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Evaluation of rat plasma proteins after bothropic venom inoculation and treatment with Mesenquimal stem cells

Abstract

The aim of this work was to evaluate the mesenchymal stem cells treatment of rats with myonecrosis caused by Rhinocerophis alternatus venom through acute phase proteins (APP) profile. The animals were distributed into three experimental groups (G1, G2 and G3). G1 and G2 were inoculated with 120 μg of R. alternatus venom diluted in 200 µL of ultra-pure water in gastrocnemic muscle, while G3 received 200 µL of ultra-pure water. Three days after, G1 was treated with 5 X 10(6) MSC diluted in PBS and G2 and G3 only with PBS. Each three days after the treatments (3rd, 6th, 9th, 12th 15th days), blood of five animals in each group was collected in order to evaluate the APP. A decrease (P<0.05) in α2-globulin fraction was observed in G1 on the 6th day. In G1 and G2, a raise (P<0.05) was observed in β globulin, a common occurrence in the late phases of inflammatory process, although no significant difference was observed between them. Concerning gamma globulins levels, on the 6th day after the treatments, in G1 and G2 groups, increase in the levels was observed. These data showed that the MSC treatment after bothropic envenomation in the rats caused alteration in APP.

Rhinocerophis alternatus venom; Rats; Mesenquimal stem cell; Inflammatory proteins


HUMAN AND ANIMAL HEALTH

Evaluation of rat plasma proteins after bothropic venom inoculation and treatment with Mesenquimal stem cells

Thalita Costa TellesI; Ana Flávia Ribeiro Machado MichelI; Maria LúciaII; Bruno Martins MeloIII; Adriane Costa-Val Pimenta BicalhoI; Natália Melo OcarinoI; Marilia Martins Melo I * * Author for correspondence: mariliamm@ufmg.br

IDepartamento de Clínica e Cirurgia Veterinárias; Escola de Veterinária; Universidade Federal de Minas Gerais; Belo Horizonte - MG - Brasil

IIDepartamento de Biologia; Universidade José do Rosário Vellano; Alfenas - MG - Brasil

IIIDepartamento de Pediatria; Faculdade de Medicina; Universidade Federal de Minas Gerais; Belo Horizonte - MG - Brasil

ABSTRACT

The aim of this work was to evaluate the mesenchymal stem cells treatment of rats with myonecrosis caused by Rhinocerophis alternatus venom through acute phase proteins (APP) profile. The animals were distributed into three experimental groups (G1, G2 and G3). G1 and G2 were inoculated with 120 μg of R. alternatus venom diluted in 200 µL of ultra-pure water in gastrocnemic muscle, while G3 received 200 µL of ultra-pure water. Three days after, G1 was treated with 5 X 106 MSC diluted in PBS and G2 and G3 only with PBS. Each three days after the treatments (3rd, 6th, 9th, 12th 15th days), blood of five animals in each group was collected in order to evaluate the APP. A decrease (P<0.05) in α2-globulin fraction was observed in G1 on the 6th day. In G1 and G2, a raise (P<0.05) was observed in β globulin, a common occurrence in the late phases of inflammatory process, although no significant difference was observed between them. Concerning gamma globulins levels, on the 6th day after the treatments, in G1 and G2 groups, increase in the levels was observed. These data showed that the MSC treatment after bothropic envenomation in the rats caused alteration in APP.

Key words:Rhinocerophis alternatus venom, Rats, Mesenquimal stem cell, Inflammatory proteins

INTRODUCTION

The majority of snake bite accidents in South America are inflicted by the species belonging to Bothrops genus (Bochner and Struchiner 2003). The bothropic venom induces a qualitatively similar pathophysiological picture, characterized by immediate and prominent local tissue damage (edema, hemorrhage and mionecrosis), vascular alterations (hemorrhage and hypovolemic shock) and coagulation disorders (defibrination) (Chiacchio et al. 2011).

If specific antivenom (antibothropic) administration is initiated rapidly after envenomation, neutralization of systemic effects is usually successfully achieved, but neutralization of the local tissue damage is a more difficult task. This therapy has low and limited effectiveness against the local myonecrosis and cytotoxicity (Gutiérrez and Ownby 2003; Quesada et al. 2006; Silva et al. 2007). In a number of snake bite cases, lack of neutralization of local effects results in permanent sequelae, with tissue loss (Battellino et al. 2003).

Due to the relevance of local effects in envenomation induced by the snakes of the genus Bothrops, several studies have been made on its different perspectives (Dourado et al. 2008). The use of phytotherapy against the snake venom has long been recognized, even in modern times but only for the last 20 years, it gained closer scientific attention (Mors et al. 2000). However, the isolation of plant compounds is difficult and expensive and often only a little amount can be isolated.

The mesenchymal stem cell (MS) therapy has been a promise for the repair of acute and chronic cutaneous wounds. MSC has the unusual capacity for self-renewal and differentiation, which has a high therapeutic value in reprogramming growth of tissues to repair injuries and treat diseases (Alonso and Fuchs 2003).

Another important property of MSC is to generate the cell types of tissues completely different from its origin, a phenomenon called plasticity (Gomillion and Burg 2006; Fuchs 2008). Recent studies have shown that MSC from the bone marrow can differentiate into various cells such as ectodermal, mesodermal and endodermal when transplanted into the body, repairing surgically induced wounds and burn injuries (Liu et al. 2008). Thus, through what is known by the regenerative medicine and cell therapy, it can be inferred that MSC can be used to repair the damaged tissue or wounds, which has minimized the complications caused by skin graft rejection of patients suffering from extensive burns or skin lesions (Metcalfe and Ferguson 2007; Liu et al. 2008).

The use of the MSC as treatment for the injuries caused by snake venom has not been reported in the literature. Considering the severity of local lesions observed in bothropic envenomation and the difficulty to reverse these manifestations, the search for novel toxin inhibitors represents a potential promise for improving the treatment of this serious aspect of this envenomation. In the present work, the ability of MSC to antagonize the myonecrosis in rats after venom injection was studied, evaluating some of the early inflammatory changes, such as acute phase proteins (APP).

MATERIAL AND METHODS

Cell Harvesting and Culture

To obtain bone marrow samples, three female rats (30 days old) were sacrificed with an overdose of anesthesia (pentobarbital sodium, 30 mg/kg). The femurs and tibias were removed from the attached muscle and connective tissue under aseptic conditions, and the epiphyses were removed (Ocarino et al. 2010). The bone marrow was flushed with Dulbecco's modified Eagle's medium (DMEM; Gibco, Grand Island, N.Y., USA), and the released cells were suspended in DMEM, supplemented with 10% fetal bovine serum (Gibco) and antibiotics (60 µg/L gentamicin, 25 µg/L amphotericin B, 100 U/mL penicillin and 100 µg/mL streptomycin; Merck, Germany) and collected in a 75-cm two-culture flask containing 10 mL of culture medium. The cells were grown at 37°C/5% CO2 for three days. The non-adherent cell population was removed and the adherent layer was washed once with fresh medium. The culture medium was changed two times in a week during the culturing.

FACS Analysis

Cells at the fourth passage were harvested with trypsin/EDTA, centrifuged at 1,400 rpm for 10 min and re-suspended at 1 X 106 cells/well in phosphate-buffered saline (PBS). The cell aliquots were incubated with individual primary or control antibodies for 30 min at 4°C and were washed in PBS and incubated with fluorophore-conjugated secondary antibody for at 4°C for 30 min. The samples were analyzed using a FACScan cytometer (Becton Dickinson) and data were analyzed using the Cellquest software (Becton Dickinson). The following primary antibodies were used: anti-CD45, anti-CD90, anti-CD73 and anti-CD54 (BD Biosciences, San Jose, Calif., USA).

Cells viability for blue trypan assay

Immediately before the injection, the cells viability was analyzed. For trypan blue exclusion assay, the cells were exposed to trypan blue for 10 min. The number of viable cells (by dye exclusion) was counted under the light microscope using a Neubauer camera and expressed as a percentage of total cells.

Venom

The venom pool from the adult Rhinocerophis alternatus (Bothrops alternatus) snakes was dried in a vacuum desiccator at room temperature immediately after milking and then stored at -20°C until the moment of utilization.

Animals Assays

Seventy-five male Wistar rats with mean weight of 120 g were kept in cages (40 x 45 x 45 cm) and were maintained under the controlled light cycle (12/12 h) and temperature (22 ± 2°C) with free access to food and water for all the experiments. The study animals were distributed into three equal groups of 25 animals each, G1, G2 and G3. Rats of G1 and G2 received 120 µg of R. alternatus venom diluted in 200 µL of ultra pure water, while G3 received only 200 µL of ultra pure water. Such doses were previously determined in a pilot experiment. In all the cases, administration occurred via intra muscular injection into right gastrocnemius muscle using a hypodermic syringe.

After three days (72 h), G1 was treated with one injection of 5 X 106 MSC diluted in 200 µL of PBS and G2 (positive control) and G3 were treated with 200 µL of PBS (negative control). The time of treatment (72 h after venom inoculation) was chosen due the kinetics of R. alternatus (B. alternatus) described by Mello et al. (2010).

Every three days after the treatments, blood was collected by cardiac puncture of five animals of each group on 3rd (TI), 6th (TII), 9th (TIII), 12th (TIV) and 15th (TV) day to perform the protein profile. All the animals were anesthetized by means of intramuscular injection in the contralateral limb of a mixture containing 10 mg/kg of xylazine hydrochloride and 75 mg/kg of ketamine (Sigma Chemical Co. - USA).

Blood samples were stored in the flasks without anticoagulant. The total protein concentration was calculated by refratometer (Ningbo Utech International CO LTD) and the fractioned proteins (albumin, alfa, beta and gamma globulins) were evaluated by eletrophoresis in agarose gel (CELMGEL) (30 min) in TRIS buffer. The gels were stained for 5 minutes in 200 mL of Amido black and destained in acid acetic solution (7%) until de gel background was completely clear. The concentration of protein fractions was determined by the use of computer-assisted software CELM SE- 250.

Statistics

The experiment followed a random design. Data were subjected to Lillifors, Kolmogorov-Smirnov and Shapiro-Wilk normality tests. The analysis of variance (ANOVA) was applied to variables that were normally distributed, the mean values of which were compared using the SNK test. Statistical analyses were carried out with the aid of SAS (Cary, NC, USA).

RESULTS AND DISCUSSION

The phenotypic characterization of the bone marrow MSC indicated that there was no CD45 expression in 96.94% of the cells. There was, however, expression of CD73, CD54 (intercellular adhesion molecule-1; ICAM-1) and CD90 in 93.99, 95.1 and 86.77.0% of the cells, respectively.

Even under the anesthesia, after venom injection, pain was observed manifestating in all the G1 and G2 animals. There was muscle fasciculation in the right hind limb, which stayed flexed for about 20 h. Same demonstration was also observed by Dourado et al. (2008) in mice inoculated with B. neuwiedi venom for 12 h. In the present study, the peak of hyperalgesia was observed after one hour after venom inoculation and clinical signs of pain gradually decreased and disappeared completely after 24 h. The pharmacological basis of hyperalgesia and allodynia induced by the bothropic venom has been investigated and the involvement of various mediators, such as bradykinin and leucotrienes has shown a multifactorial mechanism in the onset of pain (Chacur et al. 2001). This effect can be potentialized by increased local pressure caused by edema. The envenomed animals (G1 and G2) showed moderate local edema, with no extension to the rest of the limb. In the cases of bothropic envenomation, local edema is commonly found and may worsen the hypovolemia condition. Bothropic envenomation causes rapid development of edema and inflammation at the bite site. The edema induced by these venoms is associated with the action of various substances such as hemorragins (that act directly on the endothelium of capillaries and small veins, increasing the permeability), cytotoxins (induce the release of histamine, PLA2, and arachidonic acid, which releases membrane phospholipids, leading to the synthesis of prostaglandins that, in turn, increases the capillary permeability), proteases (that break kininogen, releasing kinins and leading to the production of nitric oxide and prostaglandins), vasoactive peptides (inhibit the action of the angiotensin converting enzyme and boost the action of bradykinin); and components of the complement cascade (Gutiérrez et al. 2009). The injection of ultra pure water (control group) did not modify the pain threshold of the animals.

No macroscopic signs of hemorrhage, dermonecrosis and blistering were observed in all the animals, but envenomed animals stayed apathetic, hypoxemic and hypodipsic for about 24 h, returning to normal activities after this period.

As shown in Figure 1, there were differences in serum total protein values between G1 (7.64+0.80 mg/dL) and G3 (6.56+0.26 mg/dL) in TI (3rd day), probably due to an increase in α1-globulin fraction in G1, as shown in Figure 3. On the12th day (TIV), the G1 presented a significant reduction in total protein, when compared to others studied times (TI, TII, TIII and TV). A significant decrease in albumin values, as shown in Figure 2, could be responsible for this phenomenon.




There was no difference in the albumin levels between the groups during all the times, except 12th day (TIV), when a decrease was observed (P<0.05) in G1. Albumin is a negative acute phase protein and its concentration gradually falls during the infectious and inflammatory diseases. The secretion of albumin is stimulated by a decrease in osmotic pressure but can also be affected by the pathophysiological changes such as during infectious or inflammatory disease when the secretion is reduced. This is caused by the proinflammatory cytokines such as interleukin (IL)-1, IL-6, and tumor necrosis factor- α (TNF). These cytokines are simultaneously responsible for the increased synthesis and secretion of the APP.

The results of α1-globulin showed statistical difference between groups only on 12th day (Fig. 3), when there was an increase (P<0.05) of α1-globulin in the G2 (venom + PBS).

On 3rd day (TI), the α2-globulin showed a statistically increase in the groups that received venom (G1 and G2) when compared to the control group (G3) (Fig 4). These values tended to decline over the time, and especially in G1 after 6 days (in TIII), there was a significant decrease in the α2-globulin fraction. The α2-globulin is considerate APP. Inside α2-globulin, there are two proteins, alfa-2-macroglobulin, and the haptoglobin, which is a moderate APP and responds to inflammatory and infectious disease.


Evidently on 12th day, the G2, group that received venom and was treated with PBS (placebo) showed an increase in α1 and α2 globulins. On the 3rd, 6th and 12th days, the same group, G2, also showed an increase in beta globulins.

In the animals that received bothropic venom (G1 and G2), the β-globulin was elevated until 12th day (Fig. 5) when compared to the control (G3). These data agreed with those in literature describing an increase of the β-globulin in a latter phase of inflammatory process. The beta-globulins are β -lipoprotein and complement C3, which are located in the β1 region, and transferrin and IgM which are located in the β2 region. Transferrin and complement C3 participate in many immunological and inflammatory reactions. The activation of complement C3 has been described after snake venom envenomation. But it must be stressed that in the group that received the venom and was treated with MSC (G1), there was a significant decrease of beta globulins when compared with the group that received venom and was treated with placebo (G2).


In order to understand this kind of envenomation and improve its therapeutic strategy, besides clinical and epidemiological studies, it is necessary to understand the role of inflammatory mediators such as nitric oxide (NO), cytokines and the complement system (Petricevich et al. 2000). Nitric oxide also participates in the pathogenesis of snake envenomations by two different mechanisms: it may lead to tissue damage due to its ability to generate peroxynitrite and hydroxyl radicals after interaction with superoxide ions, and, it may provoke hypotension by its vasodilator action (Radi et al. 1991; Hoog et al. 1992). The precise function of NO in snake envenomations has yet to be investigated, but it is probably important in the systemic effects caused by snake envenomations. The mechanism by which snake venoms induce the production of cytokines and NO is unknown (Petricevich et al. 2000). It has been observed that the animals experimentally injected with Bothrops venoms showed leukocyte accumulation, which was dependent on eicosanoid release and chemotactic factors derived from the serum (Farsky et al. 1997). However, the latter effect is probably due to the complement activation (Dias-da-Silva et al. 1995.

According to Gutiérrez et al. (2009), local tissue damage is induced by Bothrops venom, neutrophils, cytokines, but nitric oxide does not contribute to a significant extent in the pathogenesis of myonecrosis in animal models. The scenario that emerges from these observations is one in which the local pathology is mostly caused by the direct action of venom PLA2s and metaloproteinases in the tissue. The prominent inflammatory reaction that ensues is likely to participate in the processes of tissue repair and regeneration. Therefore, the manipulation of the local inflammatory response has to be analyzed in the light of this hypothesis in order to promote its favorable aspects that contribute to tissue regeneration.

The last fraction normally viewed in electrophoresis is immunoglobulin (IgA and IgG), therefore, express mainly the IgG immunogama-globulin, with a correlation with concentrations of immunochemistry. Thus, the statistical increase of γ-globulin in G1 and G2 compared to G3 (Fig. 6) was due to increase of IgG, a common occurrence in bothropic envenomation.


Due to the increase of the globulins in the groups that received venom, a less significant albumin / globulin relationship was observed. However, this result was not observed on 9th day (TIII), when the groups were statistically equal and differentiated on 12th and 15th day (Fig. 7).


This is first report on the activity of mesenchymal stem cells in the inflammation response caused by R. alternatus venom in vivo.

CONCLUSION

These results showed that the MSC treatment after bothropic envenomation in the rats caused a decrease in α2-globulin and beta globulin fractions.

ACKNOWLEDGEMENTS

The authors acknowledge Prof. Dr. Angela Maria Quintão Lana for statistical advice and Prof. Dr. Rogéria Serakides for cells donation.

Received: October 30, 2012;

Accepted: November 04, 2013.

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  • Publication Dates

    • Publication in this collection
      24 Feb 2014
    • Date of issue
      Feb 2014

    History

    • Accepted
      04 Nov 2013
    • Received
      30 Oct 2012
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