Abstract
Snake venom (sv) C-type lectins encompass a group of hemorrhagic toxins, which are able to interfere with hemostasis. They share significant similarity in their primary structures with C-type lectins of other animals, and also present a conserved carbohydrate recognition domain (CRD). A very well studied sv C-type lectin is the heterodimeric toxin, convulxin (CVX), from the venoms of South American rattlesnakes, Crotalus durissus terrificus and C. d. cascavella. It consists of two subunits, alfa (CVXalpha , 13.9 kDa) and beta (CVXbeta , 12.6 kDa), joined by inter and intra-chain disulfide bounds, and is arranged in a tetrameric alpha4beta4 conformation. Convulxin is able to activate platelet and induce their aggregation by acting via p62/GPVI collagen receptor. Several cDNA precursors, homolog of CVX subunits, were cloned by PCR homology screening. As determined by computational analysis, one of them, named crotacetin beta subunit, was predicted as a polypeptide with a tridimensional conformation very similar to other subunits of convulxin-like snake toxins. Crotacetin was purified from C. durissus venoms by gel permeation and reverse phase high performance liquid chromatography. The heterodimeric crotacetin is expressed in the venoms of several C. durissus subspecies, but it is prevalent in the venom of C. durissus cascavella. As inferred from homology modeling, crotacetin induces platelet aggregation but noticeably exhibits antimicrobial activity against Gram-positive and Gram-negative bacteria.
Crotalus durisssus venom; snake venom C-type lectin; homology modeling; platelet aggregation; antimicrobial activity
ORIGINAL PAPER
Crotacetin, a novel snake venom C-type lectin, is homolog of convulxin
Rádis-Baptista G.I; Moreno F. B. M. B.I; Nogueira L. L.I; Martins A. M. C.II; Toyama D. O.III; Toyama M. H.IV; Azevedo Jr W. F.V; Cavada B. S.I; Yamane T.VI
IDepartment of Biochemistry and Molecular Biology, Federal University of Ceará (UFC), Ceará, Brazil
IIDepartment of Clinical and Toxicological Analyses, Federal University of Ceará (UFC), Ceará, Brazil
IIIDepartment of Biochemistry, State University of Campinas (UNICAMP), São Paulo, Brazil
IVDepartment of Chemistry, São Paulo State University (UNESP), São Paulo, Brazil
VDepartment of Physics, Institute of Biosciences, Humanities and Exact Sciences, São Paulo State University (UNESP), São Paulo, Brazil
VIMolecular Biology Center, Institute of Nuclear Energy and Research (IPEN), São Paulo, Brazil.
CorrespondenceCorrespondence toGandhi Rádis-Baptista Departamento de Bioquímica e Biologia Molecular, Universidade Federal do Ceará Campus do Picí, P.O. Box: 6020 60451-970, Fortaleza, Ceará, Brazil Phone: +55 85 4008 9817. Fax: +55 85 4008 9789 Email: radisbra@ufc.br
ABSTRACT
Snake venom (sv) C-type lectins encompass a group of hemorrhagic toxins, which are able to interfere with hemostasis. They share significant similarity in their primary structures with C-type lectins of other animals, and also present a conserved carbohydrate recognition domain (CRD). A very well studied sv C-type lectin is the heterodimeric toxin, convulxin (CVX), from the venoms of South American rattlesnakes, Crotalus durissus terrificus and C. d. cascavella. It consists of two subunits, alfa (CVXa , 13.9 kDa) and beta (CVXb , 12.6 kDa), joined by inter and intra-chain disulfide bounds, and is arranged in a tetrameric a4b4 conformation. Convulxin is able to activate platelet and induce their aggregation by acting via p62/GPVI collagen receptor. Several cDNA precursors, homolog of CVX subunits, were cloned by PCR homology screening. As determined by computational analysis, one of them, named crotacetin b subunit, was predicted as a polypeptide with a tridimensional conformation very similar to other subunits of convulxin-like snake toxins. Crotacetin was purified from C. durissus venoms by gel permeation and reverse phase high performance liquid chromatography. The heterodimeric crotacetin is expressed in the venoms of several C. durissus subspecies, but it is prevalent in the venom of C. durissus cascavella. As inferred from homology modeling, crotacetin induces platelet aggregation but noticeably exhibits antimicrobial activity against Gram-positive and Gram-negative bacteria.
Key words: Crotalus durisssus venom, snake venom C-type lectin, homology modeling, platelet aggregation, antimicrobial activity.
INTRODUCTION
Snake venoms are complex mixtures of polypeptides and organics with the ability to paralyze, kill and digest any prey organism. The venom composition is diverse, differing between species (inter-specific venom variations) and individuals (intra-specific venom variations) (28). Hereditary and epigenetic factors (e.g., geographical distribution, diet, snake maturity) contribute to the venom variability (8, 25, 43, 44, 47). Based on the victim's symptoms of snakebite, snake venom can basically be classified as neurotoxic or hemorrhagic. Neurotoxins act on ion channels and neural receptors (17). Hemorrhagic toxins interfere with blood stasis and their major classes encompass metalloproteases, phospholipases, disintegrins, and C-type lectins, as reviewed (3, 26). C-type lectins are animal proteins of about 130 amino acids long, containing at least a carbohydrate recognition domain (CRD) capable of mediating sugar and calcium binding. The carbohydrate recognition is directly related to some biological activities like cell-cell adhesion, serum glycoprotein turnover, and innate immune responses against potential pathogens (9). Snake venom C-type lectins also contain the conserved CRD and share significant primary structure similarities with the majority of C-type lectins, but most of them neither necessarily bind to carbohydrate molecules nor require calcium ions for their activity (3, 9). For instance, convulxin (CVX), a very well studied snake venom C-type lectin, induces Ca2+-dependent platelet aggregation, which is inhibited and reversed by EDTA (49). Convulxin is a heterodimeric toxin from the venoms of South American rattlesnakes, Crotalus durissus terrificus and C. d. cascavella (36, 49). This protein consists of two subunits, alfa (CVXa , 13.9 kDa) and beta (CVXb , 12.6 kDa), joined by inter and intra-chain disulfide bounds, arranged in a tetrameric a4b4 conformation (4, 29). The Ca2+-dependent activation of platelets and their aggregation are mediated via p62/GPVI collagen receptor (35, 49). Some other snake toxins with similar properties of activating and aggregating platelets are also known. They are bitiscetin, from the venom of Bitis arietans (16); botrocetin, from Bothrops jararaca (12); flavocetin A (13); ophioluxin, a protein from Ophiophagus hannah (10); and mucrocetin, a platelet-agglutinin from Trimeresurus mucrosquamatus (20). Recombinant convulxin (rCVX) has been cloned and expressed in Drosophila cells. Purified rCVX from cell culture supernatants binds strongly to human platelet GPVI in western blot assay when whole platelet proteins or recombinant human GPVI are used as targets. Importantly, rCVX induces the aggregation of platelets in platelet-rich plasma, indicating that the recombinant CVX subunits can assemble into a functionally competent complex (14).
During the procedures for the cloning of convulxin a and b subunits, we have isolated several cDNA precursors which are CVX subunit homologs.
In this work, we have characterized one of them, a new member of the snake venom C-type lectin family, named crotacetin (CTC), with predictable platelet aggregation property and unexpected antimicrobial activity.
MATERIALS AND METHODS
Snake and snake venom
For the construction of the venom gland cDNA library, a pair of glands was excised from an adult specimen of Crotalus durissus terrificus captured in São Paulo State and provided by the Laboratory of Herpetology, Butantan Institute, São Paulo, Brazil. The snake was milked for venom collection and induction of the maximum level of RNA synthesis in the venom gland (41). The crude venom was vacuum dried and kept at -20°C until protein purification. The venom of Crotalus durissus cascavella was a gift from the Regional Snake Laboratory of Fortaleza (LAROF), Ceará, Brazil. The venom of Crotalus durissus collilineatus was purchased from the Bio-Agents Serpentarium, located in the city of Batatais, São Paulo, Brazil.
Crotalus durissus terrificus venom gland cDNA library construction
The cDNA library was constructed as described elsewhere (38). Briefly, poly(A+) RNAs were purified from a pair of venom glands excised from a single specimen of South American rattlesnake, C. d. terrificus (Cdt 9706). The complementary DNAs (cDNAs) were synthesized, selected by size, and cloned into a phagemid vector a lambda phage derivative (l ZapII, Strategene). Recombinant phagemids were packed into viable phage particles and used to infect E. coli XL1 Blue MRF cells (Stratagene, La Jolla, CA). The venom gland cDNA library was titrated, amplified, and stored at -80°C, in 7% DMSO, for posterior utilization.
PCR homology cloning
Based on nucleotide sequences of subunits a (or A) and b (or B) of convulxin (CVX) from C. durissus terrificus (GenBank accession no. AF541882 and Y16348, convulxin subunit alpha; AF541881 and Y16349, convulxin subunit beta), we were able to synthetize (Invitrogen Life Technologies, Brazil) one oligonucleotide forward primer, CVXA/B-FW1 (5-TCTCTCTGCAGGGAAGGAAG-3), and two reverse primers, CVXA-RV1A (5-TCCTTGCTTCTCCAGACTTCA-3) and CVXB-RV2B (5-ACTTCACACAGCCGGATCTT-3), which correspond to 5-UTR of CVX subunits a and b (forward primer), and to 3-UTRs of CVX subunit a (reverse primer RV1A) and subunit b (reverse primer RV2B), respectively. The gene of one subunit of crotacetin (CTC a subunit) was amplified with the same primer pair used to amplify CVX subunit a , in the following way: phage particles (107-108 pfu) of C. durissus terrificus venom gland cDNA library, 10 pmoles of each primer, and 25 µl of ExLONGase enzyme mix (Invitrogen Life Technologies, San Diego, CA) were mixed and the polymerase chain reaction (PCR) was performed according to the manufacturers instructions. The long distance PCR (LD-PCR) products were purified from the gel slice and cloned into pCR2.1-TOPO (Invitrogen Life Technologies, San Diego, CA).
The gene was sequenced with ABI Prism Big Dye Terminator (Perkin Elmer, Foster City, CA) in an automated sequencer (ABI Prism 373 or 377, Perkin Elmer) using synthetic oligonucleotides designed for CVXA/B sequences (this work). The cloned crotacetin mRNA (accession number AF541884) was compared against nucleotide sequences on the GenBank at NCBI (31), using the BLAST algorithm and the Biocomputing software Lasergene (DNAStar, Inc., Madison, WI).
Similarity search and homology modeling
The amino acid sequence predicted from the respective Crotalus durissus terrificus precursor cDNA was compared against the protein data bank (pdb) (40) using BLASTP, as a tool for protein search and alignment (2). Several sequences, chosen as the best score after alignment, were used to identify conserved residues in homologous sequences. Snake venom C-type lectin sequences from the venoms of Trimeresurus flavoviridis (pdb entry code 1C3A, chain B) (13), Trimeresurus mucrosquamatus (1V4L, chain B) (20) and Crotalus durissus terrificus (1UOS, chain B and 1UMR, chain B) (4, 29) were aligned by CLUSTALW (18) using default parameters.
To build a tridimensional structure of CTC b subunit C-type lectin, one thousand models were generated with PARMODEL (48), which parallel the MODELLER (42) software in a Beowulf cluster (16 nodes). The best model was selected according to the modeller objective function and was evaluated by PROCHECK (24), WHATCHECK (19), and 3DANALYSIS (5). The permissible angles of amino acid residues in the spatial structure of CTC b subunit were also evaluated by RAMACHANDRAN plot (39).
Crotacetin purification
Whole venom (35 mg) was dissolved in a 0.2-M ammonium bicarbonate buffer (pH 8.0) and then clarified by high-speed centrifugation (4500xg for 1 min). The supernatant was injected onto a molecular exclusion HPLC column (Superdex 75, 1 x 60 cm, GE Healthcare), previously equilibrated with the same buffer used for solubilization of the whole venom. Chromatographic process was performed with a flow rate of 0.2 ml/min, and monitored at 280 nm. Fractions corresponding to crotacetin were pooled and lyophilized. After this first step of purification, crotacetin was re-purified by reverse phase HPLC. Approximately 1 mg of the purified protein was dissolved in the buffer A (TFA 0.1% in aqueous solution), used for equilibration of the analytical µ-Bondapack C18 column (0.39 x 30 cm). The elution of highly purified crotacetin was carried out using a linear and discontinuous buffer B gradient (66% of Acetonitrile in buffer A). The chromatographic run was conducted at constant flow rate of 1.0 ml/min and monitored at 214 nm.
Reduction, S-carboxymethylation and determination of N-terminal sequence
Two milligrams of purified crotacetin were dissolved in 200 µl of a 6.0-M guanidine chloride solution (Merck, Darmstadt, Germany) containing 0.4 M Tris-HCl and 2 mM EDTA (pH 8.15). Nitrogen was blown over the top of the protein solution for 15 min, followed by molecular reduction with 200 µl of 6.0 M dithiotreitol (DTT) and further carboxymethylation with 14C-iodoacetic acid and cold iodoacetic acid. Nitrogen was again blown over the surface of the solution and the reaction tube was sealed. This solution was incubated in the dark at 37°C for 1 hour and desalted using a Sephadex G25 column (0.7 x 12 cm) with 1.0 M acetic acid buffer. The eluted RC-Crotacetin was then applied on the reverse phase HPLC µ-Bondapack C-18 column (0.39 x 30 cm), previously equilibrated with buffer A (TFA 0.1% in aqueous solution). The subunits of crotacetin were eluted with a nonlinear gradient concentration of buffer B (acetonitrile 66% in buffer A), and the fractions corresponding to each crotacetin subunit were recovered, lyophilized, and stored at -80°C. Crotacetin subunits were then sequenced by automatic Edman degradation, using a gas-liquid protein sequencer (Applied Biosystems model Precise). The amino acid phenylthiohydantoin (PTH) derivatives were identified using a PTH-analyzer (Applied Biosystems model 450 micro-gradient).
Platelet aggregation
Platelet-rich plasma (PRP) was prepared as described by Chudzinski-Tavassi et al. (7), and the evaluation of platelet aggregation was performed with a Chrono-Log Lumi aggregometer (Havertown, PA). PRP samples were incubated at 37°C for 2 min with different concentrations of purified crotacetin. Platelet agglutination was monitored by turbidimetry and expressed as an increase of light transmittance. Collagen was used as control of platelet aggregation.
Antimicrobial activity and electron microscopy
Xanthomonas axonopodis pv passiflorae (Gram-negative) or Clavibacter michiganensis michiganensis cells were harvested from fresh agar plates, and suspended in sterile distilled water (A650nm=0.3/cc 103CFU/ml). Aliquots of bacterial suspension were diluted to 10-5 CFU/ml and incubated with crotacetin (150 µg/ml) during 20 minutes at 37°C. Then, the capacity of survival was assayed on nutrient (Difco) plates (n=5). In both antibacterial assays, morphological alterations were visualized by electron microscopic, in absence (control) or presence of crotacetin (A650nm=0.3/cc 103 CFU/ml). For this purpose, bacterial samples were fixed with 1% osmium tetraoxide (Agar Scientific Ltd) for 2 h at 25°C. Sections were washed three times, dehydrated in increasing concentrations of ethanol and propylene oxide, and embedded in Epon resin (Agar Scientific). Polymerization was performed at 60°C for 48 h, and ultrathin sections were prepared with a Sorvall MT2 ultramicrotome. The sections were placed on 5% collodion-coated 100-mesh grids, and stained with 4% uranyl acetate (Agar Scientific) for 15 min, followed by 2.6% lead citrate (Agar Scientific) for 15 min. Samples were observed with a Hitachi 1100 transmission electron microscope (Hitachi Scientific Instruments, Japan), operating at 100 kV.
RESULTS
PCR homology cloning of crotacetin b subunit
The gene coding for crotacetin b subunit, CTCb , (GenBank accession number AF541884) was isolated from Crotalus durissus terrificus venom gland cDNA library by PCR-homology screening with specific primers for the 5-UTR and 3-UTR of both convulxin subunits a (CVXa ) and b (CVXb ), as described in the section materials and methods.
The cloned CTCb gene is 513 base pairs (bp) long with a 5-untranslated region (5-UTR) strictly conserved in all convulxin-like and anti-thrombin-like precursors isolated so far (Figure 1). In CTCb gene, the ATG start codon is located 28 bp downstream, and the stop codon (TGA) is located 496 bp. A sequence corresponding to the signal peptide lies between the nucleotides 28 and 96 (Figure 1, underlined).
At nucleotide level, the similarity between CTCb and CVXb is higher than between CTCb and CVXa or CTCb and anti-thrombin-like subunit (ATLs). In contrast, the similarity of CVXa and ATLs is proportionally high. The CTCb gene precursor predicts a polypeptide of 148 residues of amino acids, 23 corresponding to the leader sequence, and a molecular mass of 14.3 kDa.
Sequence alignment and tridimensional modeling
Comparison of predicted amino acid sequence of CTCb gene against protein data bank reveals high similarity between CTCb and C-type lectin subunits from the venom of Trimeresurus flavoviridis (pdb entry code 1C3A, chain B), Trimeresurus mucrosquamatus (1V4L, chain B) and Crotalus durissus terrificus (1UOS, chain B and 1UMR, chain B) (Figure 2A). The similarity between CTCb and these other snake venom aggregating toxins is around 50%. If conserved substitutions are considered, the similarity exceeds 70%. In primary structure of CTCb , the eight residues of cysteine are located in the same position of all aligned sequences. These positions include six residues that are involved in the intra-chain disulfide bridges, and two other "extra" cysteines in the carboxi- (Cys3) and amino- (Cys77) terminals. The model of CTCb , generated by computer programs, shows an overall topology of five b-strands and two a-helices forming a globular structure with a lateral loop similar to the other convulxin-like C-type lectins (Figure 2B). The lateral loop contributes to the formation of heterodimers that are stabilized by the "extra" cysteine residue.
Ramachandran diagram of CTCb model indicates that psi (y ) and phi (f ) angles of the majority of amino acid residues are located in a thermodynamically favorable region (Figure 2C).
Isolation, reduction and determination of N-terminal sequence of crotacetin from C. durissus
By exclusion chromatography, crotacetin appear as a minor fraction peak in the venom of at least three Crotalus durissus subspecies, namely, Crotalus durissus cascavella, Crotalus durissus terrificus and Crotalus durissus collilineatus (Figure 3A). In the venom of Crotalus durissus cascavella, the amount of crotacetin is significantly abundant (it represents around 0.8% of the proteins in the crude venom). Thus, crotacetin was isolated and characterized from this venom. Purified crotacetin from Crotalus durissus cascavella shows an apparent molecular mass of 70 kDa by gel permeation chromatography, and it appears as two subunits of different sizes by reverse phase HPLC (Figure 3B). Furthermore, by molecular exclusion chromatography, it appears as a high molecular weight protein, indicating the presence of oligomeric forms.
The partial N-terminal amino acid sequence of purified crotacetin (b subunit) corresponds to the one predicted from the gene sequence (Figure 3C).
Platelet aggregation assay
Crotacetin is capable of aggregating human platelet in platelet rich plasma (PRP) in a dose-dependent manner: 22% at a concentration of 32.8 µg/ml (47 µM), 36% at 49.3 µg/ml (70 µM), and 84% at 65.5 µg/ml (94 µM) (Figure 4).
Antimicrobial activity of native crotacetin and isolated a and b subunits
The whole (intact) crotacetin protein decreased the bacterial growth of two plant pathogens: Xanthomonas a. pv. passiflorae, Gram-negative, and Clavibacter m. michiganensis, Gram-positive. The inhibition rates were about 87.8% and 96.4%, respectively. The isolated chains did not show significant antimicrobial activity (Figures 5a and 5b) for the species of bacteria tested. In the case of Xanthomonas a. pv. passiflorae, crotacetin induced a massive vacuolization of cell cytoplasm and, in some cases, ruptured the cell membrane (Figures 5c and 5d).
All genes were isolated from C. d. terrificus venom gland cDNA phage library by PCR homology screening. Sequences were aligned using CLUSTALW (26) with default parameters. The Arabic numerals in the left side of each precursor correspond to their GenBank accession numbers (AF541881, convulxin subunit b mRNA; AF541882, convulxin subunit a mRNA; AF541883, anti-thrombin like mRNA; and AF541884, crotacetin subunit b mRNA, all from Crotalus durissus terrificus). Start and stop codons are boxed in gray. Strictly conserved 5-untraslated sequences (5-UTR), where the primer CVXA/B FW exactly anneals, are underlined. Asterisks represent conserved nucleotides of homologous sequences. Deduced amino acid sequence is presented under the nucleotide sequences in bold capital letters. The signal peptide is underlined.
DISCUSSION
Using specific forward primer for 5-UTR and reverse for 3-UTR for both subunits of convulxin, subunits a (CVXa ) and b (CVXb ), we have isolated several cDNA precursor homologs of convulxin (CVX) from Crotalus durissus terrificus venom gland cDNA library. The nucleotide sequence of two of these precursors, precisely of their subunits, CVXa and CVXb subunit sequences, and the deduced amino acid sequence of CTCb are shown in Figure 1. These cDNA sequences present conserved nucleotides starting at 27 bp, from the ATG initiation codon, extending several bases along the precursor. All of the isolated genes, coding for convulxin-like subunits, encompass open reading frames (ORFs) of approximately 500 nucleotides (nt) - CVXb , 490 nt; CTCb , 513 nt; CVXa , 537 nt; ATLs, 522 nt. Crotacetin b and CVXb genes are almost identical (82% of similarity, 439/537 nt), whereas CVXa and ATLs genes are more related to each other (about 83%, 409/490 nt). When CTCb mRNA is compared with other sequences in the gene databank, more than 86% identity is found. For example, mucrocetin b chain mRNA (AY390534), from Protobhotrops mucrosquamatus, shares 87% identity (439/537 nt). Hundreds of mRNA sequences of snake venom C-type lectin, from GenBank, share some similarity with crotacetin b subunit and with each other.
The high homology between C. durissus C-type lectin genes and some other aggregating toxin genes from different snakes points out to their own evolutionary history. These genes seem to have arisen from more than one single event of gene duplication, what probably occurred after the division of Viperidae and Colubridae. The a - and b - chains of the C-type lectins are restricted to viper and pit viper snakes and therefore compose a monophyletic gene clade (11). However, duplication is not the exclusive event for toxin gene evolution; nucleotide substitution (transversion and transition) and deletion also play some role. Consequently, families of homologous genes and polypeptides are generated with diverse functions or targets. In fact, toxin genes present extremely highly conserved non-coding regions, whereas hyperdiverse coding regions are found (1, 30, 33, 46). In general, the coding region of a given toxin gene lies in exon, which is separated from each other encompassing the leader sequence of the toxin and the 5-UTR (6, 34, 37). Thus, the gene organization has influenced not only its own evolution, but also the toxin diversity. For instance, gene organization contributes to accelerated evolution of polypeptides, since gene hypervariation benefits evolutionary advantage (27, 32, 45).
Comparison between a deduced amino acid sequence of crotacetin b subunit and members of snake venom hemorrhagic toxins corroborates a consensual structural characteristic of convulxin-like proteins: the eight conserved residues of cysteine. Six cysteine residues are involved in intra-chain disulfide bridges, linking at 4-15, 32-121 and 98-113 residues, and the other two cysteines are recruited in the formation of the heterodimer, in a head-to-head manner, resulting in the a4b4 quaternary structure (20, 29). To explore the structural conformation adopted by crotacetin b subunit and to build a 3-D model of CTCb , we had utilized amino acid sequences and coordinate data from convulxin-like snake venom C-type lectins, whose crystal structures were previously resolved by X-ray diffraction. It is very well known that the two most critical problems in homology modeling are the similarity degrees among target sequences and templates, and evidently the alignment fidelity (42). In the case of crotacetin b subunit, its predicted 3-D structural model is practically identical to the experimentally resolved ones.
Crotacetin b subunit was initially cloned from Crotalus durissus terrificus venom gland, but latter it was noted that crotacetin is found in the venom of diverse Crotalus durissus subspecies, appearing as a minor fraction peak in chromatograms of the venoms of Crotalus durissus cascavella, Crotalus durissus terrificus and Crotalus durissus collilineatus. In the venom of Crotalus durissus cascavella, the amount of crotacetin is significantly abundant (around 0.8% of all proteins in the crude venom). The observation that crotacetin is expressed in the venom of several subspecies of South American rattlesnakes, inhabiting distinct geographical locations, confirm the phenomenon of hypervaryability widely seen in the snake venom composition (43, 44). Interestingly, even if snake venom C-type lectins are diverse, they are restricted to the venom of Viperidae, the family of Crotalus durissus species, as mentioned above and studied in detail elsewhere (11). Thus far, crotacetin was isolated and characterized from the venom of C. d. cascavella.
Based on the fact that CTC b subunit seems to belong to the class of convulxin-like proteins, with the consensual motif of C-type lectin domains (CTLDs), including the carbohydrate recognition domain (CRD), two main biological assays with purified crotacetin were conducted: platelet aggregation and antimicrobial test.
Purified crotacetin from Crotalus durissus cascavella appears as two subunits of different sizes (apparent molecular mass of 70 kDa) and, by gel permeation, a high molecular weight oligomeric form of this protein is evidenced.
Using human platelet rich plasma, it was observed that CTC is capable of aggregating platelets in a dose-dependent manner and, in higher doses, the platelet aggregation is more sustainable than collagen. Actually, platelet aggregation is a common phenomenon of snake venom C-type lectins, usually mediated by glycoprotein receptors on platelet membranes. Kanaji et al. (22) demonstrated that in addition to GPVI, convulxin binds to native human GPIba , exhibiting dual specificity to both platelet receptors. Thus, it remains to be verified what receptor this novel member of convulxin-like family is able to bind, that is, would crotacetin be able to interact with and activate platelet via GPVI, GPIba , or other collagen receptor for platelet like GPIa-IIa (a2b1 integrin)? Furthermore, glycoprotein receptors on erythrocyte membranes appear as specific molecular target for convulxin-like snake toxins, as it was demonstrated in a recent work on recombinant BJcuL, a C-type lectin of Bhotrops jararacussu venom (23). Since this is the first report of a new convulxin homolog, it should be also essential from the biochemical point of view to determine not only the strict dependence of crotacetin by calcium ions, as observed for convulxin (49), but also the co-influence of other molecules in the activation and induction of platelet aggregation.
Noteworthy, crotacetin showed a significant antimicrobial activity against two different bacterial strains, Xanthomonas axonopodis pv passiflorae and Clavibacter michiganensis michiganensis. The oligomeric form of crotacetin reduced the overall growth of both bacteria. However, the separation of intact oligomeric protein into their isolated chains abolishes significantly its antimicrobial activity. As seen before, tetrameric form is a typical structure adopted by several snake venom convulxin-like C-type lectins, and this quaternary arrangement seems to be essential for antimicrobial activity. The microscopic effect of crotacetin on Xanthomonas a. pv. passiflorae involved the induction of cytoplasmic vacuolization and membrane rupture. From our point of view, these latter results are of particular relevance, since they concern to antimicrobial activities of a snake venom C-type lectin. The most studied CTLDs-containing proteins with the property of binding to microorganisms are the mannose binding lectins (MBLs) and the lectins receptors located on antigen-presenting cell membranes. MBLs are involved in the mammalian first-line of defense by binding to bacteria, viruses, protozoa, and helminthes, initiating a diverse range of host response (21). In addition, C-type lectin receptors (CLRs) on dendritic cells are type II transmembrane proteins implicated in the pattern recognition of pathogens and in the distinction of self and no-self antigen recognition in mammals (15).
Taken these results together, it is evident that snake venom C-type lectins have their structural domains derived from a common ancestral precursor, which comprises not only a multi-gene family, but also homologous polypeptides possessing conserved C-type lectin domains with the ability to interact with glycoproteins on blood cell membranes, and with microbial cells as well.
In this work, we report (a) the cloning of a novel C-type lectin gene from C. durissus terrificus; (b) the isolation and characterization of its gene product, crotacetin b subunit, from the venom of three C. durissus subspecies; (c) the predominant presence of crotacetin in the venom of C. durissus cascavela; and (d) the prediction of its tridimensional structure. Importantly, we demonstrated that crotacetin induces platelet aggregation and presents antimicrobial activity against both Gram-positive and Gram-negative bacteria.
ACKNOWLEDGEMENTS
We are thankful to Dr. A. M. Chudzinski-Tavassi, Laboratory of Biochemistry and Biophysics, Butantan Institute, São Paulo, Brazil, for the evaluation of platelet aggregation assays. We are also grateful to Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES, Conselho Nacional de Desenvolvimento Científico e Tecnológico - CNPq, Fundação de Amparo à Pesquisa do Estado de São Paulo - FAPESP, and Fundação Cearense de Apoio ao Desenvolvimento Científico e Tecnológico - FUNCAP (Brazil). B.S. Cavada and T. Yamane are senior investigators of CNPq (Brazil).
This work was carried out in compliance with the current guidelines governing genetic experimentation in Brazil.
Received: December 20, 2004
Accepted: May 18, 2005
Published online: October 30, 2005
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Publication Dates
-
Publication in this collection
21 Nov 2005 -
Date of issue
Dec 2005
History
-
Accepted
18 May 2005 -
Received
20 Dec 2004