Abstract
This study determined the effects of nitrite on different life stages of the Amazon river prawn Macrobrachium amazonicum. Prawns of each life stage (postlarvae, juveniles and adults) were stocked in 24 experimental units (n = 10 prawns), under a complete randomized design. Individuals were exposed to nitrite (0, 1, 2, 4, 8 and 16 mg L−1). The median lethal concentration after 96 h (96 h LC50) was calculated through the Weibull I. The mortality results showed that M. amazonicum is slightly less tolerant to nitrite than other species of Macrobrachium. The 96 h LC50 for postlarvae, juveniles and adults of M. amazonicum were of 1.49, 2.36 and 2.34 mg nitrite/L, respectively. Nitrite intoxication risk quotient suggest moderated risk to low risk to the species. Usually in production systems nitrite values are lower than safe levels suggested in this study (0.1 mg L−1 to postlarvae and 0.2 mg L−1 nitrite to juvenile and adults), which makes our results appropriate for the production of this species.
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Freshwater prawn farming has shown great increase worldwide in the last two decades (FAO 2014; Hayd et al. 2014). Although the main reared prawn in Brazil is still the exotic species Macrobrachium rosenbergii, the indigenous species M. amazonicum has demonstrated similar production potential (Moraes-Valenti et al. 2010). The production of native species is essential for the conservational aspect of good aquacultural practices. Production of native species of prawns has become a trend, as the production of Macrobrachium nipponense in China (Kutty and Weimin 2010) and Macrobrachium malcolmsonii in India (Kutty 2005; Kutty and Valenti 2010). This practice prevents possible problems caused by the introduction of exotic species in the environment (Bridger and Garber 2002), besides reducing the uncontrolled exploitation caused by fishing (Silva et al. 2007).
Physiological processes of aquatic organisms, decomposition of organic matter, and food leftovers are the main sources of nitrogen compounds in aquaculture production systems (Campos et al. 2012). Nitrite is the intermediate compound in the bacterial nitrification of ammonia to nitrate. It may present high toxicity, depending on its concentration in the environment and organism developmental stage (larvae to adult) (Miranda-Filho et al. 1995). Several studies with M. amazonicum were already carried out to better understand its biology (Boudour-Boucheker et al. 2013; Meireles et al. 2013), ecology (Moreira and Collart 1993; Dutra et al. 2014), and production features (Anger and Hayd 2010; Moraes-Valenti et al. 2010). However, studies on nitrite effects available in the literature are limited to larvae (Hayd et al. 2014), since the studies to cultured shrimps are mainly focused on penaeids (e.g., Cheng and Chen 2002; Chen and Cheng 2000). Mallasen and Valenti (2006) recommend nitrite values below 2.0 mg L−1 in the production of freshwater prawns.
Therefore, based on the hypothesis that the early stages of development of M. amazonicum are more sensitive to nitrite than later stages, the aim of the study was to assess the effect of nitrite on different life stages of the Amazon river prawn—Macrobrachium amazonicum, Heller, 1862, through the determination of 96 h LC50 concentrations of nitrite. To determine LC50 values, the prawns were submitted to six different nitrite concentrations (0, 1, 2, 4, 8 and 16 mg nitrite/L) in four replicates, during 96 h. Afterwards, the mortalities were assessed for each life stage (postlarvae, juveniles and adults).
Materials and Methods
The experimental work described here was conducted at the Prawn Culture Laboratory, located at the Federal University of Paraná—Sector Palotina, with animals provided by the Laboratory of Prawn Culture of the CA-UNESP (Universidade Estadual Paulista “Julio de Mesquita Filho”). The experiments used 240 prawns of each life stage (postlarvae, juveniles and adults). The prawns reach the post-larvae stage after they go through all larval development (nine different stages from zoea I to zoea IX), the juvenile stage is reached approximately 30 days after they reach the post-larvae stage and the prawns are considered adults when they reach the reproductive stage and can be identified through the gonadal development (Vega-Villasante and Carrillo 2006; New et al. 2010). The prawns were randomly divided into 24 experimental units, with 10 prawns in each experimental unit. The wet weight and the total length (rostrum to telson) were measured in postlarvae (0.088 ± 0.022 g; 2.250 ± 0.170 cm, mean ± SD), juveniles (2.023 ± 0.271 g; 6.729 ± 0.296 cm) and adults (6.240 ± 1.827 g; 9.084 ± 0.793 cm); n = 50 out of the 240 used, randomly chosen. As experimental units we chose beakers with a volume of 1 L to post larvae, or glass aquaria containing 10 L of useful volume to juveniles and adults. Experimental units were equipped with aeration systems and light sources for a light:dark rhythm of 12:12 h, in a climate-controlled room (25–27 °C). The design was completely randomized, with six different nitrite concentrations (0, 1, 2, 4, 8, and 16 mg nitrite/L), and four replicates per nitrite concentration. The nitrite levels resulted from the addition of appropriate volumes of the stock solution of NaNO2 PA—Synth® (stock solution of 250 mg nitrite/L) to produce the desired final nitrite concentrations. The concentrations used were based on work done with M. rosenbergii (Mallasen and Valenti 2006). Mortality was assessed by total absence of movement or reaction to mechanical stimuli using a glass rod. Prawns were observed every 1 h for the first 8 h. Between 8 h and 96 h, observations were performed every 12 h (Armstrong et al. 1976).
The following variables of water quality were daily evaluated: dissolved oxygen (Oxymeter, Hanna HI 9146), temperature (digital thermometer Incoterm), and pH (Phmeter, Tekna T-100). At the beginning and at the end of the experiment, alkalinity and hardness of water samples were assayed by titration. Total ammonia levels were determined according to Koroleff (1976), where the sample containing ammonia reacts with phenol and sodium hypochlorite in alkaline solution to form a blue color solution which is catalyzed by sodium nitroprusside. The resulting absorbance was measured in a spectrophotometer (BEL photonics 2000UV, Brazil) at 630 nm. Nitrite and nitrate levels were determined according to Mackereth et al. (1978). The nitrite concentration was determined through the formation of a purple-red solution formed by diazotization of sulfanilic acid with N-(1-naphthyl)-ethylenediamine dihydrochloride. The resulting absorbance was measured at 540 nm. Nitrate concentration was determined through the reduction of nitrate to nitrite by amalgamated cadmium. The resulting concentration (nitrite originally present in the sample plus reduced nitrate) was measured according to the methodology described above for nitrite. The concentration of nitrite originally present was subtracted from the total concentration of nitrite obtained. The nitrogenous compounds were detected and measured in a spectrophotometer, at detection limit of 0.02 mg L−1 (lower limit), 0.005 mg L−1, and 0.05 mg L−1 to ammonia, nitrite and nitrate, respectively. Afterwards, absorbance data were read against a standard curve to calculate the concentrations of the different nitrogenous compounds in the samples using the software “win-spec” (version 2.3.1). As standard compounds to determine the standard curve of ammonia, nitrite and nitrate were used ammonium chloride, sodium nitrite and potassium nitrate, respectively. Water quality variables were determined independently for each treatment in order to establish whether they remained at appropriate levels for the species (Moraes-Valenti and Valenti 2010).
The determination of the median lethal concentration (96 h LC50) was based on the manual of the Environmental Protection Agency USA (Peltier and Weber 1985). The safe level (SL) was determined by multiplying the value obtained in the test of toxicity by an application factor of 0.1, as recommended by Sprague (1971).
Scatter plots were built between the nitrite concentration (mg L−1) and the cumulative mortality for post larvae, juveniles and adults separately. Various dose–response models were tested and the best fit was achieved with the Weibull I function (Ritz et al. 2015). The choice of the “best fit” was based on the values of standard error (S) and of the coefficient of determination (r²), on the residual analysis (Sokal and Rholf 1995) and of the biological adequacy.
The intoxication risk classification by nitrite was performed by quotient method, adapted of Urban and Cook (1986). The quotient was calculated by ratio between the recommended concentration in literature to the genus Macrobrachium and the 96 h LC50 calculated value to species in study. We used the following intoxication risk classes: without risk (Q ≤ 0.1); low risk (0.1 < Q ≤ 1); moderated risk (1 < Q ≤ 10) and high risk (Q > 10).
Results and Discussion
During the experiment, temperature, pH, water hardness and alkalinity remained within suitable ranges for freshwater prawns culture (Coler et al. 1999; Sampaio et al. 2007; Vasquez et al. 2007). Ammonia concentrations measured here were lower than those levels suggested by Timmons et al. (2002), who recommended a threshold value for ammonia of 2 mg L−1 in warm water aquaculture. In the same way, the nitrate concentrations were lower than those levels recommended by Moraes-Valenti and Valenti (2010), who suggested that nitrate values should not reach levels above 80 mg L−1 (Table 1). Therefore, none of the water quality parameters measured in this study, except nitrite, were limiting or stressful for the prawns. Thus, it can be argued that the lethal effects observed were due to the nitrite concentrations evaluated.
Mortality observed for the different life stages at the control treatment (not exposed to nitrite) during the trial period was below 10 %, which may be related to the behavior of animals in competition for area (territorialism), as demonstrated in previous research (Armstrong et al. 1976; Ostrensky and Wasielesky Jr. 1995).
Independently of the life stage of prawns, it is possible to verify that mortality increased with increasing nitrite concentration. Postlarvae of M. amazonicum exposed to nitrite showed 48 ± 2 % (mean ± SD) mortality after 96 h of exposure to 1 mg nitrite/L. The concentration of 2 mg L−1 yields mortality of 90 ± 2 % in 96 h. At the concentrations of 4–16 mg nitrite/L, mortality was of 100 % in 24 h. When evaluating mortality caused by nitrite by the Weibull I function, the lethal concentration for 50 % of the prawns (LC50) after 96 h is 1.49 mg nitrite/L (Table 2; Fig. 1a).
Juvenile M. amazonicum exposed to concentrations of 2 mg L−1 and 4 mg L−1 showed average mortality of 55 ± 3 and of 95 ± 1 % after 96 h, respectively. Concentrations of 8–16 mg nitrite/L exhibited 100 % mortality after 24 h. Lethal concentration for 50 % of the juveniles in 96 h was 2.36 mg nitrite/L (Table 2; Fig. 1b).
For adult M. amazonicum, the concentrations of 1 and 2 mg L−1 produced average mortality of 27 ± 8 and 50 ± 8 % in 96 h, respectively. Concentration of 4 mg L−1 caused average mortality of 80 ± 3 % in 96 h. 100 % mortality was also observed at 8–16 mg nitrite/L in 24 h. Average mortality for 50 % of the adults after 96 h is obtained with 2.34 mg nitrite/L (Table 2; Fig. 1c). Sahoo and Chand (2006), evaluating the effect of nitrite on the immune response of adult Macrobrachium malcolmsonii, measured a LC50 of 3.14 mg L−1 after 96 h. Thus, it seems that M. amazonicum adults are slightly less tolerant to nitrite than M. malcolmsonii adults as it shows lower LC50 values: 2.34 mg L−1. Mallasen and Valenti (2006) recommend nitrite values during the production of freshwater prawns below 2.0 mg L−1. Hayd et al. (2014) claim that safe levels below 0.8 mg nitrite/L may be used as a general reference for production system. However, in the present study results pointed out that the safe levels for the production of M. amazonicum are much lower (0.14–0.23 mg L−1) (Table 2).
Regarding the classification of intoxication risk by nitrite to M. amazonicum, the values were of 1.34 to postlarvae, 0.85 to juveniles and 0.85 to adults, suggesting moderated risk to postlarvae and low risk to juvenile and adult (Urban and Cook 1986).
Comparing sensitivity to nitrite in the different life stages of M. amazonicum, it was found that the sensitivity to this compound is related to the animal’s stage of development, where the later stages showed higher resistance. The sensitivity of an organism to a toxic agent can vary depending on its size, age and stage of development (Wajsbrot et al. 1990), because several enzymes may have differential activities along development or aging (Barbieri et al. 2002). In the early stages of development the organisms are more sensitive generally due to increased mitotic activity (Barbieri 2008), and also possibly their higher surface to volume ratios, as they are smaller organisms. This variation in sensitivity of different ontogenetic stages has been observed previously in Macrobrachium, in studies with other compounds such as pesticides (Dai et al. 2014), heavy metals (Asih et al. 2013) and nitrogen compounds (ammonia and nitrite) (Lin et al. 1993; Mallasen and Valenti 2005, 2006).
In production systems, the nitrite values generally are below the safe limit determined in this study. Marques et al. (2012) observed in production systems in net pens nitrite values ranging from 0.004 to 0.011 mg L−1; Kimpara et al. (2011) found in ponds values ranging from 0.026 to 0.028 mg nitrite/L, while the recommended nitrite limits here are of 0.1 mg L−1 for post larvae and 0.2 mg L−1 for juveniles and adults. Thus, the results obtained have important implications for the production of this prawn and allow the indication of precise limit levels for the exposure of the different life stages of this species to nitrite, enabling the handling and management of these animals in production systems. Thus, monitoring this variable is important to avoid losses, mainly in larviculture and recirculation systems.
References
Anger K, Hayd L (2010) Feeding and growth in early larval shrimp Macrobrachium amazonicum from the Pantanal, southwestern Brazil. Aquat Biol 9:251–261. doi:10.3354/ab00259
Armstrong DA, Stephenson MJ, Knight AW (1976) Acute toxicity of nitrite to larvae of the giant Malaysian prawn, Macrobrachium rosenbergii. Aquaculture 9:39–46. doi:10.1016/0044-8486(76)90046-6
Asih AYP, Irawan B, Soegianto A (2013) Effect of copper on survival, osmoregulation, and gill structures of freshwater prawn (Macrobrachium rosenbergii, de Man) at different development stages. Marine Freshw Behav Physiol 46:75–88. doi:10.1080/10236244.2013.793471
Barbieri E (2008) Efeito dos Surfactantes DSS e LAS-C12 sobre o Camarão-rosa (Farfantepenaeus paulensi, Pérez-Farfante, 1967). J Braz Soc Ecotoxicol 3:35–40. doi:10.5132/jbse.2008.01.005
Barbieri E, Oliveira IR, Serralheiro PAC (2002) The use of metabolism to evaluate the toxicity of dodecyl benzen sodium sulfonate (LAS-C12) on the Mugil platanus according to the temperature and salinity. J Exp Mar Biol Ecol 277:109–127. doi:10.1016/S0022-0981(02)00236-8
Boudour-Boucheker N, Boulo V, Lorin-Nebel C, Elguero C, Grousset E, Anger K, Charmantier G (2013) Adaptation to freshwater in the palaemonid shrimp Macrobrachium amazonicum: comparative ontogeny of osmoregulatory organs. Cell Tissue Res 353:87–98. doi:10.1007/x-s00441-013-1622
Bridger CJ, Garber AF (2002) Aquacultre escapement, implications and mitigation: the salmonid case study. In: Costa-Pierce BA (ed) Ecological aquaculture the evolution of the blue revolution. Wiley-Blackwell, Oxford, pp 77–102. doi:10.1002/9780470995051.ch4
Campos BR, Miranda Filho KC, D’Incao F, Poersch L, Wasielesky W (2012) Toxicidade aguda da amônia, nitrito, nitrato sobre os juvenis de camarão rosa Farfatepenaeus brasiliensis (Latreille, 1817) (Crustacea: Decapoda). Atlanta, Rio Grande 34:75–81
Chand RK, Sahoo PK (2006) Effect of nitrite on the immune response of freshwater prawn Macrobrachium malcolmsonii and its susceptibility to Aeromonas hydrophila. Aquaculture 258:150–156. doi:10.1016/j.aquaculture.2006.05.001
Chen JC, Cheng SY (2000) Recovery of Penaeus monodon from functional anaemia after exposure to sublethal concentration of nitrite at different pH levels. Aquat Toxicol 50:73–83. doi:10.1016/S0166-445X(99)00093-4
Cheng SY, Chen JC (2002) Joint action of elevated ambient nitrite and nitrate on hemolymph nitrogenous compounds and nitrogen excretion of tiger shrimp Penaeus monodon. Comp Biochem Physiol 131:303–314. doi:10.1016/S1532-0456(02)00004-2
Coler RA, Watanable T, Xavier BF, Paz RJ (1999) A preliminary report on the application of Macrobrachium amazonicum Heller, 1862 (Decapoda: Palaemonidae) as a biomarker. Hydrobiologia 412:119–121. doi:10.1023/A:1003864702924
Dai X, Xiong Z, Xie J, Ding F (2014) Acute toxicity of organochlorine insecticide endosulfan to the giant freshwater prawn Macrobrochium rosenbergii. Chin J Oceanol Limnol 32:111–119. doi:10.1007/s00343-014-3081-y
Dutra FM, Moretto Y, Portz L, Ballester ELC (2014) Pen culture of, Macrobrachium amazonicum: use of artificial diet and impact on benthic community. Aquac Res. doi:10.1111/are.12488
FAO—Food and Agriculture Organization of the United Nations (2014) The state of world fisheries and aquaculture. http://www.fao.org/3/d1eaa9a1-5a71-4e42-86c0-f2111f07de16/i3720e.pdf. Accessed 11 April 2015
Hayd LA, Lemos D, Valenti WC (2014) Effects of ambient nitrite on Amazon river prawn, Macrobrachium amazonicum, larvae. J World Aquac Soc 45:55–64. doi:10.1111/jwas.12071
Kimpara JM, Rosa FRT, Preto BL, Valenti WC (2011) Limnology of Macrobrachium amazonicum grow-out ponds subject to high inflow of nutrient-rich water and different stocking and harvest management. Aquac Res 42:1289–1297. doi:10.1111/j.1365-2109.2010.02717.x
Koroleff F (1976) Determination of nutrients. In: Grasshoff K (ed) Methods of seawater analysis. Verlag Chemie, Weinheim, pp 117–181
Kutty MN (2005) Towards sustainable freshwater prawn aquaculture - lessons from shrimp farming, with special reference to India. Aquac Res 36:255–263. doi:10.1111/j.1365-2109.2005.01240.x
Kutty MN, Valenti WC (2010) Culture of other freshwater prawn species. In: New MB, Valenti WC, Tidwell JH, D’Abramo LR, Kutty MN (eds) Freshwater prawns: biology and farming. Wiley-Blackwell, Oxford, pp 502–523. doi:10.1002/9781444314649.ch23
Kutty MN, Weimin M (2010) Culture of the Oriental river prawn Macrobrachium nipponense. In: New MB, Valenti WC, Tidwell JH, D’Abramo LR, Kutt MN (eds) Freshwater prawns: biology and farming. Wiley-Blackwell, Oxford, pp 475–484. doi:10.1002/9781444314649.ch21
Lin H-P, Thuet P, Trilles J-P, Mounet-Guillaume R, Charmantier G (1993) Effects of ammonia on survival and osmoregulation of various development stages of the shrimp Penaeus japonicus. Marine Biol 117:591–598. doi:10.1007/BF00349770
Mackereth FJH, Heron J, Talling JF (1978) Water analysis some revised methods for limnology. Freshwater Biological Association Scientific Publication, London
Mallasen M, Valenti WC (2005) Larval development of the giant river prawn Macrobrachium rosenbergii at different ammonia concentrations and pH values. J World Aquac Soc 36:32–41. doi:10.1111/j.1749-7345.2005.tb00128.x
Mallasen M, Valenti WC (2006) Effect of nitrite on larval development of giant river prawn Macrobrachium rosenbergii. Aquaculture 261:1292–1298. doi:10.1016/j.aquaculture.2006.07.048
Marques HLA, Barros HP, Mallasen M, Boock MV, Moraes-Valenti PMC (2012) Influence of stocking densities in the nursery phase on the growth of Macrobrachium amazonicum reared in net pens. Aquaculture 358–359:240–245. doi:10.1016/j.aquaculture.2012.06.011
Meireles AL, Valenti WC, Mantelatto FL (2013) Reproductive variability of the Amazon River prawn, Macrobrachium amazonicum (Caridea, Palaemonidae): influence of life cycle on egg production. Latin Am J Aquat Res 41:718–731
Miranda-Filho K, Wasielesky-Jr WB, Maçada A (1995) Efeito da amônia e nitrito no crescimento da tainha Mugil platanus (Pisces, Mugilidae). Rev Bras Biol 55:45–50
Moraes-Valenti PMC, Valenti WC (2010) Culture of the Amazon river prawn Macrobrachium amazonicum. In: New MB, Valenti WC, Tidwell JH, D’Abramo LR, Kutt MN (eds) Freshwater prawns: biology and farming. Wiley-Blackwell, Oxford, pp 485–501. doi:10.1002/9781444314649.ch22
Moraes-Valenti PMC, Moraes PA, Preto BL, Valenti WC (2010) Effect of density on population development in the Amazon river prawn Macrobrachium amazonicum. Aquat Biol 9:291–301. doi:10.3354/ab00261
Moreira LC, Collart OO (1993) Migraçao vertical nictemeral das larvas de Macrobrachium amazonicum num lago de varzea na Amazonia central, Ilha do Careiro, Brasil. Amazoniana 12:385–398
New MB, Valenti WC, Tidwell JH, D’Abramo LR, Kutty MN (eds) (2010) Freshwater prawns: biology and farming. Wiley-Blackwell, Oxford. doi:10.1002/9781444314649
Ostrensky A, Wasielesky W Jr (1995) Acute toxicity of ammonia to various life stages of the São Paulo shrimp, Penaeus paulensis. Pérez-Farfante, 1967. Aquaculture 132:339–347
Peltier WH, Weber Cl (1985) Methods for measuring the acute toxicity of effluents to freshwater and marine organisms, 3rd edn. EPA/600/4–85/013, Environmental Protection Agency, Cincinnati
Ritz C, Baty F, Streibig JC, Gerhard D (2015) Dose-response analysis using R. Plos One 10:1–13. doi:10.1371/journal.pone.0146021
Sampaio CMS, Silva RR, Santos JA, Sales SP (2007) Reproductive cycle of Macrobrachium amazonicum females (Crustacea, Palaemonidae). Braz J Biol 67:551–559. doi:10.1590/S1519-69842007000300022
Silva MCN, Frédou F, Filho JSR (2007) Estudo do crescimento do camarão Macrobrachium amazonicum (HELLER, 1862) da ilha de Combú, Belém, Estado do Pará. Amazônia Ci Desenv Belém 2:85–104. (Abstract in English)
Sokal RR, Rohlf FJ (1995) Biometry, 3th. W. H. Freeman and company, New York
Sprague JB (1971) Measurement of polltant toxicity to fish-III: sublethal effects and “safe” concetracions. Water Res Pergamon Press 5:245–266. doi:10.1016/0043-1354(71)90171-0
Timmons MB, Ebeling JM, Weathon FW, Summerfelt ST, Vinci BJ (2002) Recirculating aquaculture system, 2nd edn. Cayuga aqua ventures, Ithaca
Urban DJ, Cook NJ (1986) Hazard evaluation division - standard evaluation procedure ecological risk assessment. USEPA Public, Washington. 540/9:86–001
Vasquez OE, Rouse DB, Rogers WA (2007) Growth response of Macrobrachium rosenbergii to different levels of hardness. J World Aquac Soc 20:90–92. doi:10.1111/j.1749-7345.1989.tb00528.x
Vega-Villasante F, Carrillo OC (2006) El dicamarón: diccionario de camaronicultura. Universidad de Guadalajara, Guadalajara
Wajsbrot N, Gasith A, Krom MD, Samocha TM (1990) Effect of dissolved oxygen and the molt stage on the acute toxicity of ammonia to juvenile green tiger prawn Penaeus semisulcatus. Toxicol Environ Chem 9:497–504. doi:10.1002/etc.5620090413
Acknowledgments
Authors would like to thank the Laboratory of prawn culture of the CA-UNESP in Jaboticabal, for the donation of the M. amazonicum. Authors also thank the financing from the CAPES and CNPq, and the Sponsor of Studies and Projects of the Ministry of Science and Technology (FINEP) and Ministry of Education (MEC/ProExt). Carolina Arruda Freire and Eduardo Luis Cupertino Ballester are research fellows of National Council for the Development of Science and Technology of Brazil (CNPq) also gratefully acknowledged.
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Dutra, F.M., Freire, C.A., Vaz dos Santos, A.M. et al. Acute Toxicity of Nitrite to Various Life Stages of the Amazon River Prawn, Macrobrachium amazonicum, Heller, 1862. Bull Environ Contam Toxicol 97, 619–625 (2016). https://doi.org/10.1007/s00128-016-1932-2
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DOI: https://doi.org/10.1007/s00128-016-1932-2