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Genetic Variability of Brycon hilarii in a Repopulation Program

ABSTRACT

Brycon hilarii, popularly called piraputanga in Brazil, is a species distributed throughout the whole basin of the river Paraguay. In recent years, the species has been on a repopulation program due to its remarkable decline as a wild species in the region. Assessment of the genetic diversity of broodstock and fingerling stocks in repopulation programs is basic to avoid genetic impacts on wild populations. The genetic variability of the wild population and of the broodstock and fingerling stocks of B. hilarii in a repopulation program in the river Itiquira MT Brazil will be determined. Seven microsatellite loci produced 52 polymorphic alleles and heterozygosity revealed rates between 0.5794 and 0.7204. FIS did not register any endogamy in the broodstock but it was present in fingerlings and wild populations. Intra- and inter-specific genetic variability rates were higher within each combination but not between groups. Grouping in fingerling groups had a lower density when compared to the others. There is a higher genetic proximity between the natural population and broodstock (0.0237) when the distance between populations was analyzed, even though the two were greatly distant from the fingerling group (0.2622 - 0.2617). Results show that the wild population and the broodstock had high genetic variability and low genetic divergence; contrastingly, fingerlings showed mild genetic variability and great divergence when compared to other groups, indicating that they were not adequately constituted.

Key words:
conservation genetics; microsatellites; piraputanga

INTRODUCTION

Evolutionary characteristics and the integration of anthropic factors resulted in the homogenization of genetic composition and stock reduction of the wild Brycon hilarii. Popularly known as piraputanga in the Brazil, the rheophile fish species is distributed throughout the basin of the river Paraguay and highly appreciated for commercial and sports fishing (Reys et al. 2009Reys P, Sabino J, Galetti M. Frugivory by the fish Brycon hilarii (Characidae) in western Brazil. Acta Oecol. 2009; 35: 136-141. ). However, populations of B. hilarii have decreased throughout the basin (Catella et al. 2014Catella AC, Albuquerque SP, Campos FLR, Santos DC. Control System the Fishing of Mato Grosso do Sul SCPESCA/MS 20-2013. Corumbá: Embrapa Pantanal; 2014.), probably due to excessive fishing and anthropic activities, such as the construction of hydroelectric dams, transposition of the riverbed and pollution.

Repopulation programs may not only help in the reconstruction of populations but even minimize impacts on the abundance of several fish species caused by excessive fishing and the destruction of their natural habitat. However, genetic repercussions caused by the introduction of other specimens over the wild population structure should be taken into account (Laikre et al. 2010Laikre L, Schwartz MK, Waples RS, Ryman N. Compromising genetic diversity in the wild: unmonitored large-scale release of plants and animals. Trends Ecol Evol. 2010; 25(9): 520-529. ; González-Wangüemert et al. 2012González-Wangüemert M, Fernández TV, Pérez-Ruzafa A, Giacalone M, D'Anna G, Badalamenti F. Genetic considerations on the introduction of farmed fish in marine protected areas: The case of study of white seabream restocking in the Gulf of Castellammare (Southern Tyrrhenian Sea). J Sea Res. 2012; 68: 41-48. ). The genetic characteristics of fish groups released in certain environments through repopulation program are highly relevant due to the genetic impact on wild populations. Genetic interaction among the fish released and wild populations may cause loss of alleles, especially those related to adaptation (Povh et al. 2008Povh JA, Ribeiro RP, Sirol RN, Streit Jr DP, Lopera-Barrero NM, Vargas L, et al. Genetic diversity of pacu from the Paranapanema River and from the broodstock of a stock enhancement program. Pesq Agropec Bras. 2008; 43(2): 201-206. ).

Molecular markers, especially microsatellites, have been widely used for information on the genetic variability of broodstocks and wild populations (Povh et al. 2011Povh JA, Ribeiro RP, Lopera-Barrero NM, Jacometo CB, Vargas L, Gomes PC, et al. Microsatellite analysis of pacu broodstocks used in the stocking program of Paranapanema river. Sci Agric. 2011; 68(3): 308-313. ; Almeida et al. 2013Almeida FSD, Lopes CM, Orsi ML, Sirol RN, Sodré LMK. Genetic monitoring by rapid markers for repopulation programs of Salminus brasiliensis (Pisces, Characiformes). Acta Sci Anim Sci. 2013; 35(2): 119-126. ; Lopera-Barrero et al. 2015Lopera-Barrero NM, Santos SCA, Rodríguez-Rodríguez MP, Fornari DC, Zancheta C, Poveda Parra AR, et al. Genetic diversity of wild populations and broodstocks of curimba for restocking programmes in the Tietê, Grande, Pardo and Mogi-Guaçu rivers (Brazil). B Inst Pesca. 2015; 41(2): 287-304.). Microsatellites warrant a more specific analysis in population structures since they have high genetic mutation rates when compared to other DNA parts. They are actually the best for studies on mating and genic flow (Yue and Orban 2002Yue GH, Orban L. Microsatellites from genes show polymorphism in two related Oreochromis species. Mol Ecol Notes . 2002; 2(2): 99-100.).

Current assay determines the genetic variability of a wild population, broodstock and fingerlings of Brycon hilarii used in a repopulation program in the river Itiquira MT Brazil, by microsatellite markers.

MATERIALS AND METHODS

Samples were retrieved from the caudal fins of 30 Brycon hilarii, a broodstock used in repopulation reproductions, 96 fingerlings for repopulation and 30 specimens caught from the mid-river Itiquira MT Brazil, where repopulations programs were undertaken. The 30 broodstocks came from a fish-breeding stock in the municipality of Santo Antônio do Leverger MT Brazil (15° 51'S; 56º 04' W).

DNA extraction of samples from fragments of the caudal fin (0.5 cm2) followed protocol by Lopera-Barrero et al. (2008Lopera-Barrero NM, Povh JA, Ribeiro RP, Gomes PC, Jacometo CB, Lopes TS. Comparison of DNA extraction protocols of fish fin and larvae samples: modified salt (NaCl) extraction. Cien Inv Agr. 2008; 35(1): 77-86.). Samples were collected in 1.5 L microtube, to which were added 550 (L of a lysis buffer (50 mM Tris-HCl; 50 mM EDTA; 100 mM NaCl and 1% SDS) and 7 (L of proteinase K (200 (g/mL). Samples were kept in a warm bath overnight at 50ºC. DNA was then purified with 400 (L sodium chlorate (5 M) and centrifuged for 10 min at 14000 rpm; it was later precipitated with 700 (L iced absolute ethanol. Precipitate DNA was washed in ethanol 70%, re-suspended in TE (10 mM Tris and 1 mM EDTA), treated with 6 (L RNAse (30 (g/mL), and kept in a warm bath at 37ºC for 40 min.

DNA was counted in a Shimadzu spectrophotometer (Shimadzu Corporation, Kyoto, Japan), absorbance 260 nm, while samples were standardized for a concentration of 10 ng/µL. DNA quality was checked by agar gel electrophoresis gel 1%, in buffer TBE 1X (500 mM Tris-HC1, 60 mM boric acid and 83 mM EDTA) for 1 h at 70 volts. The gel was monitored under ultraviolet radiation after exposure to ethidium bromide (0.5 µg/ml) for one hour.

Seven microsatellite loci (Bh5, Bh6, Bh8, Bh13, Bh15, Bh16, Bh17), described by Sanches and Galetti Jr (2006Sanches A, Galetti Jr PM. Microsatellites loci isolated in the freshwater fish Brycon hilarii. Mol Ecol Notes. 2006; 6(4): 1045-1046. ), were amplified (Table 1). DNA was amplified in a 20 μL reaction volume with buffer 1X Tris-KCl, 2.0 mM MgCl2, 0.8 µM of each primer (forward and reverse), 0.2 mM of each dNTP, one unit of Platinum Taq DNA Polymerase and 20 ng DNA. DNA was first de-natured at 94ºC for four minutes and then 30 consecutive circles were performed, made up of 30 initial seconds at 94ºC, one minute annealing (Bh5: 52ºC; Bh6, Bh8, Bh13, Bh15 and Bh17: 56ºC; and Bh16: 58ºC) and one extension minute at 72ºC. There was a final extension at 72ºC for 10 minutes. The reactions were amplified in a Bio-Rad thermocycler (BIO-RAD, Hercules CA USA) and amplified samples underwent polyacrylamide gel electrophoresis 10% (acrylamide:bisacrylamide - 29:1) de-naturing (6 M urea) for 12 hours at 15 mA. Staining by silver nitrate visualized the alleles (Bassam et al. 1991Bassam BJ, Caetano-Anollés G, Gresshoff PM. Fast and sensitive silver staining of DNA in polyacrylamide gels. Anal Biochem. 1991; 196(1): 80-83. ). Gel underwent three types of solution: the first was constituted by a fixation solution (10% ethanol and 0.5% acetic acid) for 20 minutes; the second was an impregnation solution (6 mM silver nitrate) for 10 minutes; the third was a revelation solution (0.75 M NaOH and 0.22% formaldehyde 40%), photographed by Canon CoolPix 5200. Size of fragments was estimated by comparing with standard 10, 50 and 100 bp ladder (Invitrogen, USA).

Table 1
Characterization of microsatellite loci, sequence of loci, size and number of alleles (bp) and number of alleles per locus of wild population (WP), broodstock (BS) and fingerlings (FG) of Brycon hilarii.

Observed (Ho) and expected (He) heterozygosity, number of migrants (Nm), fixation index (FIS) and Hardy-Weinberg equilibrium (Wright 1978Wright S. Evolution and Genetics of Populations. Chicago: University of Chicago; 1978.) were calculated by GENEPOP 1.2 (Raymond and Rousset 1995Raymond M, Rousset F. Genepop (version 1.2): population genetics software for exact tests and ecumenicism. J Hered. 1995; 86(3): 248-249.), while PopGene 1.31 calculated allele frequency, distance and genetic identity and true number of alleles (Âe) (Yeh et al. 1999Yeh FC, Boyle TYZ, Xiyan JM. PopGene Version 131: Microsoft Window-based freeware for population genetic analysis. Alberta: University of Alberta and Center for International Forestry Research; 1999.). MEGA 5.2.2 (Tamura et al. 2011) prepared the dendrogram, while Weir and Cockerham´s method (1984Weir BS, Cockerham CC. Estimating F- statistics for the analysis of population structure. Evolution. 1984; 38(6): 1358-1370.) with FSTAT 2.9.3 (Goudet 2001Goudet J. FSTAT, a Program to Estimate and Test Gene Diversities and Fixation Indices Version 2.9.3. Lausanne: Lausanne University; 2001. ) estimated rates of genetic differentiation (FST). Arlequin 3.0 (Excoffier et al. 2005Excoffier L, Laval G, Schneider S. Arlequin Ver. 3.1: an integrated software package for population genetics data analysis. Evol Bioinform. 2005; 1: 47-50.) determined genetic differentiation by FST estimates (Weir and Cockerham 1984) and for Analysis of Molecular Variance (AMOVA) (Excoffier et al. 1992).

RESULTS AND DISCUSSION

The seven microsatellite loci provided 52 polymorphic alleles. Allele size ranged between 125 bp (Bh13 and Bh15) and 233 bp (Bh8). At the most, twelve alleles were observed for locus Bh8 and a minimum of three alleles for Bh15. There was a minimum of one allele (Bh15) and a maximum of seven alleles (Bh17 and Bh8) within each group of wild population and fingerlings. The former had the greatest number of alleles (4.3), followed by those from the broodstock (4.2) and fingerling stocks (4.1) (Table 1).

Allele size and number per locus in current assay were similar to size and number for B. hilarii reported by Sanches and Galetti Jr (2006Sanches A, Galetti Jr PM. Microsatellites loci isolated in the freshwater fish Brycon hilarii. Mol Ecol Notes. 2006; 6(4): 1045-1046. ). The number of alleles for the three genetic groups under analysis was higher than that registered by Lopera-Barrero et al. (2014Lopera-Barrero NM, Alvarez CAR, Rodriguez-Rodriguez MDP, Povh JA, Vargas L, Streit Júnior DP, et al. Genetic diversity and paternity of Brycon orbignyanus offspring obtained for different reproductive systems. Semina. 2014; 35(1): 541-554.) for broodstock and wild population of B. hilarii, by Lopera-Barrero et al. (2015) for broodstock and wild population of Prochilodus lineatus, and by Povh et al. (2011Povh JA, Ribeiro RP, Lopera-Barrero NM, Jacometo CB, Vargas L, Gomes PC, et al. Microsatellite analysis of pacu broodstocks used in the stocking program of Paranapanema river. Sci Agric. 2011; 68(3): 308-313. ) for broodstock and fingerling stocks of Piaractus mesopotamicus, respectively with 11, 44 and 31 alleles. Therefore, the number of alleles in current assay is adequate when compared to that in similar experiments.

The three exclusive alleles in locus Bh5 for fingerling stocks demonstrate that the group´s ancestry manifests genetic difference when contrasted to broodstock and wild population analyzed. Most probably the fingerling stock group had been formed by an ancestry that was not highly representative of the broodstocks and that adopted reproduction management should have benefitted the ancestry that failed to be represented in the broodstock sampling.

Low frequency alleles (< 0.1000) were reported in the three groups, with a higher percentage in the wild population (9 alleles) when compared to the stock of broodstocks (7 alleles) and fingerlings (6 alleles); the lowest allele frequency (0.0053) was registered in locus Bh8 (145 bp) and the highest (0.7384) in locus Bh16 (145 bp), in the fingerling stock. Twenty-one exclusive alleles (alleles of locus Bh5) were reported in the fingerling stock, five in the wild population and four in the broodstock (Table 2). Since no alleles were reported in loci Bh6 and Bh17, a lack of equilibrium was detected in the link between the alleles of the three groups.

Table 2
Characterization of allele frequency of wild population (WP), broodstock (BS) and fingerlings (FG) of Brycon hilarii.

Alleles´ frequency size between the broodstocks and the wild population remained stable. Although locus Bh6 has the most discrepant allele frequencies among broodstock and wild population, most alleles of the other loci had similar frequencies among these groups. Three out of the four alleles were similar in locus Bh16 for broodstock and wild population, corroborating the genetic similarity between the two groups. Locus Bh13 had a similar situation, or rather, all the alleles in the broodstocks and wild population were similar, with similarity in only one allele in fingerlings (150 bp - 0.3032). A greater number of exclusive alleles in fingerlings reveals genetic difference of the group when compared to broodstocks and wild population.

Data of mean observed heterozygosity (Ho) indicate a greater genetic variability in the wild population and broodstock (0.6290; 0.7204) when compared to the fingerling stock (0.5794). The low genetic variability of the wild population when compared to the broodstock may be due to the appearance of nil alleles in two loci (Bh6 and Bh17), revealing a lower occurrence of heterozygosity which, albeit with small intensity, may provide a distancing from the Hardy-Weinberg´s equilibrium percentage which is not expected in wild populations. Only Bh8 among the loci studies complied with the expected Hardy-Weinberg´s equilibrium in the three populations, forming a higher percentage of heterozygotes (Table 3).

Table 3
Observed heterozygosity (Ho), expected heterozygosity (He), fixation index (FIS), Hardy-Weinberg equilibrium test (HWE), number of alleles per locus (NA) and allele richness (AR ) of wild population (WP), broodstock (BS) and fingerlings (FG) of Brycon hilarii.

Sanches and Galetti Jr (2012Sanches A, Galetti Jr PM. Population genetic structure revealed by a school of the freshwater migratory fish, Brycon hilarii. Lat Am J Aquat Res. 2012; 40(2): 408-417.) analyzed populations of B. hilarii collected in several different places of the sub-basin of the river Miranda (river Paraguay basin) by seven microsatellite loci and reported two genetic populations. However, loci Bh6 and Bh13 failed to comply with the expected Hardy-Weinberg equilibrium. In fact, there was a deficit in heterozygosity, corroborating results in the wild populations reported in current analysis (Table 3). On the other hand, the inability of separating near-sized alleles, made difficult by stutter bands in the di-nucleotide microsatellite electrophorese, may have also decreased heterozygosity rates (Hassanien and Gilbey 2005Hassanien HA, Gilbey J. Genetic diversity and differentiation of Nile tilapia (Oreochromis niloticus) revealed by DNA microsatellites. Aquacult Res. 2005; 36(14): 1450-1457. ; Shyamala et al. 2014Shyamala GC, Marx KK, Jeyasekaran G. Genetic diversity in farmed Nile and red hybrid tilapia stocks in India using microsatellite genetic markers. J Aquacult Trop. 2014; 29(3-4): 131-143. ).

In the case of the fingerling group, mean rates for Ho reached 0.5794 and deviants in the Hardy-Weinberg equilibrium were reported in loci Bh5, Bh13, Bh15 and Bh16 with heterozygous deficits, corroborated by the mean rate of the fixation index (FIS= 0.1100). The above results revealed a close genetic factor among these specimens, perhaps due to reproduction management, already indicated by Lopera-Barrero et al. (2014Lopera-Barrero NM, Alvarez CAR, Rodriguez-Rodriguez MDP, Povh JA, Vargas L, Streit Júnior DP, et al. Genetic diversity and paternity of Brycon orbignyanus offspring obtained for different reproductive systems. Semina. 2014; 35(1): 541-554.), or to the control of cannibalism, as underscored by Borba et al. (2006Borba MR, Fracalossi DM, Pezzato LE. Dietary energy requeriment of piracanjuba fingerlings, Brycon orbignianus, and relative utilization of dietary carbohydrate and lipid. Aquacult nutr. 2006; 12: 183-191.). The two factors may have reduced the effective number of broodstocks and genetic variability.

The use of small numbers of broodstocks (with specimens in total spawning) and non-intentional selection (selection of broodstocks with certain specific characteristics) are usually the main factors that decrease genetic variability and increase endogamy in fingerlings. Further, in the case of inadequate management, possible cannibalism by post-larvae B. hilarii during the early phase (usually 36 - 96 hours old) may have decreased the effective number of broodstocks and, consequently, genetic variability.

A selection of beneficent characteristics for breeding, such as fish selection merely based on external characteristics (male: semen release after encephalic-caudal pressure; female: swelled belly and a reddened urogenital orifice), maturation stage of oocytes (migrated nucleus), regardless of parenthood, variability and genetic divergence, and the effective number of broodstocks (Povh et al. 2011Povh JA, Ribeiro RP, Lopera-Barrero NM, Jacometo CB, Vargas L, Gomes PC, et al. Microsatellite analysis of pacu broodstocks used in the stocking program of Paranapanema river. Sci Agric. 2011; 68(3): 308-313. ) may greatly reduce genetic variability within a single generation and decrease fingerlings´ viability within the natural environment (Christie et al. 2012Christie MR, Marine ML, French RA, Blouin MS. Genetic adaptation to captivity can occur in a single generation. Proc Natl Acad Sci. 2012; 109(1): 238-242. ). Povh et al. (2008) studied populations of pacu (P. mesopotamicus) for genetic monitoring and registered high rates of genetic variability in fingerlings when compared to broodstocks on the same site. This fact demonstrates that management in fish breeding maintained the ancestors´ genetic base. Since the above has not been observed in current assay, the fingerling sampling evaluated may reveal that repopulation may be including gene pools different from those from natural populations, or the absence of important genes for the feasibility of fish in the environment.

Fixation Index (FIS) provided negative rates (excess of heterozygotes) in six loci of broodstock population, averaging -0.0927, albeit with a non-significant Hardy-Weinberg equilibrium, which indicated absence of endogamy (Table 3). In the wild population, average FIS was positive (0.0110), with significant Hardy-Weinberg equilibrium, which indicated mild endogamy, perhaps related to the decrease in size of B. hilarii population. In fact, the capture of the species decreased in the last few years (Catella et al. 2014Catella AC, Albuquerque SP, Campos FLR, Santos DC. Control System the Fishing of Mato Grosso do Sul SCPESCA/MS 20-2013. Corumbá: Embrapa Pantanal; 2014.).

With regard to allele richness (AR) (Table 3), there was a slight variation in the number of alleles in all groups studied (wild population AR =4.33 - 4.36), (broodstocks AR = 4.17 - 4.26), (fingerlings AR = 4.14 - 4.11). Purcell et al. (2012Purcell KM, Ling N, Stockwell CA. Evaluation of the introduction history and genetic diversity of a serially introduced fish population in New Zealand. Biol Invasions. 2012; 14(10): 2057-2065. ) also reported higher allele richness in the wild population of Gambusia affinis (AR = 11.4-12.3) when compared to that of introduced populations (AR = 4.5-7.7). Decrease in allele richness in broodstocks may cause the animals to lose or limit their capacity to respond to changes in the natural environment (Christie et al. 2012Christie MR, Marine ML, French RA, Blouin MS. Genetic adaptation to captivity can occur in a single generation. Proc Natl Acad Sci. 2012; 109(1): 238-242. ).

AMOVA results show that most variability lies within each population (97.62; 73.77; 73.83), in the three groupings (wild population x broodstocks; wild population x fingerlings; broodstocks x fingerlings), respectively (Table 4). Rates are more representatives in the grouping wild population x broodstocks, and indicate that the two form a single genetically structured population. Comparison data between wild population and broodstocks with fingerlings reveal that fingerlings have a basic genetic structure that is different from natural populations and from broodstocks. There may have been a decrease in the true number of broodstocks (Ne) due to reproduction management or to cannibalism-control management, or even to the fact that the sample of the broodstocks was not representative.

Table 4
Analysis of molecular variance (AMOVA) of different groupings with wild population, broodstock and fingerlings of Brycon hilarii.

AMOVA data, confirmed by Wright´s genetic differentiation rates (1978Wright S. Evolution and Genetics of Populations. Chicago: University of Chicago; 1978.) and the coefficient of ancestrality (FST) (Table 5), revealed that fingerlings demonstrated high genetic differentiation from the other groups. They may be a single population unit, since the group had not been constituted with enough genetic variability. The genetic identity in the groupings wild population x fingerlings (0.2154) and broodstocks x fingerlings (0.2169) and their identities (1.535 and 1.5282 respectively) reinforce the slight genetic closeness of natural populations and broodstocks with the fingerlings (Table 5).

Table 5
Coefficient of ancestrality (F ST), Wright´s genetic differentiation (1978Wright S. Evolution and Genetics of Populations. Chicago: University of Chicago; 1978.) (Wright), genetic identity (GI), genetic distance (GD) and number of migrants (Nm) of different groupings of wild population, broodstock and fingerlings of Brycon hilarii.

Since lowest FST rate occurred between the wild population and the brookstocks (0.02377), only a small genetic differentiation was extant (Wright 1978Wright S. Evolution and Genetics of Populations. Chicago: University of Chicago; 1978.). The rate of genetic identity (0.8662) and genetic distance (0.1424) for the same group revealed genetic relationship. A higher rate for the number of migrants (6.1021) has been reported in the grouping (wild population x broodstocks), probably caused by the evidence of genic flux of these populations (Table 5). Dendrogram (Fig. 1) shows the genetic relationship between the three groups (wild population, broodstocks and fingerlings) and the shortest distance between the wild population and the broodstocks.

Figure 1
Dendrogram of groups wild population (WP), broodstock (BS) and fingerlings (FG) of Brycon hilarii, based on Nei´s genetic distance (Nei, 1972Nei M. Genetic distance between populations. Am Nat. 1972; 106: 283-292.).

Results show that the wild population of B. hilarii should be further analyzed, since a decrease in heterozygosity may occur even with the best variability levels, due to the introduction of animals with low genetic diversity coupled to reduction in population levels. Lower variability will produce not only several changes in allele frequencies, with a subsequent Hardy-Weinberg imbalance, but also disorders in the populations´ genic links.

Analyses of fish broodstocks revealed that the animals kept intact their genetic base. It is highly recommended that, due to the fingerlings´ genetic variability, further analyses should be performed with a larger sample of B. hilarii. Further, the species´s reproduction management should also be investigated by assessing the number of broodstocks, type of reproduction system (extrusion or semi-natural) since reproduction management and control of cannibalism may directly affect the offspring´s genetic variability.

Results in current study revealed the profile of fingerling stocks used in the repopulation of B. hilarii in the river Itiquira MT Brazil and recommended that new reproduction management and control of cannibalism should be taken for the preservation of the species, coupled to the maintenance of the genetic integrity of the population in its natural environment.

CONCLUSIONS

Genetic variability in the natural population and in broodstocks was high, albeit moderate in the fingerling stock. Genetic distancing was small between the wild population and the broodstocks, both of which had great genetic differentiation with the fingerling group.

ACKNOWLEDGMENTS

The authors would like to thank Group Bom Futuro and Nortox for their financial support.

REFERENCES

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  • Wright S. Evolution and Genetics of Populations. Chicago: University of Chicago; 1978.
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Publication Dates

  • Publication in this collection
    2016

History

  • Received
    07 May 2016
  • Accepted
    01 June 2016
Instituto de Tecnologia do Paraná - Tecpar Rua Prof. Algacyr Munhoz Mader, 3775 - CIC, 81350-010 Curitiba PR Brazil, Tel.: +55 41 3316-3052/3054, Fax: +55 41 3346-2872 - Curitiba - PR - Brazil
E-mail: babt@tecpar.br