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In vitro hemolytic activity of Bothrops lanceolatus (fer-de-lance) venom

Abstract

Bothrops lanceolatus venom contains a variety of enzymatic and biological activities. The present work investigated the hemolytic activity of this venom and its phospholipase A2 (PLA2). Bothrops lanceolatus venom (6.7 µg/mL) caused indirect hemolysis of cow, horse, rat and sheep erythrocytes, with horse erythrocytes being the most sensitive; no direct hemolysis was observed. Hemolysis in sheep erythrocytes was concentration-dependent (5-11.7 µg/mL) and markedly attenuated by heating the venom for 30 minutes at ≥ 40°C and by the PLA2 inhibitor p-bromophenacyl bromide. An acidic PLA2 (5 µg/mL) purified from B. lanceolatus venom also caused hemolysis. This PLA2 showed immunoprecipitin lines with antivenom against B. lanceolatus, which suggests that the enzymatic and hemolytic activities of this enzyme may be neutralized during antivenom therapy. These results indicate that B. lanceolatus venom and its PLA2 can cause hemolysis in vitro.

Bothrops lanceolatus; hemolytic activity; phospholipase A2; snake venom


ORIGINAL PAPER

In vitro hemolytic activity of Bothrops lanceolatus (fer-de-lance) venom

Martins LJI; de Araújo PMFII; Bon CIII,†; Hyslop SI; de Araújo ALI

IDepartment of Pharmacology, School of Medical Sciences, State University of Campinas, Unicamp, Campinas, São Paulo State, Brazil

IIDepartment of Microbiology and Immunobiology, Institute of Biology, State University of Campinas, Unicamp, Campinas, São Paulo State, Brazil

IIINational Museum of Natural History, Paris, France

Correspondence to Correspondence to: Albetiza Lôbo de Araújo Departamento de Farmacologia Faculdade de Ciências Médicas Universidade Estadual de Campinas, UNICAMP, Caixa Postal 6111, Campinas, SP, 13.083-970, Brasil Phone: +55 19 3521 9529 Fax: +55 19 3289 2968 Email: albetiza@fcm.unicamp.br

ABSTRACT

Bothrops lanceolatus venom contains a variety of enzymatic and biological activities. The present work investigated the hemolytic activity of this venom and its phospholipase A2 (PLA2). Bothrops lanceolatus venom (6.7 µg/mL) caused indirect hemolysis of cow, horse, rat and sheep erythrocytes, with horse erythrocytes being the most sensitive; no direct hemolysis was observed. Hemolysis in sheep erythrocytes was concentration-dependent (5-11.7 µg/mL) and markedly attenuated by heating the venom for 30 minutes at ≥ 40°C and by the PLA2 inhibitor p-bromophenacyl bromide. An acidic PLA2 (5 µg/mL) purified from B. lanceolatus venom also caused hemolysis. This PLA2 showed immunoprecipitin lines with antivenom against B. lanceolatus, which suggests that the enzymatic and hemolytic activities of this enzyme may be neutralized during antivenom therapy. These results indicate that B. lanceolatus venom and its PLA2 can cause hemolysis in vitro.

Key words:Bothrops lanceolatus, hemolytic activity, phospholipase A2, snake venom.

INTRODUCTION

Bothrops lanceolatus is endemic to the Caribbean island of Martinique (1). Envenomation by this species produces local (edema, pain, hemorrhage, necrosis) and systemic (coagulopathy) effects, with coagulation disturbances (thrombosis) being the most important cause of clinical complications and mortality (2-4). Enzymes that may contribute to these effects include an esterase (5), a caseinolytic protease (6), a hemorrhagic metalloproteinase (7) and an acidic phospholipase (8). The hemolytic activity of B. lanceolatus venom and involvement of PLA2 in this phenomenon have not been extensively studied, although Bogarín et al. (9) reported that the hemolytic activity of B. lanceolatus venom was neutralized by homologous antivenom. In this report, we describe some characteristics of the hemolysis caused by B. lanceolatus venom in vitro.

MATERIALS AND METHODS

Venom, PLA2 and Antivenom

Bothrops lanceolatus venom was supplied by the Unité des Venins, Institut Pasteur (Paris, France) and was stored at -20°C until use. Acidic PLA2 (fraction F32) was purified from B. lanceolatus venom by a combination of gel filtration and ion-exchange chromatography, as previously described (8). Antivenom (batch BO 278, Pasteur Institute, Paris) produced in horses immunized with B. lanceolatus venom was stored in lyophilized form.

Assay for Hemolytic Activity

Sheep blood was obtained from a commercial sheep breeder (Biotério Boa Vista, Fazenda São Sebastião, Patrocínio Paulista, SP, Brazil), cow and horse blood were obtained from a commercial slaughterhouse, and blood from Wistar rats was collected from animals provided by the university's Multidisciplinary Center for Biological Investigation (CEMIB/UNICAMP). Suspensions of washed erythrocytes were prepared in phosphate-buffered saline (PBS) using standard procedures whereas the indirect hemolytic activity was assayed in a mixture containing venom or PLA2, hen egg-yolk lecithin and erythrocytes, essentially as described by Gutiérrez et al. (10). The relationship between venom concentration and hemolysis was investigated in sheep erythrocytes. Direct hemolytic activity was assessed in incubations without egg-yolk lecithin. Hemolytic activity was expressed as a percentage of the total hemolysis (100%) obtained by lysing erythrocytes in distilled water.

Heat Stability of the Hemolytic Activity

The heat stability of the hemolytic activity was determined by incubating venom at 25, 40, 50, 70 and 90°C for 30 minutes followed by cooling and then assaying the residual hemolytic activity in sheep erythrocytes.

Role of PLA2 in the Hemolytic Activity

The role of PLA2 in the hemolytic activity of the venom was assessed by incubating venom with 2.88 mM p-bromophenacyl bromide (pBPB) (Sigma Chemical Co., USA) for 30 minutes at 37°C, after which the residual PLA2 and hemolytic activities were assayed in 96-well plates, as described by Nishida et al. (11). Each well contained 200 µL of hen egg-yolk emulsion as substrate in PBS containing 2 mM CaCl2 and 40 µL of venom. The increase in absorbance at 750 nm was recorded for up to 40 minutes in a SpectraMax 340® multiwell plate reader (Molecular Devices, USA) and the activity was expressed as the increase in absorbance at 750 nm/minute. Hemolytic activity was assayed as described above, using sheep erythrocytes. All assays were run in duplicate and corrected for appropriate blanks.

Immunological Analysis

Immunodiffusion of the venom and purified PLA2 was done in PBS in 1% agar gels, as described by Ouchterlony (12), using a 10% (w/v) solution of B. lanceolatus antivenom. After incubation in a humidified chamber for 48 hours at room temperature, the slides were washed extensively in 0.9% (w/v) NaCl and the immunoprecipitin bands were detected by Coomassie blue staining.

Immunoelectrophoresis was done in 1% agar gels poured on glass slides. Samples of venom and purified PLA2 were applied to the gels and run for one hour at 6 V/cm in 50 mM veronal buffer, pH 8.4 (13). Following electrophoresis, a 10% (w/v) solution of B. lanceolatus antivenom was placed in the central trough and the slides were incubated for 48 hours at room temperature in a humidified chamber. After extensive washing in 0.9% (w/v) NaCl, the gels were dried and stained with Coomassie blue.

Statistical Analysis

The results were expressed as the mean ± S.E.M., and statistical comparisons (p < 0.05) were done using Student's t-test or analysis of variance (ANOVA) followed by the Tukey test.

RESULTS

Hemolytic Activity of B. lanceolatus Venom and Purified PLA2

Figure 1A shows that B. lanceolatus venom caused indirect hemolysis of erythrocytes in all of the species examined, with horse erythrocytes being the most susceptible and sheep erythrocytes the least susceptible (p < 0.05); there was no significant difference between the degree of hemolysis of rat and cow erythrocytes (p > 0.05). No direct hemolysis was observed with any of these species (data not shown; n = 4). In subsequent experiments, sheep erythrocytes were used because these were readily obtained from an established laboratory.


   





Bothrops lanceolatus venom caused concentration-dependent hemolysis of sheep erythrocytes that was maximal at > 10 µg/mL (Figure 1B). This hemolytic activity was markedly attenuated by heating the venom for 30 minutes at ≥ 40°C, with complete inhibition of hemolytic activity occurring at ≥ 50°C (Figure 1C). Incubation with pBPB significantly (p < 0.05) inhibited the PLA2 activity of the venom (from 74.0 A750nm/minute to 3.7 A750nm/minute) and completely abolished the hemolytic activity (n = 4). Purified PLA2 (5 µg/mL) caused total hemolysis of sheep erythrocytes (a complete concentration-response curve of this hemolytic activity was not obtained because of the limited amount of pure PLA2 available) (Figure 1D).

Immunological Studies

Figure 2 shows the immunoprecipitin lines obtained with B. lanceolatus venom and purified PLA2 after incubation with antivenom. Multiple lines were obtained with the venom but only one major line was seen with PLA2 in immunodiffusion and immunoelectrophoresis.


DISCUSSION

The results of this study indicate that B. lanceolatus venom can cause indirect hemolysis of erythrocytes from a variety of mammalian species. This action on erythrocytes was indirect since there was no hemolysis in the absence of egg-yolk lecithin. The hemolytic activity was concentration-dependent and thermolabile since heating the venom at ≥ 40°C resulted in little or no hemolysis. These findings generally agree with reports on the hemolytic activity of other Bothrops venoms (14-16). Variation in species sensitivity to hemolysis as seen herein (sheep < cow/rat < horse) has also been observed with other Bothrops venoms, e.g., B. asper venom causes direct hemolysis of mouse erythrocytes but has no effect on goat, horse, rabbit, sheep and toad erythrocytes; in contrast, lysis of human erythrocytes requires bovine serum albumin and Ca2+ (17). These variations may reflect differences in the phospholipid composition of the erythrocyte plasma membrane of these species (18-20), as well as the accessibility of the cellular membrane targets such as negative phospholipids to PLA2 action (17, 18). Incubation of the venom at different temperatures indicated that the venom component responsible for hemolysis is thermolabile. Other biological activities of B. lanceolatus, such as rat paw edema, leukocyte migration and hemorrhagic activity, are also thermolabile (7, 21, 22).

A role for venom PLA2 in the hemolytic activity was suggested by the finding that the loss of hemolysis paralleled the inhibition of PLA2 activity by pBPB. In addition, purified PLA2 also caused hemolysis. In agreement with this, various studies have shown that PLA2s are the principal component of Bothrops venoms responsible for hemolysis (23-26). In addition to the hemolytic activity described herein, the PLA2 of B. lanceolatus venom also contributes to neutrophil migration during inflammation caused by this venom (21) and may be involved in the anticoagulant action of the venom (27).

The immunoprecipitin lines observed with purified PLA2 and B. lanceolatus antivenom in immunodiffusion and immunoelectrophoresis indicated that this protein was antigenic and was recognized by the antivenom. This finding supports the results of Bogarín et al. (9), who showed that this antivenom neutralized the indirect hemolytic activity of B. lanceolatus venom. Other studies have also shown that bothropic antivenoms can neutralize the PLA2 and hemolytic activities of homologous and heterologous Bothrops venoms (16, 28-32).

Although intravascular hemolysis has been observed following envenomation by Bothrops species (33), this phenomenon has not been documented after bites by B. lanceolatus, the main effects of which are edema, pain and coagulation disturbances (2-4). Hence, the clinical relevance of the findings described herein remains to be determined.

In conclusion, B. lanceolatus venom causes concentration-dependent hemolysis in vitro, with the order of susceptibility among erythrocytes from different species being sheep < cow/rat < horse. This activity is thermolabile and is apparently mediated by the PLA2 of the venom. The cross-reactivity of the venom and PLA2 with antivenom suggests that the hemolytic activity may be neutralized by antivenom.

ACKNOWLEDGMENTS

The authors thank José Ilton dos Santos, Alessandra Priscila Ponciano, Célia A. A. C. Garcia and José Raimundo R. dos Reis for technical assistance, Marcelo Carvalho, Paulo A. F. Nunes and Paula L. Dotto for help with some of the experiments, and Silvia P. Irazusta for helpful comments on the manuscript. S.H. is supported by a research fellowship from CNPq.

Received: October 14, 2008

Accepted: July 8, 2009

Abstract published online: July 17, 2009

Full paper published online: August 31, 2009

CONFLICTS OF INTEREST: There is no conflict.

FINANCIAL SOURCE: CNPq.

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  • Correspondence to:
    Albetiza Lôbo de Araújo
    Departamento de Farmacologia
    Faculdade de Ciências Médicas
    Universidade Estadual de Campinas, UNICAMP, Caixa Postal 6111, Campinas, SP, 13.083-970, Brasil
    Phone: +55 19 3521 9529
    Fax: +55 19 3289 2968
    Email:
  • Publication Dates

    • Publication in this collection
      14 Sept 2009
    • Date of issue
      2009

    History

    • Accepted
      08 July 2009
    • Received
      14 Oct 2008
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