment completely deafferented most but not all bulbar loci for aliphatic acids and at least disrupted those for propyl and amyl acetate. In posttreatment tests, experimental rats performed somewhat but not significantly more poorly than controls and about as well on the acid detection and discrimination tasks as on the corresponding acetate tests.     

Functional capacity of the rat olfactory bulb after neonatal naris occlusion

Adult rats which had one naris closed when 1 –6 days oldwere trained using operant conditioning to detect differentconcentrations of amyl acetate and discriminate between ethylacetate and linalyl acetate. After removal of the olfactorybulb ipsilateral to the open naris, animals were able to detectand discriminate odors, although, relative to pre-operativeperformance, they were less accurate in initial trials of thelowest amyl acetate concentration and on the two-odor discriminationtask. In five additional rats histological analysis demonstrateda marked reduction in the size of the bulb ipsilateral to theclosed naris. The control olfactory bulb was removed and theipsilateral nasal fossa was syringed with horseradish peroxidase(HRP) in one animal. Examination of the contralateral olfactorybulb demonstrated anterograde axonal transport of HRP from sensoryaxons to olfactory bulb glomeruli. These data demonstrate thatneonatal naris closure does not completely deprive the ipsilateralolfactory receptors of vapor stimulation, that several monthsafter naris closure the ipsilateral olfactory receptor neuronsare functional and that vapors entering one nasal fossa canstimulate receptors in the contralateral fossa. The channelfor this intra-nasal communication is probably the nasopharyngealcanal (‘septal window’).     

Self- and cross-adaptation to chemical stimulation of the nasal trigeminal nerve in the rat

Electrophysiological, multi-unit responses from the ethmoidbranch of the trigeminal nerve to chemical stimuli (amyl acetate,d-carvone, l-carvone, l-menthol and toluene) were examined,using self- and cross-adaptation paradigms, to address the questionof whether different chemical stimuli may stimulate trigeminalnerve fibers using different ‘receptive pathways’and thus to suggest whether qualitative distinctions betweendifferent compounds may be made by trigeminal chemoreceptors.No adaptation occurred between l-menthol and toluene, suggestingthat these two compounds activate different receptive pathwaysin the trigeminal nerve which may be capable of making qualitativediscriminations between these two compounds. Symmetrical adaptationoccurred between amyl acetate and d-carvone, amyl acetate andl-carvone, amyl acetate and toluene, and l-carvone and d-carvonesuggesting that these compounds may activate the same receptivepathways in the trigeminal nerve which may not be capable ofmaking qualitative discriminations between these compounds.Asymmetrical adaptation occurred between amyl acetate and l-menthol,d-carvone and l-menthol, l-carvone and l-menthol, d-carvoneand toluene, and l-carvone and toluene. This implies that theprocessing of these stimuli by trigeminal nerve fibers may bemore complex than anticipated previously.     

Odorants presented to the rat nasal cavity increase cortical blood flow

Complaints about unpleasant environmental odorants, both outdoor and indoor, are increasingly being reported. The main complaints of health symptoms from environmental odorants are eye, nose and throat irritation, headache and drowsiness. Complaints may arise from the stimulation of olfactory receptors or trigeminal chemoreceptors. Stimulation of cerebrovascular nociceptors originating from a branch of the trigeminal nerve may be associated with an increase in cortical blood flow which is thought to be related to headache. Since odorants are reported to elicit headaches, the possibility that odorants may increase cortical blood flow was examined. Cortical blood flow was monitored in rats using a laser-Doppler flowmeter. The flowmeter probe was placed over the left frontal cortex while propionic acid, cyclohexanone, amyl acetate or butanol was delivered to the nasal cavity via an olfactometer. Cortical blood flow increased as the concentration increased for three of the odorants tested. The greatest increase in blood flow occurred to the presentation of propionic acid, followed by cyclohexanone and amyl acetate. There was no response to butanol. These data demonstrate that odorants can alter cerebrovascular blood flow, which may account, in part, for one of the health symptoms reported for odorants.     

大壁虎与嗅觉相关的学习记忆

壁虎科动物鼻腔较大,化学感觉系统发达,类似于对化学信息敏感的舌端游离的蜥蜴目动物（Malan,1946),并且嗅黏膜面积很大,感觉器神经元多,嗅神经系统十分完善（Gabe and Saint,1976).     

Stimulus parameters and temporal evolution of the olfactory evoked potential in rats

Evoked potentials were recorded from olfactory bulb, piriformcortex and scalp in urethane anesthetized rats in response tobrief odorant stimuli (amyl acetate, phenylethyl alcohol, eugenol)presented through a nasal cannula by means of a constant flowolfactometer. The effects of stimulus duration, nasal cannulaposition, flow rate, concentration and interstimulus intervalwere examined. The highest amplitude potentials were evokedby 10% amyl acetate at 20 ms duration, 1000 ml/min flow rateand a 60-s interstimulus interval with the stimulus deliveredat the nares. Odorant evoked potentials from deep within theolfactory bulb consisted of a triphasic wave with major componentsat 60 ms (P60), 90 ms (N90) and 140 ms (P140) with the lattertwo reversing polarity close to the surface of the bulb. Potentialsrecorded from layer I of piriform cortex were of similar amplitude,but opposite in polarity to the deep olfactory bulb potentials.Recordings from the skin over the nose elicited waveforms ofsimilar morphology to the deep olfactory bulb potentials, butone-quarter the amplitude and of opposite polarity The evokedpotentials changed with repetitive stimulation The N90 componentwas not present initially and only appeared after several stimuli.The appearance of the N90 component depended on the integrityof the olfactory peduncle. Thus, olfactory evoked potentialsto odorant stimuli reflect dynamic aspects of the encoding ofolfactory information dependent on connections between olfactorybulb and piriform cortex     

Olfactory event-related potentials: older males demonstrate the greatest deficits

Olfactory event-related potentials (OERPs) were recorded monopolarly at the Fz, Cz, and Pz electrode sites in 16 young adults (8M/8F) and 16 older adults (8M/8F) with inter-stimulus intervals (ISI) of 45, 60 and 90 s using amyl acetate as the odorant stimulus. N1, P2, and N2 peak amplitudes and latencies were measured. Young participants demonstrated significantly shorter peak latencies than older participants. Older males demonstrated significantly smaller peak amplitudes than the other participant groups. Peak amplitudes also increased with longer ISIs for older males. The OERP is compared to traditional olfactory psychophysical testing.     

Response patterns of single neurons in the tortoise olfactory epithelium and olfactory bulb

The responses to odor stimulation of 40 single units in the olfactory mucosa and of 18 units in the olfactory bulb of the tortoise (Gopherus polyphemus) were recorded with indium-filled, Pt-black-tipped microelectrodes. The test battery consisted of 27 odorants which were proved effective by recording from small bundles of olfactory nerve. Two concentrations of each odorant were employed. These values were adjusted for response magnitudes equal to those for amyl acetate at –2.5 and –3.5 log concentration in olfactory twig recording. Varying concentrations were generated by an injection-type olfactometer. The mucosal responses were exclusively facilitory with a peak frequency of 16 impulses/sec. 19 mucosal units responded to at least one odorant and each unit was sensitive to a limited number of odorants (1–15). The sensitivity pattern of each unit was highly individual, with no clear-cut types, either chemical or qualitative, emerging. Of the 18 olfactory bulb units sampled, all responded to at least one odorant. The maximum frequency observed during a response was 39 impulses/sec. The bulbar neurons can be classified into two types. There are neurons that respond exclusively with facilitation and others that respond with facilitation to some odorants and with inhibition to others. Qualitatively or chemically similar odorants did not generate similar patterns across bulbar units.     

Identification of carbonic anhydrase activity in bullfrog olfactory receptor neurons: histochemical localization and role in CO2 chemoreception

The objectives of this study were to determine: (1) the frequency and distribution of carbonic anhydrase (CA) activity in the bullfrog nasal cavities, and (2)␣whether inhibition of nasal CA affects the olfactory receptor response to CO₂ or other odorants. It was found, using Hansson's staining technique, that some olfactory receptor neurons exhibited CA activity and that these CA-positive receptors were distributed throughout the nasal cavity with peak densities in the dorsal and ventral sensory epithelial regions. To test for the role of CA in olfactory transduction, electro-olfactograms (EOGs) were recorded from the surface of the ventral sensory epithelium in response to 2-s pulses of 5% CO₂ and amyl acetate before and after topical CA inhibition with acetazolamide (10⁻³mol · l⁻¹). In 52 bullfrogs, 1222 sites on the ventral epithelium were tested resulting in 23 locations that exhibited a response to 5% CO₂. Inhibition of CA caused an immediate 65% reduction in the EOG response to CO₂ while the response to amyl acetate was not affected. These results, along with the histochemical localization of CA in some olfactory receptor neurons, indicate that CA plays a role in the detection of CO₂ in frog olfactory neurons and that only a small population of olfactory receptor neurons are CO₂ sensitive. Accepted: 31 July 1997     

Effects of antibodies against odorant binding proteins on electrophysiological responses to odorants

Monoclonal antibodies against two olfactory mucosal proteins, one with affinity for anisole-like and the other for benzaldehyde-like compounds, were applied to mouse olfactory epithelium. Responses to three odorants (anisole, benzaldehyde and amyl acetate) were measured. Of 26 antibodies, three (12%) inhibited responses only to the odorant with affinity for the antigen, nine (35%) inhibited responses to all three odorants, and 14 (54%) were without effect. None reduced responses by as much as 50%. The data support the hypothesis that there is a class of related proteins in olfactory neuronal cell membranes that function as receptor molecules and that other mechanisms also mediate odorant stimulation.     

Physiological and Histological Recovery of the Olfactory Mucosa of the Frog After a Dichlobenil Injection

Four days after a single systemic injection of 50 mg/kg of dichlobenil(2,6-dichlorobenzonitrile), the olfactory neuroepithelium ofthe frog is extensively damaged. At the same time, electrophysiologicalresponses to odorant stimulations (2-heptanone, D-limonene,amyl acetate, camphor) are largely reduced. Pretreatment ofthe animals with metyrapone, an inhibitor of cytochrome P-450enzymatic systems, inhibits the histological and physiologicaltoxic effects of the dichlobenil injection. The olfactory tissuerecovered 3months after the dichlobenil injections and responsesto odorant stimulations returned. The same dichlobenil injectionsdid not induce lesions in the vomeronasal neuroepithelium. Chem.Senses 20: 433–440, 1995.     

Degenerative and regenerative processes in the olfactory system of homing pigeons.

Experimental resection of the olfactory nerve in the homing pigeon induces a total degeneration of the nerve and olfactory epithelium. The orthograde degenerative process starts before the retrograde one. Ten days after resection, new neurons begin to differentiate from the basal cells. The axon forms earlier than the distal dendritic process, and the speed of growth increases slowly. The regenerated axons only reach the bulb in the 5th month. Two months after resection the olfactory epithelium is similar to that of the intact control side. The ultrastructural features of the mucosa and olfactory axons are similar to those of normal ones.     

Olfactory event-related potentials in young and elderly adults: evaluation of tracking task versus eyes open/closed recording.

The purpose of the present study was to evaluate olfactory event-related potentials (OERPs) elicited by amyl acetate from subjects performing a visuomotor tracking task compared with the no-task conditions of eyes open and eyes closed. Task condition did not produce any reliable effects for any amplitude measure. Task type weakly influenced only P2 latency. Elder adults evinced smaller P2 and N1/P2 amplitudes and longer N1 and P2 latencies than young adults. The results suggest that tracking task performance is not necessary to obtain robust OERPs from normal subjects of a wide age range.     

'Microsmatic' primates revisited: olfactory sensitivity in the squirrel monkey

Using a conditioning paradigm, the olfactory sensitivity of three squirrel monkeys to nine odorants representing different chemical classes as well as members of a homologous series of substances was investigated. The animals significantly discriminated dilutions as low as 1:10,000 n-propionic acid, 1:30,000 n-butanoic acid and n-pentanoic acid, 1:100,000 n-hexanoic acid, 1:1Mio n-heptanoic acid, 1:30, 000 1-pentanol, 1:300,000 1,8-cineole, 1:1Mio n-heptanal and 1:30Mio amyl acetate from the near-odorless solvent, with single individuals scoring even slightly better. The results showed (i) the squirrel monkey to have an unexpectedly high olfactory sensitivity, which for some substances matches or even is better than that of species such as the rat or the dog, and (ii) a significant negative correlation between perceptibility in terms of olfactory detection thresholds and carbon chain length of carboxylic acids. These findings support the assumptions that olfaction may play a significant and hitherto underestimated role in the regulation of primate behavior, and that the concept of primates as primarily visual and 'microsmatic' animals needs to be revised.     

Biofiltration of ethyl acetate and amyl acetate using a composite bead biofilter

Biodegradation kinetic behaviors of ethyl acetate and amyl acetate in a composite bead biofilter were investigated. The composite bead was the spherical PVA/peat/KNO(3)/GAC composite bead which was prepared in our previous works. Both microbial growth rate and biochemical reaction rate were inhibited at higher inlet concentration. For the microbial growth process, the microbial growth rate of ethyl acetate was greater than that of amyl acetate in the inlet concentration range of 100-400ppm. The degree of inhibitive effect was almost the same for ethyl acetate and amyl acetate in this concentration range. The half-saturation constant K(s) values of ethyl acetate and amyl acetate were 16.26 and 12.65ppm, respectively. The maximum reaction rate V(m) values of ethyl acetate and amyl acetate were 4.08 and 3.53gCh(-1)kg(-1) packed material, respectively. Zero-order kinetic with the diffusion limitation could be regarded as the most adequate biochemical reaction model. For the biochemical reaction process, the biochemical reaction rate of ethyl acetate was greater than that of amyl acetate in the inlet concentration range of 100-400ppm. The inhibitive effect for ethyl acetate was more pronounced than that for AA in this concentration range. The maximum elimination capacity of ethyl acetate and amyl acetate were 82.3 and 37.93gCh(-1)m(-3) bed volume, respectively. Ethyl acetate degraded by microbial was easier than amyl acetate did.     

The participation of the cAMP intracellular signal system in the olfactory transduction of camphor and amyl alcohol]

In the frog isolated olfactory epithelium, the cAMP intracellular signal system was shown to take part in olfactory transduction of amyl alcohol but not camphor.     

Electrophysiological characterization of olfactory cell types in the antennae and palps of the housefly

A set of odours was presented to the housefly Musca domestica and the electrophysiological responses of single olfactory receptor cells in the antennae and palps were recorded. The olfactory cells in the antennae of the housefly showed a large variability of response profiles, but multidimensional cluster analysis suggested a moderate clustering in olfactory response types. Receptor cells with similar or with different odour response profiles can reside in one and the same sensillum. No fixed spatial distribution of olfactory response types over the antennal of palpal surface was found. The odours of 1-octen-3-ol, amyl acetate, 3-methylphenol, 2-pentanone and R(+)limonene elicited the largest responses in antennal cells. Most odours elicited responses in cells of only a few of the clusters, but 1-octen-3-ol was detected by cells of almost all clusters of the antenna. Surprisingly, rather low responses were found to acetic acid, skatole, indole and muscalure, odours that are known to attract flies. Response profiles of palpal cells differed considerably from those of antennal cells. Palpal cells mostly responded to 3-methylphenol and 2-pentanone. In the palps, the clusters of cells responding to 3-methylphenol and 2-pentanone are clearly separated from the other olfactory cells.     

Sensitivity to odours in the embryo of the domestic fowl

Sensitivity to odours in the embryo of the domestic fowl was investigated on the day before hatching. Embryos were tested with four odorants: dichloroethane, cineole, amyl acetate and formic acid. Three odorants (dichloroethane, formic acid and cineole) produced an increase in the heart rate and a rise in the rates of beak-clapping and the first two increased the amount of head-shaking. Odorants had little effect on other types of activity. The response to amyl acetate varied between experiments. Blocking the nostrils with wax abolished the response. Some implications of these results are discussed briefly.