Abstract
Background:
In recent decades, snake venom disintegrins have received special attention due to their potential use in anticancer therapy. Disintegrins are small and cysteine-rich proteins present in snake venoms and can interact with specific integrins to inhibit their activities in cell-cell and cell-ECM interactions. These molecules, known to inhibit platelet aggregation, are also capable of interacting with certain cancer-related integrins, and may interfere in important processes involved in carcinogenesis. Therefore, disintegrin from Crotalus durissus collilineatus venom was isolated, structurally characterized and evaluated for its toxicity and ability to interfere with cell proliferation and migration in MDA-MB-231, a human breast cancer cell line.
Methods:
Based on previous studies, disintegrin was isolated by FPLC, through two chromatographic steps, both on reversed phase C-18 columns. The isolated disintegrin was structurally characterized by Tris-Tricine-SDS-PAGE, mass spectrometry and N-terminal sequencing. For the functional assays, MTT and wound-healing assays were performed in order to investigate cytotoxicity and effect on cell migration in vitro, respectively.
Results:
Disintegrin presented a molecular mass of 7287.4 Da and its amino acid sequence shared similarity with the disintegrin domain of P-II metalloproteases. Using functional assays, the disintegrin showed low cytotoxicity (15% and 17%, at 3 and 6 μg/mL, respectively) after 24 h of incubation and in the wound-healing assay, the disintegrin (3 μg/mL) was able to significantly inhibit cell migration (24%, p < 0.05), compared to negative control.
Conclusion:
Thus, our results demonstrate that non-RGD disintegrin from C. d. collilineatus induces low cytotoxicity and inhibits migration of human breast cancer cells. Therefore, it may be a very useful molecular tool for understanding ECM-cell interaction cancer-related mechanisms involved in an important integrin family that highlights molecular aspects of tumorigenesis. Also, non-RGD disintegrin has potential to serve as an agent in anticancer therapy or adjuvant component combined with other anticancer drugs.
Keywords:
Crotalus durissus collilineatus; Non-RGD disintegrin; Cell migration; Cell adhesion; Human breast cancer; MDA-MB-231
Background
Disintegrins are low-molecular-mass cysteine-rich peptides found in snake venom that comprise from 40 to 100 amino acid residues [11. Kini RM, Evans HJ. Structural domains in venom proteins: evidence that metalloproteinases and nonenzymatic platelet aggregation inhibitors (disintegrins) from snake venoms are derived by proteolysis from a common precursor. Toxicon. 1992;30(3):265–93.
2. Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9.-33. Huang TF, Holt JC, Lukasiewicz H, Niewiarowski S. Trigramin. A low molecular weight peptide inhibiting fibrinogen interaction with platelet receptors expressed on glycoprotein IIb-IIIa complex. J Biol Chem. 1987; 262(33):16157-63.]. In 1987 Huang et al. observed that a small protein isolated from Trimeresurus gramineus venom, called “trigramin”, presenting the arginine-glycine-aspartic acid (RGD) domain, was able to inhibit platelet aggregation, by preventing the connection between fibrinogen and platelets stimulated by ADP [33. Huang TF, Holt JC, Lukasiewicz H, Niewiarowski S. Trigramin. A low molecular weight peptide inhibiting fibrinogen interaction with platelet receptors expressed on glycoprotein IIb-IIIa complex. J Biol Chem. 1987; 262(33):16157-63.]. The term “disintegrin” was coined by Gould et al. when they demonstrated that the mechanism for inhibition of platelet aggregation was related to interaction between fibrinogen and αΠb,β3 platelet integrins [44. Gould RJ, Polokoff MA, Friedman PA, Huang TF, Holt JC, Cook JJ, et al. Disintegrins: a family of integrin inhibitory proteins from viper venoms. Proc Soc Exp Biol Med. 1990;195(2):168-71.].
Most snake venom disintegrins are believed to be released by proteolytic processing of snake venom metalloproteases (SVMP) from the class P-II [11. Kini RM, Evans HJ. Structural domains in venom proteins: evidence that metalloproteinases and nonenzymatic platelet aggregation inhibitors (disintegrins) from snake venoms are derived by proteolysis from a common precursor. Toxicon. 1992;30(3):265–93., 55. Selistre-de-Araujo HS, Pontes CLS, Montenegro CF, Martin ACBM. Snake venom disintegrins and cell migration. Toxins (Basel). 2010;2(11):2606–21.]. Briefly, SVMP can be classified into three classes according to domain composition present in their structures: (i) P-I SVMP only contains a domain of metalloproteases; (ii) P-II SVMP has a metalloprotease domain and a disintegrin domain on its C-terminal tail, that can be released; (iii) and P-III SVMP contains a metalloprotease domain, a disintegrin-like domain and cysteine-rich domain [66. Sanchez EF, Flores-Ortiz RJ, Alvarenga VG, Eble JA. Direct fibrinolytic snake venom metalloproteinases affecting hemostasis: structural, biochemical features and therapeutic potential. Toxins (Basel). 2017;9:12.].
Similarly to metalloproteases, disintegrins can also be classified according to their structure, considering the numbers of disulfide bonds and amino acid residues: (i) short disintegrins contain 41 to 51 amino acid residues, stabilized by 4 disulfide bonds; (ii) medium-sized disintegrins contain approximately 70 amino acid residues and 6 disulfide bonds; (iii) long disintegrins, with approximately 84 residues and 7 disulfide bonds; (iv) and the last group that comprises homo- and heterodimeric dis-integrins, with approximately 67 residues per subunit, 4 intrachain disulfide bonds, in addition to 2 interchain cystine bonds, stabilizing the molecules [77. Calvete JJ, Jürgens M, Marcinkiewicz C, Romero A, Schrader M, Niewiarowski S. Disulphide-bond pattern and molecular modelling of the dimeric disintegrin EMF-10, a potent and selective integrin α5β1 antagonist from Eristocophis macmahoni venom. Biochem J. 2000;345(3):573-81.
8. Bilgrami S, Yadav S, Kaur P, Sharma S, Perbandt M, Betzel C, et al. Crystal structure of the disintegrin heterodimer from saw-scaled viper (Echis carinatus) at 1.9 a resolution. Biochemistry. 2005;44(33):11058-66.
9. Bilgrami S, Tomar S, Yadav S, Kaur P, Kumar J, Jabeen T, et al. Crystal structure of schistatin, a disintegrin homodimer from saw-scaled viper (Echis carinatus) at 2.5 a resolution. J Mol Biol. 2004;341(3):829-37.-1010. Calvete JJ, Moreno-Murciano MP, Theakston RD, Kisiel DG, Marcinkiewicz C. Snake venom disintegrins: novel dimeric disintegrins and structural diversification by disulphide bond engineering. Biochem J. 2003;372(Pt 3): 725-34.].
In general, these molecules carry this name because they have the RGD motif in their primary amino acid sequence, which is capable of binding to integrins [44. Gould RJ, Polokoff MA, Friedman PA, Huang TF, Holt JC, Cook JJ, et al. Disintegrins: a family of integrin inhibitory proteins from viper venoms. Proc Soc Exp Biol Med. 1990;195(2):168-71.]. However, due to a mutation or a sequence of up to three mutations, other domains can be generated, also characterizing a disintegrin by inhibiting other types of integrins [22. Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9., 1111. Juárez P, Comas I, González-Candelas F, Calvete JJ. Evolution of snake venom disintegrins by positive Darwinian selection. Mol Biol Evol. 2008; 25(11):2391–407.]. The classical RGD domain is capable of blocking αΠb,β3, α5β1, α8β1, αvβ1 and αvβ3 integrins, while the KGD domain inhibits integrin αΠb,β3 with high selectivity; WGD domain inhibits αIIbβ3, α5β1, and αvβ3 integrins; MGD and VGD domains can affect the α5β1 integrin function; KTS and RTS domains are inhibitors of α1β1 integrin; MLD domain targets the integrins α3β1, α4β1, α4β7, α6β1, α7β1 and α9β1; and the adhesive function of αIIbβ3 can be blocked by the MVD domain [1212. Sanz L, Bazaa A, Marrakchi N, Pérez A, Chenik M, Bel Lasfer Z, et al. Molecular cloning of disintegrins from Cerastes vipera and Macrovipera lebetina transmediterranea venom gland cDNA libraries: insight into the evolution of the snake venom integrin-inhibition system. Biochem J. 2006; 395(2):385–92.
13. Calvete JJ, Juárez P, Sanz L. Snake venomics and disintegrins: portrait and evolution of a family of snake venom integrin antagonists. In: Mackessy SP, editor. Handbook of venoms and toxins of reptiles. Boca Ratón: CRC Press, Taylor & Francis; 2009. p. 337–57.-1414. Calvete JJ. Brief history and molecular determinants of snake venom disintegrin evolution. In: Kini RM, Markland F, McLane MA, Morita T, editors. Toxins and hemostasis: from bench to bedside. Amsterdam: Springer; 2010. p. 285–300.]. As an example, we can mention ussuristatin 2 Agkistrodon ussuriensis venom [1515. Oshikawa K, Terada S. Ussuristatin 2, a novel KGD-bearing disintegrin from Agkistrodon ussuriensis venom. J Biochem. 1999;125(1):31–5.] and barbourin from Sistrurus M. barbouri [1616. Scarborough RM, Rose JW, Hsu MA, Phillips DR, Fried VA, Campbell AM, et al. Barbourin. A GPIIb-IIIa-specific integrin antagonist from the venom of Sistrurus m. barbouri. J Biol Chem. 1991;266(15):9359–62.], which lack the classical RGD domain, as well as atrolysin E from Crotalus atrox, from P-II SVMP, which possesses the MVD motif [1717. Hite LA, Shannon JD, Bjarnason JB, Fox JW. Sequence of a cDNA clone encoding the zinc metalloproteinase hemorrhagic toxin e from Crotalus atrox: evidence for signal, zymogen, and disintegrin-like structures. Biochemistry. 1992;31(27):6203–11.].
Due to this ability related to integrins, disintegrins also can be used for the therapy of vascular diseases and bacterial infections (α5β1), autoimmune diseases and inflammation (α4β1, α7β1 and α9β1), thrombosis and acute coronary syndromes (αΠbβ3), rheumatoid arthritis and osteoporosis (αvβ3), tumor angiogenesis (α1β1 and αvβ3) and metastasis (αvβ3) [22. Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9.]. Nowadays, there are two drugs approved by the Food and Drug Administration (FDA) whose design is based on two disintegrins isolated from snake venoms. Eptifibatide (Integrilin®) and Tirofiban (Aggrastat®) were approved in 1998 and 1999, respectively, and are used for acute coronary syndromes because they target the αΠb,β3 integrin [1818. King GF. Venoms as a platform for human drugs: translating toxins into therapeutics. Expert Opin Biol Ther. 2011;11(11):1469–84.]. Eptifibatide is based on the KGD motif from barbourin, a disintegrin from Sistrurus miliarius barbourin [1919. O'Shea JC, Tcheng JE. Eptifibatide: a potent inhibitor of the platelet receptor integrin glycoprotein IIb/IIIa. Expert Opin Pharmacother. 2002;3(8):1199–210.], while Tirofiban is based on the RGD motif from echistatin, a disintegrin from Echis carinatus [2020. Menozzi A, Merlini PA, Ardissino D. Tirofiban in acute coronary syndromes. Expert Rev Cardiovasc Ther. 2005;3(2):193–206.].
Integrins are closely related to the initiation, promotion and progression of tumors and metastasis [2121. Arruda Macêdo JK, Fox JW, de Souza Castro M. Disintegrins from snake venoms and their applications in cancer research and therapy. Curr Protein Pept Sci. 2015;16(6):532–48.]. Therefore, disintegrins may play an important therapeutic role as a potential anticancer drug, as is the case of contortrostatin [22. Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9.]. Zhou et al. observed that this dis- integrin from Agkistrodon contortrix contortrix venom was not able to cause cytotoxicity in MDA-MB-435 cells (human melanoma cells formerly classified as a human breast cancer cell line), and also prevented the binding of these cells to integrins (αvβ3) and extracellular matrix proteins, such as vitronectin and fibronectin, thus inhibiting the adhesion process [2222. Zhou Q, Sherwin RP, Parrish C, Richters V, Groshen SG, Tsao-Wei D, et al. Contortrostatin, a dimeric disintegrin from Agkistrodon contortrix contortrix, inhibits breast cancer progression. Breast Cancer Res Treat. 2000;61(3):249–60.]. There are many other examples of disintegrins that act as anticancer agents, such as saxatilin, from Gloydius saxatilis, which is capable of inhibiting the growth of tumors [2323. Kim KS, Kim DS, Chung KH, Park YS. Inhibition of angiogenesis and tumor progression by hydrodynamic cotransfection of angiostatin K1-3, endostatin, and saxatilin genes. Cancer Gene Ther. 2006;13(6):563–71.], leucurogin, from Bothrops leucurus, that has an anti-angiogenic effect [2424. Higuchi DA, Almeida MC, Barros CC, Sanchez EF, Pesquero PR, Lang EA, et al. Leucurogin, a new recombinant disintegrin cloned from Bothrops leucurus (white-tailed-jararaca) with potent activity upon platelet aggregation and tumor growth. Toxicon. 2011;58(1):123–9.] and the adinbitor, from Agkistrodon halys stejneger, which also inhibits angiogenesis both in vitro and in vivo [2525. Wang JH, Wu Y, Ren F, Lü L, Zhao BC. Cloning and characterization of Adinbitor, a novel disintegrin from the snake venom of Agkistrodon halys brevicaudus stejneger. Acta Biochim Biophys Sin Shanghai. 2004;36(6):425–9.]. Eritostatin, from Eristicophis macmahoni venom, was able to inhibit the migration of melanoma cells, an effect mediated by binding of fibronectin to integrins [2626. Tian J, Paquette-Straub C, Sage EH, Funk SE, Patel V, Galileo D, et al. Inhibition of melanoma cell motility by the snake venom disintegrin eristostatin. Toxicon. 2007;49(7):899–908.], whereas crotatroxin 2, from Crotalus atrox venom, inhibited cell migration of breast carcinoma cells [2727. Galán JA, Sánchez EE, Rodríguez-Acosta A, Soto JG, Bashir S, McLane MA, et al. Inhibition of lung tumor colonization and cell migration with the disintegrin crotatroxin 2 isolated from the venom of Crotalus atrox. Toxicon. 2008;51(7):1186–96.]. Interestingly, cilengitide, a cyclic mimetic peptide that has affinity for αvβ3 and αvβ5 integrins, displays antiangiogenic action in low amounts. However, in phase III clinical trials, this drug did not show positive results for patients newly diagnosed with glioblastoma [2828. Zakraoui O, Marcinkiewicz C, Aloui Z, Othman H, Grépin R, Haoues M, et al. Lebein, a snake venom disintegrin, suppresses human colon cancer cells proliferation and tumor-induced angiogenesis through cell cycle arrest, apoptosis induction and inhibition of VEGF expression. Mol Carcinog. 2017; 56(1):18–35., 2929. Desgrosellier JS, Cheresh DA. Integrins in cancer: biological implications and therapeutic opportunities. Nat Rev Cancer. 2010;10(1):9–22.]. There are also studies that evaluated the effects of disintegrins on individual stages of metastasis, including cell cycle arrest, extravasation and cell migration [2121. Arruda Macêdo JK, Fox JW, de Souza Castro M. Disintegrins from snake venoms and their applications in cancer research and therapy. Curr Protein Pept Sci. 2015;16(6):532–48.].
Snake toxins, including disintegrins, are attracting more interest in the fields of medicine and biotechnology. Based on that, this study reports the isolation and structural characterization of a non-RGD disintegrin from Crotalus durissus collilineatus, as well as its cytotoxic effect and functional role in the migration of MDA-MD-231 human breast cancer cells, a highly metastatic cell line which is triple negative to progesterone and estrogen receptors [3030. Chavez KJ, Garimella SV, Lipkowitz S. Triple negative breast cancer cell lines: one tool in the search for better treatment of triple negative breast cancer. Breast Dis. 2010;32(1–2):35–48., 3131. Zhao F, Li L, Guan L, Yang H, Wu C, Liu Y. Roles for GP IIb/IIIa and αvβ3 integrins in MDA-MB-231 cell invasion and shear flow-induced cancer cell mechanotransduction. Cancer Lett. 2014;344(1):62–73.].
Methods
Snake venoms
Crotalus durissus collilineatus venom was provided by the Serpentarium at the School of Medicine of Ribeirão Preto, University of São Paulo, Brazil, accredited by Brazilian Institute of the Environment and Renewable Natural Resources (IBAMA), and registered under number 1506748, for scientific purposes. All animals were adult and crotamine-negative. The extracted venoms were dried at room temperature for 6 h in a vacuum desiccator and stored at – 20 °C until use.
Purification of disintegrin
Disintegrin from C. d. collilineatus venom was purified through two chromatographic steps carried out in a Fast Protein Liquid Chromatography (FPLC) system (Äkta Purifier UPC 900, GE Healthcare, Uppsala, Sweden). The venom (30 mg) was dispersed in 0.1% trifluoroacetic acid (TFA, solution A) and 1% formic acid, and centrifuged at 13,000 × g at 4 °C for 10 min. The supernatant was fractionated on a C18 column (250 × 10 mm, 5 μm particles, 300 Å, Phenomenex, Torrence, CA, USA) at a flow rate of 5 mL/min, using the concentration gradient described by Calvete et al. [3232. Calvete JJ, Juarez P, Sanz L. Snake venomics. Strategy and applications. J Mass Spectrom. 2007;42:1405–14.]. The second step was performed on another C18 column (250 × 4.6 mm, 3.6 μm particles, Phenomenex, Torrence, CA, USA) at a flow rate of 1 mL/min and the proteins were eluted using a segmented concentration gradient from 6.3 to 100% of solution B (80% acetonitrile, ACN, in 0.1% TFA). In both steps, the protein elution was monitored by absorbance at 214 nm. Fractions of interest were collected, frozen and lyophilized for further analysis.
Mass determination
The fractions of interest were analyzed by Tris-Tricine-SDS-PAGE (16.5%) [3333. Shagger H, von Jagow G. Tricine-SDS-PAGE for the separation of proteins in the 1–100 kDa range. Anal Biochem. 1987;168:368–79.] under reducing conditions. The molecular mass markers of 97.0-14.4 kDa (17—0446-01, GE Healthcare) and 26.6—1.06 kDa (M3546-1VL, Sigma-Aldrich, Saint Louis, MO, USA) were used. Proteins were stained with 0.2% Coomassie Brilliant Blue G-250 (Sigma).
Also, the accurate molecular mass was determined by matrix-assisted laser desorption/ionization (MALDI) with time of flight (TOF) analyzer and Smartbeam II laser, an ultrafleXtreme instrument with the software FlexControl, version 3.3 (Bruker Daltonics GmbH, Leipzig, Germany) for the acquisition of data. The parameters employed to obtain the data were 500 laser shots per spectrum, 1000 Hz laser frequency and the instrument operating in positive reflected mode, within a range of 5 to 50 kDa, according to the manufacturer's instructions. UltrafleXtreme instrument was calibrated using a mixture of peptides (Peptide calibration standard, NC9846988) and proteins (Protein calibration standard I, NC0239984, and Protein calibration standard II, NC0416074) from Bruker Daltonics. A saturated solution of a-cyano-4-hydroxycinnamic acid (α-CHCA) matrix was prepared in ACN and 0.1% TFA (V/V), at the ratio of 1:1 (V/V). Data analysis was performed by the software FlexAnalysis, version 3.3 (Bruker Daltonics GmbH, Leipzig, Germany).
Protein identification
For protein identification, the fraction of interest was submitted to N-terminal and MS/MS sequencings.
N-terminal sequencing was performed by the Edman degradation method [3434. Edman P, Begg G. A protein sequenator. Eur J Biochem. 1967;1(1):80–91.], using the automated protein sequencer model PPSQ-33A (Shimadzu, Kyoto, Japan), according to the manufacturer's instructions. The similarity of the amino acid sequences obtained in relation to sequences already deposited in databanks was evaluated by the Basic Local Alignment Search Tool (BLAST) [3535. Altschul SF, Gish W, Miller W, Myers EW, Lipman DJ. Basic local alignment search tool. J Mol Biol. 1990;215(3):403–10.].
The fraction of interest was reduced, alkylated, digested with sequencing grade porcine pancreatic trypsin and applied on a reversed phase C18 column (0.075 × 100 mm, 1.7 μm particles, 130 Å, Waters, Manchester, UK) for ultra-performance liquid chromatography (UPLC) coupled to electrospray (ESI) mass spectrometer, with quadrupole-time of flight (Q-TOF) analyzer (API-US, Waters, Manchester, UK). Data were interpreted with a licensed version of the MASCOT program against databank protein sequence deposited in the SwissProt (554,241 sequences, 198,410,167 amino acid residues) database and a databank of protein sequences filtered for snake venoms (27,207 sequences, 10,540,234 amino acid residues), generated from UniProt Knowledgebase (UniProtKB) [3636. The UniProt Consortium. UniProt: the universal protein knowledgebase. Nucleic Acids Res. 2017;45:D158–69.]. Precursor mass tolerance was 1.2 Da and MS/MS mass tolerance was set to ±0.8 Da, carbamidomethyl cysteine was set as fixed modification and oxidation of methionine as variable modification.
Functional assays
To verify whether the protein has cytotoxic activity and interferes with cell migration, two functional tests were carried out: cell viability assay by MTT and cell migration assay by wound healing in monoculture (MDA-MB-231). Human breast cancer cell line (MDA-MB-231), obtained from American Type Culture Collection (ATCC, Cat No. HTB-26), was cultured in Dulbecco's Modified Eagle's Medium (DMEM) medium supplemented with 4 mM L-glutamine, 10% fetal bovine serum and 1% antibiotics (streptomycin, gentamycin and neomycin). Cells were maintained under standard conditions at 37 °C, 5% CO2 and 95% humidity in a Forma Series II stove, Water Jacket CO2 Incubator (ThermoFisher Scientific, Waltham, Massachusetts, USA). All the experiments were conducted between the third and the eighth cell passage.
MDA-MB-231 cells were submitted to 3-[4, 5-dimethylthiazol-2-yl]-2, 5 diphenyl tetrazolium bromide (MTT) assay according to Mosmann [3737. Mosmann T. Rapid colorimetric assay for cellular growth and survival: application to proliferation and cytotoxicity assays. J Immunol Methods. 1983;65(1 –2):55–63.]. Initially, MDA-MB-231 cells were seeded in 96-well culture plates at the density of 1 × 104 cells per well. Subsequently, the plates were incubated at 37 °C in 5% CO2 for 24 h. After the incubation time, the cells were treated with the toxin at concentrations of 0.75; 1.50; 3.00; 6,00 μg/mL. Phosphate buffered saline (PBS) was used as negative control, and methyl methanesulfonate (MMS) as positive control (300 μM or 33,039 mg/L). After 24 h of treatment, 20 μL of MTT solution (5 mg/ mL) was diluted in PBS and added to each well and the plate was incubated for 3 h. After the incubation time, the plates were centrifuged for 5 min at 1027 × g, the supernatant removed and 200 μL of dimethyl sulfoxide (DMSO) added. Absorbance reading was done at 570 nm using a microplate reader (Biotek EL800 -Winooski, USA). The percentage of cell viability was obtained by the ratio between the absorbance of each treatment well and the absorbance of the wells of the negative control cultures, with cell viability considered 100%.
For the wound healing assay, 3.0 μg/mL of disintegrin was used, and the assay was performed according to Liang, Park and Guan [3838. Liang CC, Park AY, Guan JL. In vitro scratch assay: a convenient and inexpensive method for analysis of cell migration in vitro. J Immunol Methods. 1983;65:55–63.]. MDA-MB-231 cells (1.5 × 105 cells/well) were grown to 90% confluence on a 12-well plate. Then, with the aid of a sterile tip, a cicatrix was performed on the adherent monolayer of tumor cells. The culture medium was changed to remove the cell debris and a new culture medium added containing the lowest concentration (3.0 μg/mL) of dis-integrin which demonstrated effects on the cell line in the MTT assay and PBS as CN. Images of the wounds were recorded with a camera coupled to the inverted microscope at times 0, 4, 8 and 24 h of incubation. The mean distance of the internal area was determined as the percentage migration using the software AxionVision according to the following equation:
All the results were expressed as the mean ± standard deviation (SD). Data from three independent experiments (n = 3) were statistically analyzed using the software GraphPad Prism 5 (La Jolla, CA, USA). After assessing normality of variable distributions using the Kolmogorov-Smirnov test, experimental data were analyzed using one-way analysis of variance (ANOVA) followed by Dunnett's test. Statistical significance was considered at p < 0.05.
Results
Purification and identification of non-RGD disintegrin
Purification of disintegrin was performed in two steps, both on reversed phase C18 columns. The first step resulted in 22 fractions (Fig. 1a) and Fraction 2 was chosen for further analysis. In order to isolate the disintegrin, Fraction 2 was refractionated by reversed phase chromatography on a FPLC system with a segmented acetonitrile gradient represented by the dashed line in blue (Fig. 1b). The final chromatographic profile presented 10 fractions, with Fraction 6 being the major and most probable fraction where the disintegrin may have eluted, representing 0.43% of the total venom (Table 1).
Chromatographic profiles of non-RGD disintegrin from C. d. collilineatus venom using RP-FPLC system. a C. d. collilineatus venom (30 mg) was applied on a C18 column (250 × 10 mm, 5 μm particles, 300 Å), at a flow rate of 5 mL/min and (b) Fraction 2 (200 μg) on a C18 column (250×4.6 mm, 3.6 μm particles), at a flow rate of 0.5 mL/min. Elution in both chromatograms was carried out in a segmented concentration gradient from 6.3 to 100% of solution B (80% ACN in 0.1% TFA, represented by the blue dashed line) and absorbance was monitored at 214 nm. Inset panel - whole chromatographic profile without magnification
Protein recovery (%) during the purification procedure of disintegrin from Crotalus durissus collilineatus venom
The fractions of interest were analyzed by Tris-Tricine-SDS-PAGE (16.5%). The electrophoretic profile revealed that Fraction 2 exhibits a protein band of apparent 7 kDa molecular mass and some contaminants (Fig. 2a). After the second chromatographic step, it was possible to observe in Fraction 6 a single band of nearly 7 kDa corresponding to disintegrin. Thus, it was possible to separate disintegrin from its contaminants of approximately 14 kDa, which eluted in fractions 7 and 8. The molecular mass of the peptide present in Fraction 6 was determined by MALDI-TOF as 7287.402 Da (Fig. 2b).
Isolation profile of non-RGD disintegrin from C. d. collilineatus venom. a Tris-tricine-SDS-PAGE (16.5%), In non-reduced conditions and the gel was stained with 0.2% Coomassie Brilliant Blue G-250. MW1 - molecular mass (97.0-14.4 kDa); Cdc - C. d. collilineatus venom; 2 - Fraction 2 from RP-FPLC first step; 6-8 - fractions 6, 7 and 8, respectively, from RP-FPLC second step; MW2 - molecular mass (26.6-1.06 kDa). b Mass spectrum of Fraction 6 eluted from RP-FPLC second step obtained by MALDI-TOF (positive linear mode) using a-cyano-4-hydroxycinnamic acid (α-CHCA) matrix
The first 43 amino acid residues of the N-terminal region of the Fraction 6 were sequenced by Edman degradation and shared identity with others disintegrins (Fig. 3a). In addition, Fraction 6 was digested with trypsin and submitted to MS/MS sequencing. Data from obtained sequences are shown in Table 2.
Alignment and primary structure of disintegrins. a Sequence alignment between C. d. collilineatus (C0L2T8) and C. d. durissus (Q2QA03) disintegrins, peptides determined by mass spectrometry analysis (Fr6_MS/MS) and sequence obtained by Edman degradation (Fr6_Nterm) of Fraction 6. b Comparison between the classical RGD disintegrin structure pattern and the determined primary structure of Fraction 6 (LVN disintegrin). Bold - cysteines ©; Black box - consensus of all data sequence; Gray box - consensus of three data sequence; Red - pattern signature of disintegrin domain involving five conserved cysteines forming disulfide bonds; Green - RGD motif site; Blue - disulfide bond pattern of disintegrin structure; x - any amino acid residue
As to the in silico analysis, it was observed that these sequences shared similarity with the disintegrin domain (amino acid residues 397 to 478) of metalloproteases PII from C. d. collilineatus (C0L2T8) and C. d. durissus (Q2QA03), including the conservation of cysteine amino acid residues (Fig. 3a). Comparing the amino acid residues obtained from Fraction 6 with the primary sequences of both disintegrins, there was 76.8% coverage of the total sequence using Edman degradation and mass spectrometry procedures. In addition, these results show that the disintegrin of this study is a non-RGD disintegrin. The classic RGD motif, the conserved cysteine amino acid residues and the disulfide bond pattern commonly observed in disintegrins, as well as the determined sequence of Fraction 6 (LVN disintegrin) are shown in Fig. 3b for comparison purposes.
Functional assays with non-RGD disintegrin
Cell viability of MDA-MB-231 was determined in the presence of disintegrin; it was observed that the concentrations of 3 and 6 μg/mL of disintegrin significantly decreased cell viability in approximately 15% and 17%, respectively (Fig. 4a). Considering that disintegrin presented low yield in the purification steps (0.43%, Table 1) and that the two concentrations did not differ statistically (t test - data not shown), we chose to use the concentration of 3 μg/mL in the wound healing assay.
Functional assays with MDA-MB-231 cells. a Cell viability (%) after 24 h of treatment with disintegrin (0.75-6.00 μg/mL). C (-) - negative control(PBS); C (+) - positive control(MMS – 300 μM). The results were analyzed by ANOVA, followed by Dunett's post-hoc test (*p <0.05). b and c Cell migration after different times (0, 4, 8 and 24 h) of treatment with non-RGD disintegrin (3 μg/mL). C (-) - negative control (PBS). The dashed yellow lines delimit the region where no cell growth is observed. Data (n = 3) are presented as mean ± SD, which were analyzed by Student's t test (*p < 0.05)
The cell migration assay based on wound healing showed that disintegrin was able to significantly inhibit cell migration of MDA-MB-231 (24%, p < 0.05 compared to negative control), after 24 h of incubation (Fig. 4b and c).
Discussion
In the present study, we aimed to perform the isolation, structural and functional characterization of a non-RGD disintegrin from C. d. collilineatus venom, which had never before been described. Only two chromatographic steps were sufficient to isolate non-RGD disintegrin. The choice of the methodology was based on previous venomic studies that had reported the presence of disintegrin in this subspecies venoms [3939. Oliveira IS, Cardoso IA, KCF B, Carone SEI, Boldrini-França J, Pucca MB, et al. Global proteomic and functional analysis of Crotalus durissus collilineatus individual venom variation and its impact on envenoming. J Proteome. 2018., 4040. Boldrini-Franca J, Corrêa-Netto C, Silva MMS, Rodrigues RS, De La Torre P, Perez A, et al. Snake venomics and antivenomics of Crotalus durissus subspecies from Brazil: assessment of geographic variation and its implication on snakebite management. J Proteome. 2010;73(9):1758–76.].
Pure non-RGD disintegrin corresponds to 0.43% of soluble venom. This protein recovery is within the range of 0.4-0.5% of disintegrins in the venom of this subspecies determined by proteomic techniques [4040. Boldrini-Franca J, Corrêa-Netto C, Silva MMS, Rodrigues RS, De La Torre P, Perez A, et al. Snake venomics and antivenomics of Crotalus durissus subspecies from Brazil: assessment of geographic variation and its implication on snakebite management. J Proteome. 2010;73(9):1758–76.]. Due to low amounts of disintegrins in snake venoms [4040. Boldrini-Franca J, Corrêa-Netto C, Silva MMS, Rodrigues RS, De La Torre P, Perez A, et al. Snake venomics and antivenomics of Crotalus durissus subspecies from Brazil: assessment of geographic variation and its implication on snakebite management. J Proteome. 2010;73(9):1758–76., 4141. Nicolau CA, Carvalho PC, Junqueira-de-Azevedo IL, Teixeira-Ferreira A, Junqueira M, Perales J, et al. An in-depth snake venom proteopeptidome characterization: benchmarking Bothrops jararaca. J Proteome. 2017;151: 214–31.], is necessary to produce recombinant disintegrins as similar to contortrostatin [4242. Zhou Q, Hu P, Ritter MR, Swenson SD, Argounova S, Epstein AL, et al. Molecular cloning and functional expression of contortrostatin, a homodimeric disintegrin from southern copperhead snake venom. Arch Biochem Biophys. 2000;375(2):278-88.], r-colombistatins 2, 3, and 4 [4343. Suntravat M, Helmke TJ, Atphaisit C, Cuevas E, Lucena SE, Uzcátegui NL, et al. Expression, purification, and analysis of three recombinant ECD disintegrins (r-colombistatins) from P-III class snake venom metalloproteinases affecting platelet aggregation and SK-MEL-28 cell adhesion. Toxicon. 2016;122:43-9.] and r-Cam-dis [4444. Suntravat M, Barret HS, Jurica CA, Lucena SE, Perez JC, Sánchez EE. Recombinant disintegrin (r-cam-dis) from Crotalus adamanteus inhibits adhesion of human pancreatic cancer cell lines to laminin-1 and vitronectin. J Venom Res. 2015;6:1-10.], among others.
Non-RGD disintegrin from C. d. collilineatus presents 7287.4 Da, as determined by MALDI-TOF, and it is similar to the molecular mass of others snake venom disintegrins, such as tzabcanin (7.1 kDa) [4545. Saviola AJ, Modahl CM, Mackessy SP. Disintegrins of Crotalus simus tzabcan venom: isolation, characterization and evaluation of the cytotoxic and antiadhesion activities of tzabcanin, a new RGD disintegrin. Biochimie. 2015;116: 92-102.], disintegrin from C. simus (7.1 kDa) [4646. Angulo Y, Castro A, Lomonte B, Rucavado A, Fernández J, Calvete JJ, et al. Isolation and characterization of four medium-size disintegrins from the venoms of central American viperid snakes of the genera Atropoides, Bothrops, Cerrophidion and Crotalus. Biochimie. 2014;107(Pt B):376-84.] and proteomic data of C. d. collilineatus [3939. Oliveira IS, Cardoso IA, KCF B, Carone SEI, Boldrini-França J, Pucca MB, et al. Global proteomic and functional analysis of Crotalus durissus collilineatus individual venom variation and its impact on envenoming. J Proteome. 2018., 4040. Boldrini-Franca J, Corrêa-Netto C, Silva MMS, Rodrigues RS, De La Torre P, Perez A, et al. Snake venomics and antivenomics of Crotalus durissus subspecies from Brazil: assessment of geographic variation and its implication on snakebite management. J Proteome. 2010;73(9):1758–76.].
As to the primary sequence obtained through Edman degradation and mass spectrometry procedures, Cdc non-RGD disintegrin isolated in this study is absent from the classical RGD motif or any other motif previously observed in this protein family or glutamate- cysteine-aspartate (ECD) motif which characterize disintegrin-like proteins that may inhibit tumor progression [4747. Moritz MNO, Eustáquio LMS, Micocci KC, Nunes ACC, Dos Santos PK, de Castro Vieira T, et al. Alternagin-C binding to α2β1 integrin controls matrix metalloprotease-9 and matrix metalloprotease-2 in breast tumor cells and endothelial cells. J Venom Anim Toxins incl Trop Dis. 2018;24:13. https://doi.org/10.1186/s40409-018-0150-2.
https://doi.org/10.1186/s40409-018-0150-...
]. In the same position of this domain, this toxin presents a triad of amino acids LVN, which was found in disintegrins of C. d. collilineatus by transcriptome techniques [4848. Boldrini-França J, Rodrigues RS, Fonseca FP, Menaldo DL, Ferreira FB, Henrique- Silva F, et al. Crotalus durissus collilineatus venom gland transcriptome: analysis of gene expression profile. Biochimie. 2009;91(5):586-95.], as well as in the disintegrin domains of P-II SVMP of C. d. collilineatus (C0L2T8) and C. atrox (Q2QA03). On the other hand, these disintegrins, as well as that of our study, present the disulfide bond pattern of this protein family, another signature that characterizes disintegrins. This pattern of disulfide bonds has already been well reported and is closely related to the formation of the protein loop and activity. If disintegrins are reduced and alkylated their biological activity is decreased [4949. Calvete JJ, Schäfer W, Soszka T, Lu WQ, Cook JJ, Jameson BA, et al. Identification of the disulfide bond pattern in albolabrin, an RGD-containing peptide from the venom of Trimeresurus albolabris: significance for the expression of platelet aggregation inhibitory activity. Biochemistry. 1991; 30(21):5225-9.
50. Huang TF, Holt JC, Kirby EP, Niewiarowski S. Trigramin: primary structure and its inhibition of von Willebrand factor binding to glycoprotein IIb/IIIa complex on human platelets. Biochemistry. 1989;28(2):661-6.
51. Knudsen KA, Tuszynski GP, Huang TF, Niewiarowski S. Trigramin, an RGD-containing peptide from snake venom, inhibits cell-substratum adhesion of human melanoma cells. Exp Cell Res. 1988;179(1):42-9.
52. Saudek V, Atkinson RA, Lepage P, Pelton JT. The secondary structure of echistatin from 1H-NMR, circular-dichroism and Raman spectroscopy. Eur J Biochem. 1991;202(2):329-38.-5353. Calvete JJ, Wang Y, Mann K, Schäfer W, Niewiarowski S, Stewart GJ. The disulfide bridge pattern of snake venom disintegrins, flavoridin and echistatin. FEBS Lett. 1992;309(3):316-20.].
Disintegrins are known to be potent inhibitors of platelet aggregation, and some drugs based on its structure were developed and approved by the FDA [5454. Chan YS, Cheung RCF, Xia L, Wong JH, Ng TB, Chan WY. Snake venom toxins: toxicity and medicinal applications. Appl Microbiol Biotechnol. 2016; 100(14):6165-81.], such as Eptifibatide [1919. O'Shea JC, Tcheng JE. Eptifibatide: a potent inhibitor of the platelet receptor integrin glycoprotein IIb/IIIa. Expert Opin Pharmacother. 2002;3(8):1199–210.] and Tirofiban [2020. Menozzi A, Merlini PA, Ardissino D. Tirofiban in acute coronary syndromes. Expert Rev Cardiovasc Ther. 2005;3(2):193–206.]. The main mechanism for such inhibition is that the disintegrins bind to the αΠbβ3 platelet integrins, preventing their binding to fibrinogen and consequently inhibiting platelet aggregation [33. Huang TF, Holt JC, Lukasiewicz H, Niewiarowski S. Trigramin. A low molecular weight peptide inhibiting fibrinogen interaction with platelet receptors expressed on glycoprotein IIb-IIIa complex. J Biol Chem. 1987; 262(33):16157-63.]. Knowing that the integrins of platelets (αΠbβ3) and breast cancer cells (αvβ3) are similar, disintegrins are considered candidates to be anticancer agents [22. Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9.]. Integrins are transmembrane proteins, that are part of cell adhesion molecules (CAM) group, and are formed by two subunits, α, of approximately 120 to 180 kDa, and β, of approximately 90 to 110 kDa, non-covalently linked [5555. Ferraz FB, Fernandez JF. Integrinas na adesão, migração e sinalização celular: associação com patologias e estudos clínicos. Revista Científica da FMC. 2014;9(2):25-34 http://www.fmc.br/revista/V9N2P25-34.pdf.
http://www.fmc.br/revista/V9N2P25-34.pdf...
]. They are able to perform the cell-cell and cell-ECM interactions [5656. Hou S, Isaji T, Hang Q, Im S, Fukuda T, Gu J. Distinct effects of β1 integrin on cell proliferation and cellular signaling in MDA-MB-231 breast cancer cells. Sci Rep. 2016;6:18430.], and are essential for the development of tumor cells [5757. Jin H, Varner J. Integrins: roles in cancer development and as treatment targets. Br J Cancer. 2004;90(3):561-5.].
Since disintegrins are considered candidates to be agents of anticancer therapy, we performed cytotoxicity and cell migration assays on metastatic breast cancer cells, namely MDA-MB-231 cells. This cell line is able to express low levels of the subunits α2 and β5 and moderate levels of αv α3 and β1 integrins [5858. Gui GP, Puddefoot JR, Vinson GP, Wells CA, Carpenter R. In vitro regulation of human breast cancer cell adhesion and invasion via integrin receptors to the extracellular matrix. Br J Surg. 1995;82(9):1192-6.]. Taherian et al. demonstrated that MDA-MB-231 cells express higher levels of β5 and αvβ5 integrins when compared with non-breast cancer cell line (Hek-293) [5959. Taherian A, Li X, Liu Y, Haas TA. Differences in integrin expression and signaling within human breast cancer cells. BMC Cancer. 2011;11:293.]. Our results show that non-RGD disintegrin from C. d. colilineatus venom presents low cytotoxicity, although its toxicity increases with the concentration, having a dose-response effect. As in our results, the tzabcanin also showed dose-dependent toxicity against human malignant melanoma (A-357) and human colorectal adenocarcinoma (Colo-205) cell lines, but the viabilities of human breast adenocarcinoma (MCF-7) and human lung adenocarcinoma (A-549) cell lines were not affected [4545. Saviola AJ, Modahl CM, Mackessy SP. Disintegrins of Crotalus simus tzabcan venom: isolation, characterization and evaluation of the cytotoxic and antiadhesion activities of tzabcanin, a new RGD disintegrin. Biochimie. 2015;116: 92-102., 6060. Saviola AJ, Burns PD, Mukherjee AK, Mackessy SP. The disintegrin tzabcanin inhibits adhesion and migration in melanoma and lung cancer cells. Int J Biol Macromol. 2016;88:457-64.]. Lebein inhibited the viability of human colon adenocarcinoma (HT29, LS174 and HCT116) and melanoma (SK-MEL-28 and LU-1205) cell lines [2828. Zakraoui O, Marcinkiewicz C, Aloui Z, Othman H, Grépin R, Haoues M, et al. Lebein, a snake venom disintegrin, suppresses human colon cancer cells proliferation and tumor-induced angiogenesis through cell cycle arrest, apoptosis induction and inhibition of VEGF expression. Mol Carcinog. 2017; 56(1):18–35., 6161. Hammouda MB, Montenegro MF, Sánchez-del-Campo L, Zakraoui O, Aloui Z, Riahi-Chebbi I, et al. Lebein, a snake venom disintegrin, induces apoptosis in human melanoma cells. Toxins (Basel). 2016;8(7):1-14.].
The cell migration assay showed that Cdc non-RGD disintegrin was able to inhibit the migration of MDA-MB-231 cells after 24 h of incubation, demonstrating that it is a possible anticancer agent with potential to inhibit the formation of breast cancer tumors. Similar results were obtained from tzabcanin, which inhibited cell migration of A-375 and A-549 cell lines [6060. Saviola AJ, Burns PD, Mukherjee AK, Mackessy SP. The disintegrin tzabcanin inhibits adhesion and migration in melanoma and lung cancer cells. Int J Biol Macromol. 2016;88:457-64.], r-Viridistatin 2, from Crotalus viridis viridis, and r-mojastin 1, from Crotalus scutulatus scutulatus, that inhibited the migration of human pancreatic adenocarcinoma cancer cells (BXPC-3) [6262. Lucena S, Castro R, Lundin C, Hofstetter A, Alaniz A, Suntravat M, et al. Inhibition of pancreatic tumoral cells by snake venom disintegrins. Toxicon. 2015;93:136-43.].
In addition, considering the potential of disintegrins as anticancer therapeutic agents, they can also be used in combination with known chemotherapeutics. For example, echistatin combined with cisplatin (CDDP) was capable of increasing the expression of nuclear factor kappa B (NFκB), caspase-9 and caspase-3, leading to increased apoptosis in MDA-MB-231 cells. These data suggest that the combination of this disintegrin with CDDP may serve as a new type of anticancer therapy [6363. Czarnomysy R, Surażyński A, Popławska B, Rysiak E, Pawlowska N, Czajkowska A, et al. Synergistic action of cisplatin and echistatin in MDA- MB-231 breast cancer cells. Mol Cell Biochem. 2017;427(1):13-22.].
Conclusion
In this study, we described the isolation and characterization of the first disintegrin with an LVN motif from C. d. collilineatus venom. The studies performed on the human breast cancer MDA-MB-231 cell line demonstrate that this disintegrin is able to inhibit cell migration, without severely affecting cell viability. Therefore, it may be a very useful molecular tool for understanding ECM-cell interaction cancer-related mechanisms involved important family of integrin that would elucidate molecular aspects of tumorigenesis. Also, this non-RGD disintegrin has potential to serve as an agent in anticancer therapy or adjuvant component combined with other anti-cancer drugs.
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FundingFinancial support is from the Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP, São Paulo Research Foundation, grant n. 2011/23236-4, 2012/14996-8, 2015/18432 and scholarships to ISO n. 2017/03580-9 and RVM n. 2016/11578-1) and Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES, Coordination for the Improvement of Higher Education Personnel, Finance Code 001, scholarships to ARTM and IGF). Also, this work was supported in part by CAPES through Programa Editoração CAPES (edital n. 13/2016, auxílio n. 0722/2017, process n. 88881.142062/2017-01) and by Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq, The National Council for Scientific and Technological Development) through Programa Editorial CNPq/CAPES (chamada n. 26/2017, process n. 440954/201 7-7).
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Ethics approval and consent to participateNot applicable.
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Consent for publicationNot applicable.
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Publisher's NoteSpringer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
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Abbreviations
- ACN Acetonitrile
- ADP Adenosine diphosphate
- ANOVA Analysis of variance
- ATCC American Type Culture Collection
- BLAST Basic Local Alignment Search Tool
- CAM Cell adhesion molecules
- CDDP Cisplatin
- DMEM Dulbecco's Modified Eagle's Medium
- DMSO Dimethyl sulfoxide
- ECD Glutamate-cysteine-aspartate
- ECM Extracellular matrix
- ESI Electrospray
- FDA Food and Drug Administration
- FPLC Fast Protein Liquid Chromatography
- IBAMA Brazilian Institute of the Environment and Renewable Natural Resources
- KGD Lysine-glycine-aspartic acid
- LVN Leucine-valine-asparagine
- MALDI Matrix-assisted laser desorption/ionization
- MDC Metalloprotease/disintegrin/cysteine-rich
- MGD Methionine-glycine-aspartic acid
- MLD Methionine-leucine-aspartic acid
- MMS Methyl methanesulfonate
- MS/MS Tandem mass spectrometry
- MTT 3-[4, 5-dimethylthiazol-2-yl]-2, 5 diphenyl tetrazolium bromide
- MVD Methionine-valine-aspartic acid
- PBS Phosphate buffered saline
- Q-TOF quadrupole-time of flight
- RGD Arginine-glycine-aspartic acid
- SDS-PAGE Sodium dodecyl sulfate polyacrylamide gel electrophoresis
- SVMP Snake venom metalloproteases
- TFA Trifluoroacetic acid
- TOF Time of flight
- UPLC Ultra-performance liquid chromatography
- VGD Valine-glycine-aspartic acid
- WGD Tryptophan-glycine-aspartic acid
- α-CHCA α-cyano-4-hydroxycinnamic acid
References
-
1Kini RM, Evans HJ. Structural domains in venom proteins: evidence that metalloproteinases and nonenzymatic platelet aggregation inhibitors (disintegrins) from snake venoms are derived by proteolysis from a common precursor. Toxicon. 1992;30(3):265–93.
-
2Calvete JJ. The continuing saga of snake venom disintegrins. Toxicon. 2013; 62:40-9.
-
3Huang TF, Holt JC, Lukasiewicz H, Niewiarowski S. Trigramin. A low molecular weight peptide inhibiting fibrinogen interaction with platelet receptors expressed on glycoprotein IIb-IIIa complex. J Biol Chem. 1987; 262(33):16157-63.
-
4Gould RJ, Polokoff MA, Friedman PA, Huang TF, Holt JC, Cook JJ, et al. Disintegrins: a family of integrin inhibitory proteins from viper venoms. Proc Soc Exp Biol Med. 1990;195(2):168-71.
-
5Selistre-de-Araujo HS, Pontes CLS, Montenegro CF, Martin ACBM. Snake venom disintegrins and cell migration. Toxins (Basel). 2010;2(11):2606–21.
-
6Sanchez EF, Flores-Ortiz RJ, Alvarenga VG, Eble JA. Direct fibrinolytic snake venom metalloproteinases affecting hemostasis: structural, biochemical features and therapeutic potential. Toxins (Basel). 2017;9:12.
-
7Calvete JJ, Jürgens M, Marcinkiewicz C, Romero A, Schrader M, Niewiarowski S. Disulphide-bond pattern and molecular modelling of the dimeric disintegrin EMF-10, a potent and selective integrin α5β1 antagonist from Eristocophis macmahoni venom. Biochem J. 2000;345(3):573-81.
-
8Bilgrami S, Yadav S, Kaur P, Sharma S, Perbandt M, Betzel C, et al. Crystal structure of the disintegrin heterodimer from saw-scaled viper (Echis carinatus) at 1.9 a resolution. Biochemistry. 2005;44(33):11058-66.
-
9Bilgrami S, Tomar S, Yadav S, Kaur P, Kumar J, Jabeen T, et al. Crystal structure of schistatin, a disintegrin homodimer from saw-scaled viper (Echis carinatus) at 2.5 a resolution. J Mol Biol. 2004;341(3):829-37.
-
10Calvete JJ, Moreno-Murciano MP, Theakston RD, Kisiel DG, Marcinkiewicz C. Snake venom disintegrins: novel dimeric disintegrins and structural diversification by disulphide bond engineering. Biochem J. 2003;372(Pt 3): 725-34.
-
11Juárez P, Comas I, González-Candelas F, Calvete JJ. Evolution of snake venom disintegrins by positive Darwinian selection. Mol Biol Evol. 2008; 25(11):2391–407.
-
12Sanz L, Bazaa A, Marrakchi N, Pérez A, Chenik M, Bel Lasfer Z, et al. Molecular cloning of disintegrins from Cerastes vipera and Macrovipera lebetina transmediterranea venom gland cDNA libraries: insight into the evolution of the snake venom integrin-inhibition system. Biochem J. 2006; 395(2):385–92.
-
13Calvete JJ, Juárez P, Sanz L. Snake venomics and disintegrins: portrait and evolution of a family of snake venom integrin antagonists. In: Mackessy SP, editor. Handbook of venoms and toxins of reptiles. Boca Ratón: CRC Press, Taylor & Francis; 2009. p. 337–57.
-
14Calvete JJ. Brief history and molecular determinants of snake venom disintegrin evolution. In: Kini RM, Markland F, McLane MA, Morita T, editors. Toxins and hemostasis: from bench to bedside. Amsterdam: Springer; 2010. p. 285–300.
-
15Oshikawa K, Terada S. Ussuristatin 2, a novel KGD-bearing disintegrin from Agkistrodon ussuriensis venom. J Biochem. 1999;125(1):31–5.
-
16Scarborough RM, Rose JW, Hsu MA, Phillips DR, Fried VA, Campbell AM, et al. Barbourin. A GPIIb-IIIa-specific integrin antagonist from the venom of Sistrurus m. barbouri. J Biol Chem. 1991;266(15):9359–62.
-
17Hite LA, Shannon JD, Bjarnason JB, Fox JW. Sequence of a cDNA clone encoding the zinc metalloproteinase hemorrhagic toxin e from Crotalus atrox: evidence for signal, zymogen, and disintegrin-like structures. Biochemistry. 1992;31(27):6203–11.
-
18King GF. Venoms as a platform for human drugs: translating toxins into therapeutics. Expert Opin Biol Ther. 2011;11(11):1469–84.
-
19O'Shea JC, Tcheng JE. Eptifibatide: a potent inhibitor of the platelet receptor integrin glycoprotein IIb/IIIa. Expert Opin Pharmacother. 2002;3(8):1199–210.
-
20Menozzi A, Merlini PA, Ardissino D. Tirofiban in acute coronary syndromes. Expert Rev Cardiovasc Ther. 2005;3(2):193–206.
-
21Arruda Macêdo JK, Fox JW, de Souza Castro M. Disintegrins from snake venoms and their applications in cancer research and therapy. Curr Protein Pept Sci. 2015;16(6):532–48.
-
22Zhou Q, Sherwin RP, Parrish C, Richters V, Groshen SG, Tsao-Wei D, et al. Contortrostatin, a dimeric disintegrin from Agkistrodon contortrix contortrix, inhibits breast cancer progression. Breast Cancer Res Treat. 2000;61(3):249–60.
-
23Kim KS, Kim DS, Chung KH, Park YS. Inhibition of angiogenesis and tumor progression by hydrodynamic cotransfection of angiostatin K1-3, endostatin, and saxatilin genes. Cancer Gene Ther. 2006;13(6):563–71.
-
24Higuchi DA, Almeida MC, Barros CC, Sanchez EF, Pesquero PR, Lang EA, et al. Leucurogin, a new recombinant disintegrin cloned from Bothrops leucurus (white-tailed-jararaca) with potent activity upon platelet aggregation and tumor growth. Toxicon. 2011;58(1):123–9.
-
25Wang JH, Wu Y, Ren F, Lü L, Zhao BC. Cloning and characterization of Adinbitor, a novel disintegrin from the snake venom of Agkistrodon halys brevicaudus stejneger. Acta Biochim Biophys Sin Shanghai. 2004;36(6):425–9.
-
26Tian J, Paquette-Straub C, Sage EH, Funk SE, Patel V, Galileo D, et al. Inhibition of melanoma cell motility by the snake venom disintegrin eristostatin. Toxicon. 2007;49(7):899–908.
-
27Galán JA, Sánchez EE, Rodríguez-Acosta A, Soto JG, Bashir S, McLane MA, et al. Inhibition of lung tumor colonization and cell migration with the disintegrin crotatroxin 2 isolated from the venom of Crotalus atrox. Toxicon. 2008;51(7):1186–96.
-
28Zakraoui O, Marcinkiewicz C, Aloui Z, Othman H, Grépin R, Haoues M, et al. Lebein, a snake venom disintegrin, suppresses human colon cancer cells proliferation and tumor-induced angiogenesis through cell cycle arrest, apoptosis induction and inhibition of VEGF expression. Mol Carcinog. 2017; 56(1):18–35.
-
29Desgrosellier JS, Cheresh DA. Integrins in cancer: biological implications and therapeutic opportunities. Nat Rev Cancer. 2010;10(1):9–22.
-
30Chavez KJ, Garimella SV, Lipkowitz S. Triple negative breast cancer cell lines: one tool in the search for better treatment of triple negative breast cancer. Breast Dis. 2010;32(1–2):35–48.
-
31Zhao F, Li L, Guan L, Yang H, Wu C, Liu Y. Roles for GP IIb/IIIa and αvβ3 integrins in MDA-MB-231 cell invasion and shear flow-induced cancer cell mechanotransduction. Cancer Lett. 2014;344(1):62–73.
-
32Calvete JJ, Juarez P, Sanz L. Snake venomics. Strategy and applications. J Mass Spectrom. 2007;42:1405–14.
-
33Shagger H, von Jagow G. Tricine-SDS-PAGE for the separation of proteins in the 1–100 kDa range. Anal Biochem. 1987;168:368–79.
-
34Edman P, Begg G. A protein sequenator. Eur J Biochem. 1967;1(1):80–91.
-
35Altschul SF, Gish W, Miller W, Myers EW, Lipman DJ. Basic local alignment search tool. J Mol Biol. 1990;215(3):403–10.
-
36The UniProt Consortium. UniProt: the universal protein knowledgebase. Nucleic Acids Res. 2017;45:D158–69.
-
37Mosmann T. Rapid colorimetric assay for cellular growth and survival: application to proliferation and cytotoxicity assays. J Immunol Methods. 1983;65(1 –2):55–63.
-
38Liang CC, Park AY, Guan JL. In vitro scratch assay: a convenient and inexpensive method for analysis of cell migration in vitro. J Immunol Methods. 1983;65:55–63.
-
39Oliveira IS, Cardoso IA, KCF B, Carone SEI, Boldrini-França J, Pucca MB, et al. Global proteomic and functional analysis of Crotalus durissus collilineatus individual venom variation and its impact on envenoming. J Proteome. 2018.
-
40Boldrini-Franca J, Corrêa-Netto C, Silva MMS, Rodrigues RS, De La Torre P, Perez A, et al. Snake venomics and antivenomics of Crotalus durissus subspecies from Brazil: assessment of geographic variation and its implication on snakebite management. J Proteome. 2010;73(9):1758–76.
-
41Nicolau CA, Carvalho PC, Junqueira-de-Azevedo IL, Teixeira-Ferreira A, Junqueira M, Perales J, et al. An in-depth snake venom proteopeptidome characterization: benchmarking Bothrops jararaca. J Proteome. 2017;151: 214–31.
-
42Zhou Q, Hu P, Ritter MR, Swenson SD, Argounova S, Epstein AL, et al. Molecular cloning and functional expression of contortrostatin, a homodimeric disintegrin from southern copperhead snake venom. Arch Biochem Biophys. 2000;375(2):278-88.
-
43Suntravat M, Helmke TJ, Atphaisit C, Cuevas E, Lucena SE, Uzcátegui NL, et al. Expression, purification, and analysis of three recombinant ECD disintegrins (r-colombistatins) from P-III class snake venom metalloproteinases affecting platelet aggregation and SK-MEL-28 cell adhesion. Toxicon. 2016;122:43-9.
-
44Suntravat M, Barret HS, Jurica CA, Lucena SE, Perez JC, Sánchez EE. Recombinant disintegrin (r-cam-dis) from Crotalus adamanteus inhibits adhesion of human pancreatic cancer cell lines to laminin-1 and vitronectin. J Venom Res. 2015;6:1-10.
-
45Saviola AJ, Modahl CM, Mackessy SP. Disintegrins of Crotalus simus tzabcan venom: isolation, characterization and evaluation of the cytotoxic and antiadhesion activities of tzabcanin, a new RGD disintegrin. Biochimie. 2015;116: 92-102.
-
46Angulo Y, Castro A, Lomonte B, Rucavado A, Fernández J, Calvete JJ, et al. Isolation and characterization of four medium-size disintegrins from the venoms of central American viperid snakes of the genera Atropoides, Bothrops, Cerrophidion and Crotalus. Biochimie. 2014;107(Pt B):376-84.
-
47Moritz MNO, Eustáquio LMS, Micocci KC, Nunes ACC, Dos Santos PK, de Castro Vieira T, et al. Alternagin-C binding to α2β1 integrin controls matrix metalloprotease-9 and matrix metalloprotease-2 in breast tumor cells and endothelial cells. J Venom Anim Toxins incl Trop Dis. 2018;24:13. https://doi.org/10.1186/s40409-018-0150-2
» https://doi.org/10.1186/s40409-018-0150-2 -
48Boldrini-França J, Rodrigues RS, Fonseca FP, Menaldo DL, Ferreira FB, Henrique- Silva F, et al. Crotalus durissus collilineatus venom gland transcriptome: analysis of gene expression profile. Biochimie. 2009;91(5):586-95.
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49Calvete JJ, Schäfer W, Soszka T, Lu WQ, Cook JJ, Jameson BA, et al. Identification of the disulfide bond pattern in albolabrin, an RGD-containing peptide from the venom of Trimeresurus albolabris: significance for the expression of platelet aggregation inhibitory activity. Biochemistry. 1991; 30(21):5225-9.
-
50Huang TF, Holt JC, Kirby EP, Niewiarowski S. Trigramin: primary structure and its inhibition of von Willebrand factor binding to glycoprotein IIb/IIIa complex on human platelets. Biochemistry. 1989;28(2):661-6.
-
51Knudsen KA, Tuszynski GP, Huang TF, Niewiarowski S. Trigramin, an RGD-containing peptide from snake venom, inhibits cell-substratum adhesion of human melanoma cells. Exp Cell Res. 1988;179(1):42-9.
-
52Saudek V, Atkinson RA, Lepage P, Pelton JT. The secondary structure of echistatin from 1H-NMR, circular-dichroism and Raman spectroscopy. Eur J Biochem. 1991;202(2):329-38.
-
53Calvete JJ, Wang Y, Mann K, Schäfer W, Niewiarowski S, Stewart GJ. The disulfide bridge pattern of snake venom disintegrins, flavoridin and echistatin. FEBS Lett. 1992;309(3):316-20.
-
54Chan YS, Cheung RCF, Xia L, Wong JH, Ng TB, Chan WY. Snake venom toxins: toxicity and medicinal applications. Appl Microbiol Biotechnol. 2016; 100(14):6165-81.
-
55Ferraz FB, Fernandez JF. Integrinas na adesão, migração e sinalização celular: associação com patologias e estudos clínicos. Revista Científica da FMC. 2014;9(2):25-34 http://www.fmc.br/revista/V9N2P25-34.pdf
» http://www.fmc.br/revista/V9N2P25-34.pdf -
56Hou S, Isaji T, Hang Q, Im S, Fukuda T, Gu J. Distinct effects of β1 integrin on cell proliferation and cellular signaling in MDA-MB-231 breast cancer cells. Sci Rep. 2016;6:18430.
-
57Jin H, Varner J. Integrins: roles in cancer development and as treatment targets. Br J Cancer. 2004;90(3):561-5.
-
58Gui GP, Puddefoot JR, Vinson GP, Wells CA, Carpenter R. In vitro regulation of human breast cancer cell adhesion and invasion via integrin receptors to the extracellular matrix. Br J Surg. 1995;82(9):1192-6.
-
59Taherian A, Li X, Liu Y, Haas TA. Differences in integrin expression and signaling within human breast cancer cells. BMC Cancer. 2011;11:293.
-
60Saviola AJ, Burns PD, Mukherjee AK, Mackessy SP. The disintegrin tzabcanin inhibits adhesion and migration in melanoma and lung cancer cells. Int J Biol Macromol. 2016;88:457-64.
-
61Hammouda MB, Montenegro MF, Sánchez-del-Campo L, Zakraoui O, Aloui Z, Riahi-Chebbi I, et al. Lebein, a snake venom disintegrin, induces apoptosis in human melanoma cells. Toxins (Basel). 2016;8(7):1-14.
-
62Lucena S, Castro R, Lundin C, Hofstetter A, Alaniz A, Suntravat M, et al. Inhibition of pancreatic tumoral cells by snake venom disintegrins. Toxicon. 2015;93:136-43.
-
63Czarnomysy R, Surażyński A, Popławska B, Rysiak E, Pawlowska N, Czajkowska A, et al. Synergistic action of cisplatin and echistatin in MDA- MB-231 breast cancer cells. Mol Cell Biochem. 2017;427(1):13-22.
Publication Dates
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Publication in this collection
29 Nov 2018 -
Date of issue
2018
History
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Received
06 July 2018 -
Accepted
05 Oct 2018 -
Published
20 Oct 2018