Ventilatory frequency and anesthetic efficacy in silver catfish, Rhamdia quelen: a comparative approach between different essential oils

This study investigated the efficacy of essential oils of Lippia alba (EOLA) citral chemotype and Lippia origanoides (EOLO) and their effects on ventilatory frequency (VF) of silver catfish, Rhamdia quelen. Fish were exposed to 50-300 μL L−1 of EOLA and 25-300 μL L−1 of EOLO to determine induction times to sedation, anesthesia, and recovery. Moreover, VF was determined in fish exposed to 5 or 10 μL L−1 of EOLA and of EOLO for 8 h. The increasing concentration of essential oils proportionally decreased sedation and anesthesia induction times. The highest EOLA concentration increased VF of fish from the control group at 1 h of exposure, but VF decreased at both EOLO concentrations after 2 h. The EOLA citral chemotype and EOLO were effective sedatives and anesthetics for silver catfish. However, EOLO was the most suitable sedative for additional studies regarding fish transport as it reduced VF and did not induce VF increase in silver catfish. The EOLA citral chemotype and EOLO are effective sedatives and anesthetics for silver catfish. Moreover, the EOLO is recommended for transport of silver catfish, because it maintains the ventilatory frequency constant, avoiding a possible metabolic stress.

Therefore, the present study is the first to report the efficacy of EO of L. origanoides (EOLO) and EOLA as anesthetics in fish.Moreover, we analyzed ventilatory frequency to help understand the effects of these EO on fish behavior.
Dissolved oxygen and temperature were determined with a YSI oxygen meter (Model Y5512; YSI Inc., Yellow Springs, OH, USA); pH, with a DMPH-2 pH meter (Digimed, SP, Brazil); alkalinity, according to Boyd and Tucker (1992); total ammonia nitrogen levels, through the salicylate method (Verdouw et al., 1978); and un-ionized ammonia was obtained from a conversion table for fresh water.
The methodology of this experiment was approved by the local Ethical and Animal Welfare Committee (case no.046/2010).
Leaves of L. alba were collected in Santarém (Pará, Brazil) in June 2012, and identification was performed by Dr. Fátima Salimena (voucher number CESJ 65276, Universidade Federal de Juiz de Fora, Minas Gerais, Brazil).Leaves of L. origanoides were collected in August 2008 in Alter do Chão (Santarém, Pará, Brazil), also identified by Dr. Salimena, and the voucher was deposited in Empresa Brasileira de Pesquisa Agropecuária (EMBRAPA) under the number IAN 184688.
Extraction of EO was performed by hydrodistillation for 3 or 6 h through a Clevenger-type apparatus (European Pharmacopoeia, 2007).About 100 g of fresh leaves were immersed in distilled water at a ratio of 1:10 (w/v), and the oil was separated from water after reaching room temperature.Average yield was 1.4% EOLA and 2.7% EOLO.Essential oils were transferred to glass flasks, filled to the top, and kept at a temperature of 10 ºC for further analysis.
Analysis of EOLA and EOLO by gas chromatographymass spectrometry-thin ion chromatography was performed using an Agilent-6890 gas chromatograph coupled with an Agilent 5973 mass selective detector with a HP5-MS column (5% phenyl, 95% methylsiloxane, 30 m × 0.25 mm i.d.× 0.25 µm) as described by Silva et al. (2012).The chemical constituents of these EO were identified by comparison of the Kovats retention index and mass spectra with a mass spectral library and literature data (NIST/EPA/NIH, 2005; Adams, 2007;Mondello, 2011).
Fish were transferred to 1-L aquaria (n = 10 each concentration) and exposed to the following EO concentrations (in µL L −1 ): 50,100,150,200,and 300 of EOLA and 25,50,100,200, and 300 of EOLO.All EO were previously diluted in ethanol (1:10).The concentrations tested were slightly different between the EO because their efficacy was variable (see results).Induction times of sedation and anesthesia as well as recovery were evaluated, and anesthesia stages were characterized as described by Small (2003), with a maximum observation time of 30 min.Silver catfish were placed in an aquarium with anestheticfree water for recovery.We used a digital chronometer to record all times, expressed in seconds.
The second experiment determined ventilatory frequency (VF) using concentrations with potential application in transporting procedures.Ventilatory frequency was quantified at 0, 0.25, 1, 2, 4, and 8 h of exposure, as reported by Alvarenga and Volpato (1995): visual count of 20 successive buccal or opercular movements, recording the elapsed time with a digital chronometer.We used the following EO concentrations (previously diluted in ethanol and expressed in µL L −1 ): 5 or 10 for EOLA and 5 or 10 for EOLO.Moreover, water (control) and ethanol groups were evaluated.
All results were expressed as mean±SEM.Evaluation of anesthetic activity was performed by regression analysis (concentration × time of anesthesia induction; concentration × time of recovery from anesthesia), using the SigmaPlot version 11.0 software.The homogeneity of variances of VF data was tested with Levene's test.These data did not show homoscedasticity and were subjected to Kruskal-Wallis ANOVA, followed by multiple comparisons of mean ranks for all groups.The software used was Statistica 7.0 (Stat Soft, Tulsa, OK), and the minimum significance level was set at P<0.05.
Ventilatory frequency of the control group decreased significantly 15 min after fish were placed in the aquaria and kept unchanged for 8 h.Silver catfish exposed to ethanol also progressively reduced VF up to 4 h, with significantly higher values than those for control fish after exposure of 15 min to 1 h.Fish exposed to EOLA presented lower VF than control and/or ethanol groups in some measurements, but the highest EOLA concentration also increased VF at 1 h.Ventilatory frequency values of fish exposed to both concentrations of EOLO from 15 min to 8 h were significantly lower than those in control and ethanol groups in all measurements, with the exception of 1 h for the highest concentration of EOLO, in which the values were similar to those in the control (Table 2).

Discussion
Essential oil of Lippia alba citral chemotype used in the present study had citral (55.28% geranial + neral) as major constituent, therefore belonging to the citral chemotype (Hennebelle et al., 2008), which was previously observed in another city of Minas Gerais, albeit with a lower citral content (Oliveira et al., 2006).The lowest EOLA concentration used in the present experiment (50 µL L −1 ) sedated silver catfish within 8 min, and a concentration of 200 µL L −1 was needed to anesthetize this species within 3 min, in agreement with the results observed by Souza et al. (2017) in the same species.A. triphylla EO, which has citral as its main compound (72% E-citral + Z-citral) (Parodi et al., 2012) also sedated silver catfish within 8 min at 50 µL L −1 (Parodi et al. 2014), but a concentration of 200 µL L −1 induced anesthesia after 6 to 10 min, depending on fish size (Gressler et al., 2014, Parodi et al., 2014).Even considering fish size, EOLA citral chemotype was more efficient in anesthetizing silver catfish than A. triphylla EO, which can probably be explained by the presence of limonene (around 9%) in EOLA.Limonene is the main compound (97.66%) of the Citrus sinensis EO, which has an anxiolytic effect in Wistar rats (Faturi et al., 2010).
The main compound of EOLO was carvacrol (47.20%), which corresponds to the carvacrol chemotype of L. origanoides (Stashenko et al., 2010).The anesthetic effect of EOLO in silver catfish was expected because,
Figure 1 -Times required for induction and recovery from anesthesia in silver catfish, Rhamdia quelen, exposed to the essential oils of Lippia alba (A) and Lippia origanoides (B).
R. Bras.Zootec., 47:e20170185, 2018 in a study by Silva et al. (2013), L. sidoides EO (67.89% carvacrol) induced anesthesia in this species.Time to induce sedation with the lowest EOLO concentration in this experiment was similar, but time to induce anesthesia (around 1 min with 200-300 µL L −1 ) was much shorter than in the study of Silva et al. (2013) (around 20 min with 150-300 µL L −1 ).In addition, the results of our study differed in several other aspects from those of Silva et al. (2013): we observed no involuntary contractions and jumping behavior toward the surface, and all fish recovered within 10-11 min, even at the highest concentration tested.As carvacrol inhibits acetylcholinesterase activity in vitro (Jukic et al., 2007), Silva et al. (2013) hypothesized that this compound could be mainly responsible for involuntary contractions and jumping behavior of silver catfish exposed to L. sidoides EO.However, carvacrol had an anxiolytic-like effect in one study (Melo et al., 2010) and increased the latency for the development of convulsions in mice (Quintans-Júnior et al., 2010).It also blocks neuronal excitability by a direct inhibition of the voltagegated sodium current (Joca et al., 2012), which is similar to the mechanism of action of eugenol (Cho et al., 2008), an effective anesthetic in silver catfish (Cunha et al., 2010b).Ventilatory frequency of control fish decreased a few minutes after they were placed in aquaria.This was expected, because the presence of the anesthetic in the water may provoke a transitory stress which increases VF levels, as observed previously in this species (Becker et al., 2012).The same was observed in silver catfish exposed to 10-20 µL L −1 EOLA chemotype linalool (Becker et al., 2012).The use of anesthetic concentrations (150-450 µL L −1 ) of EOLA chemotype linalool also induced the same VF response (Toni et al., 2014).The EOLA chemotype citral, used in the present experiment, reduced VF in some measurements.In addition, anesthesia with this EO also prevented the increase of plasma cortisol in silver catfish caused by handling (Souza et al., 2017;2018).However, anesthesia with EOLA citral chemotype increased protein carbonylation levels in the kidney and liver of silver catfish, indicating that this EO may provoke renal and hepatic damage (Souza et al., 2018).There are no studies regarding VF of fish exposed to this EO or to A. triphylla EO.It is therefore not clear if A. triphylla EO reduced metabolism, because, at the end of 5 h of transport of silver catfish, CO 2 levels of the water were lower, but O 2 levels remained unchanged (Parodi et al., 2014).Essentia oil of L. origanoides was the most effective EO to reduce VF and apparently did not induce any initial stress response.

Conclusions
The essential oils of Lippia alba citral chemotype and Lippia origanoides are effective sedatives and anesthetics for silver catfish.Moreover, the essential oils of Lippia origanoides are recommended for transport of silver catfish, because they maintain the ventilatory frequency constant, reducing a possible metabolic stress.

Table 2 -
Effects of the essential oils of Lippia alba (EOLA) and Lippia origanoides (EOLO) on ventilatory frequency (opercular or buccal movements min −1 ) of silver catfish (Rhamdia quelen) -standard error of the mean.Values are means ± SEM.Different uppercase letters in the rows indicate significant differences between groups in the same time (P<0.05).Different lowercase letters in the columns indicate significant differences between times in the same group (P<0.05). SEM