S- and P-type cobra venom cardiotoxins differ in their action on isolated rat heart

Averin, Alexey S.; Goltyaev, Mikhail V.; Andreeva, Tatyana V.; Starkov, Vladislav G.; Tsetlin, Victor I.; Utkin, Yuri N.

doi:10.1590/1678-9199-JVATITD-2021-0110

Abstract

Background:

The cardiovascular system is one of the first systems to be affected by snake toxins; but not many toxins exert a direct effect on the heart. Cobra venom cardiotoxins are among those few toxins that attack the heart. Although the two cardiotoxin types (S and P) differ in their central-loop structure, it is not known whether they differ in their effect on the mammalian heart. We compared the effects of S- and P-type cardiotoxins, CTХ-1 and CTХ-2, respectively, from the cobra Naja oxiana, on the isolated rat heart.

Methods:

An isolated rat heart perfused according to the Langendorff technique was used in this study to investigate the activity of cardiotoxins CTX-1 and CTX-2. The following parameters were registered: the left ventricular developed pressure, calculated as the difference between systolic and diastolic pressure in the left ventricle, the end-diastolic pressure, the heart rate, time to maximal end-diastolic pressure (heart contracture), and time to depression of the heart contraction.

Results:

Both cardiotoxins at the concentration of 5 μg/mL initially produce a slight increase in systolic intraventricular pressure, followed by its rapid decrease with a simultaneous increase in diastolic intraventricular pressure until reaching contracture. CTX-2 blocks cardiac contractions faster than CTX-1; in its presence the maximum diastolic pressure is reached faster and the magnitude of the developed contracture is higher.

Conclusion:

The P-type cardiotoxin CTX-2 more strongly impairs rat heart functional activity than the S-type cardiotoxin CTX-1, as expressed in its faster blockage of cardiac contractions as well as in more rapid development and greater magnitude of contracture in its presence.

Keywords:
Cardiotoxin; Cobra venom; Contraction; Contracture; Myocardium; Perfused rat heart; Ventricular pressure

Background

Among the vast family of three-finger snake venom toxins, there is a group of proteins called cardiotoxins (CaTXs) or cytotoxins that exert damaging effects on the heart. In particular, CaTXs cause systolic heart arrest and induce a membrane leakage of cardiomyocytes. They are β-structured proteins consisting of 59 to 61 amino-acid residues with the structure stabilized by four disulfide bonds. This group of toxins is characterized by direct interaction with the membrane, leading to membrane depolarization and cell death (see reviews [11. Dubovskii PV, Konshina AG, Efremov RG. Cobra cardiotoxins: membrane interactions and pharmacological potential. Curr Med Chem. 2014;21(3):270-87., 22. Dubovskii PV, Utkin YN. Antiproliferative activity of cobra venom cytotoxins. Curr Top Med Chem. 2015;15(7):638-48.]).

CaTXs are classified into two types, P and S: P-type includes CaTXs with a proline residue at position 30 of the amino-acid sequences and alanine at position 28 in most sequences, while S-type toxins have a serine residue at position 28 (Figure 1) and never contain proline at position 30, which is usually occupied by leucine, lysine or serine residues. The data available to date indicate that toxins of both types destabilize the lipid bilayer of anionic phospholipid-containing membranes, but with different efficiencies [33. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Konshina AG, Utkin YN, Efremov RG, Arseniev AS. Interaction of three-finger toxins with phospholipid membranes: comparison of S- and P-type cytotoxins. Biochem J. 2005 May 1;387(Pt 3):807-15.]; P-type toxins damage the lipid bilayer more severely.

The effects of various CaTXs on myocardial tissue develop quite typically: the initial increase in contractility is followed by its suppression and by an increase in diastolic tension [44. Harvey AL, Marshall RJ, Karlsson E. Effects of purified cardiotoxins from the Thailand cobra (Naja naja siamensis) on isolated skeletal and cardiac muscle preparations. Toxicon. 1982;20(2):379-96. , 55. Sun JJ, Walker MJ. Actions of cardiotoxins from the southern Chinese cobra (Naja naja atra) on rat cardiac tissue. Toxicon. 1986;24(3):233-45.]. At the same time, there are CaTXs that, at fairly high concentrations of tens of μM, produce an increase in the contraction force without the contracture development [44. Harvey AL, Marshall RJ, Karlsson E. Effects of purified cardiotoxins from the Thailand cobra (Naja naja siamensis) on isolated skeletal and cardiac muscle preparations. Toxicon. 1982;20(2):379-96. ]. It should be noted that CaTXs affect the blood vessels as well, and this is done in two phases: the initial phase of relaxation, dependent on the endothelium, is then replaced by a slowly developing tonic contraction [66. Chen KM, Guan YY, Sun JJ. Effects of direct lytic factors from southern Chinese cobra venom on Ca2+ movement in rabbit aorta strip. Zhongguo Yao Li Xue Bao. 1993 Nov;14(6):500-4., 77. Ho KH, Kwan CY, Huang SJ, Bourreau JP. Dual effect of cobra cardiotoxin on vascular smooth muscle and endothelium. Zhongguo Yao Li Xue Bao. 1998 May;19(3):197-202.]. However, there are practically no data on the similarities or differences in the effect of different types of CaTXs on the heart and blood vessels.

Cytotoxins (cardiotoxins) 1 (CTX-1) and 2 (CTX-2) from the venom of the Central Asian cobra Naja oxiana belong to the S- and P-types, respectively [88. Grishin EV, Sukhikh AP, Adamovich TB, Ovchinnikov YA. Isolation, properties, and amino acid sequence of two cytotoxins from the venom of the Central Asian cobra Naja naja oxiana. Bioorg Khim. 1976;2(8):1018-34.]. In our recent work [99. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6.], we studied the effect of CTX-1 and CTX-2 on papillary muscle from the right ventricle of the rat heart. CTX-2 was found to show greater activity than CTX-1 [99. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6.]. However, in view of the tissue-specificity of the cardiotoxin effects [77. Ho KH, Kwan CY, Huang SJ, Bourreau JP. Dual effect of cobra cardiotoxin on vascular smooth muscle and endothelium. Zhongguo Yao Li Xue Bao. 1998 May;19(3):197-202., 1010. Wang CH, Monette R, Lee SC, Morley P, Wu WG. Cobra cardiotoxin-induced cell death in fetal rat cardiomyocytes and cortical neurons: different pathway but similar cell surface target. Toxicon. 2005 Sep 15;46(4):430-40.-1212. Lertwanakarn T, Suntravat M, Sanchez EE, Boonhoh W, Solaro RJ, Wolska BM, Martin JL, de Tombe PP, Tachampa K. Suppression of cardiomyocyte functions by β-CTX isolated from the Thai king cobra (Ophiophagus hannah) venom via an alternative method. J Venom Anim Toxins incl Trop Dis. 2020 Jul 17;26:e20200005. doi: 10.1590/1678-9199-JVATITD-2020-0005.
https://doi.org/10.1590/1678-9199-JVATIT... ], it remained unclear whether these differences would extend to cardiotoxin action on such a complex object as a whole heart containing several types of tissues.

It was shown previously that CTX-2 at the concentration of 10 μg/mL produced a decrease in the amplitude of heart contractions, bradycardia and cardiac arrest in systole of an isolated frog heart, while CTX-1 caused arrhythmia, and at significantly higher concentrations also caused systolic cardiac arrest [88. Grishin EV, Sukhikh AP, Adamovich TB, Ovchinnikov YA. Isolation, properties, and amino acid sequence of two cytotoxins from the venom of the Central Asian cobra Naja naja oxiana. Bioorg Khim. 1976;2(8):1018-34.]. The explanation for these differences has not been clarified. Furthermore, the question of the applicability of the data obtained on the amphibian heart to mammalian physiology and, in particular, the human heart, remains unresolved. It should be noted that the effect of Naja naja atra cobra venom and some of its fractions, identified by the authors as cardiotoxic to the rat heart, was studied previously [55. Sun JJ, Walker MJ. Actions of cardiotoxins from the southern Chinese cobra (Naja naja atra) on rat cardiac tissue. Toxicon. 1986;24(3):233-45.]. However, data on the composition of the investigated venom fractions were not given. In this work, we investigated the effects of individual well-characterized cardiotoxins, namely CTX-1 (S-type) and CTX-2 (P-type), on the contractile parameters of a whole rat heart perfused according to the Langendorff technique.

Figure 1.
Amino-acid sequences of CTX-1 (UniProtKB accession # P01451 (3SA1_NAJOX)) and CTX-2 (UniProtKB accession # P01441 (3SA2_NAJOX)). Serine 28 (S) and proline 30 (P) residues are shown in red.

Methods

Cardiotoxins were purified from Naja oxiana cobra venom as described previously [33. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Konshina AG, Utkin YN, Efremov RG, Arseniev AS. Interaction of three-finger toxins with phospholipid membranes: comparison of S- and P-type cytotoxins. Biochem J. 2005 May 1;387(Pt 3):807-15., 1313. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Utkin YN, Arseniev AS. Interaction of the P-type cardiotoxin with phospholipid membranes. Eur J Biochem. 2003 May;270(9):2038-46.], and their purity and structure were confirmed by HPLC and mass-spectrometry.

Adult male Wistar rats (body weight, 200-250 g) were used for the experiments. The study was conducted according to the guidelines of the Declaration of Helsinki, Directive 2010/63/EU of the European Parliament and of the Council on the protection of animals used for scientific purposes (22 September 2010) and approved by the Biological Safety and Ethics Committee of the Institute of Cellular Biophysics (Instruction for the use of laboratory animals in the Institute of Cellular Biophysics №57 of 30.12.2011). Hearts were perfused using the Langendorff technique essentially as previously described [1414. Minasian SM, Galagudza MM, Dmitriev YV, Kurapeev DI, Vlasov TD. Myocardial protection against global ischemia with Krebs-Henseleit buffer-based cardioplegic solution. J Cardiothorac Surg. 2013 Apr 2;8:60.]. Rats were anesthetized with sodium pentobarbital (50 mg/kg), the hearts were removed from the opened chest, immediately attached by the aorta to a cannula, and the retrograde perfusion of the isolated heart was performed under stable perfusion pressure of 75-80 mmHg with non-recirculating Tyrode solution containing (in mM): NaCl, 135; KCl, 4; MgCl₂,1; CaCl₂, 1.8; NaHCO₃, 14.5; NaH₂PO₄, 1.8; glucose, 11; pH 7.4. The perfusion solution was aerated with 95% O₂/5% CO₂, while its temperature was held constant at 37 ± 0.1°C. Left ventricular pressure (LVP) was measured isovolumetrically using a latex balloon introduced into the left ventricle through an incision in the left atrium and inflated to a baseline diastolic pressure of 10 mmHg. The balloon was connected to the pressure transducer, and the diastolic, systolic, and pulse LVP were recorded and processed using the software PhysExp (Cardioprotect Ltd., Saint Petersburg, Russian Federation).

After 30 minutes of equilibration, CTX-1 or CTX-2 was added to the solution and was maintained during the whole experiment at the concentration of 5 µg/mL. A group of 6 rats was used for CTX-1 measurements and another of 5 rats for CTX-2. The following parameters were registered: the left ventricular developed pressure (LVDP), calculated as the difference between systolic and diastolic pressure in the left ventricle; the end-diastolic pressure (LVEDP); the heart rate; time to maximum LVEDP (contracture of the heart) and time to depression of heart contractions (LVDP lower than 5 mmHg). In every experiment, the preparation was allowed to stabilize for 30 minutes before the measurement; the parameters registered for 10 seconds before CaTx application were used as control values.

The data were checked for normal distribution using the Shapiro−Wilk test. Statistical significance of the obtained results at p < 0.05 was assessed using the paired and unpaired Student’s t test. Data were presented as means ± SEM. Statistical data analysis was carried out using the software packages Microsoft Excel 2019 and GraphPad Prism 8.

Results

To compare the action of toxins, the concentration of 5 μg/mL was chosen since at lower concentrations the effect develops fairly slowly (during 30 to 60 minutes) [99. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6.], which can complicate data interpretation due to hypoxic phenomena that may occur in the myocardium. At the same time, the use of higher concentrations can mask possible differences in the activity of toxins [1515. Huang SJ, Kwan CY. Inhibition by multivalent cations of contraction induced by Chinese cobra venom cardiotoxin in guinea pig papillary muscle. Life Sci. 1996;59(4):PL55-60.]. In the experiments with CaTXs, the hearts used were those in which the LVDP levels after the stabilization period practically did not differ and were 80 ± 2 and 82 ± 2 mm Hg for CTX-1 and CTX-2, respectively. A study of the effect of toxins on the cardiac contractile activity showed that the two toxins acted similarly (Figure 2B and 2C): after a short latency period of 6-8 minutes for CTX-1 and 3-5 minutes for CTX-2, there was a short-term increase in systolic LVDP up to 103 ± 4 mmHg under the influence of CTX-1 and up to 123 ± 14 mmHg under the influence of CTX-2. Although this increase was statistically significant compared to the LVDP value before the application of CaTXs, the effects of two CaTXs did not differ significantly. This means that both toxins increased the strength of left ventricular contractions, the effect being slightly more pronounced with CTX-2 (Figure 2D). Next, there was a decrease in LVDP up to complete cardiac arrest with a simultaneous elevation in LVEDP, which was much stronger in the case of CTX-2, being 181 ± 24 mmHg versus 104 ± 14 mmHg for CTX-1, a statistically significant difference (Figure 2E). It should also be noted that it took significantly longer for the effects to fully develop under the influence of CTX-1, compared to CTX-2. Thus, from the beginning of exposure, CTX-1 and CTX-2 suppressed cardiac contractility at 676 ± 13 and 413 ± 35 seconds and caused contracture at 624 ± 32 and 529 ± 20 seconds, respectively, differences that were statistically significant (Figure 2F and 2G). Thus, CTX-1, belonging to the S type, demonstrated lower potency in the impairment of functional heart activity than the P-type CTX-2. It should also be noted that CTX-1 and CTX-2 did not induce significant changes in heart rate at the time when the positive inotropic effect on LVDP was already at its maximum (Figure 3).

Figure 2.
CaTX effects on the ventricular pressure parameters and effect development time. Representative traces of (A) untreated control and the effect of (B) CTX-1 and (C) CTX-2 at the concentration of 5 μg/mL on the contractile activity of the heart. (D) The magnitude of the temporary increase in LVDP and the maximum of (E) the developed contracture of the heart under the influence of CaTXs. The time required for complete suppression of contractile activity (F) in the left ventricle and (G) for reaching the maximum of LVEDP. CTX-1 (n = 6) and CTX-2 (n = 5). Data are presented as means ± standard error of the mean (*p < 0.05 compared to CTX-1 with unpaired two-tailed Student’s t test).

Figure 3.
The effects of CTX-1 and CTX-2 at the concentration of 5 μg/mL on the heart rate. Representative traces of the effect of (A) CTX-1 and (C) CTX-2 on the heart rate. Histograms showing heart rate in (B) CTX-1 (n = 6) and (D) CTX-2 (n = 5) groups. BPM: beats per min. Ten-second intervals were taken at the time when the positive inotropic effect on LVDP was already at its maximum (indicated as CTX-1 and CTX-2) and just before addition of CaTX (control). Data are presented as means ± standard error of the mean. No difference was observed at p < 0.05 by the paired two-tailed Student’s t test.

Discussion

CaTXs are the main components of cobra venom and manifest cytotoxicity against different types of cells [1616. Feofanov AV, Sharonov GV, Astapova MV, Rodionov DI, Utkin YN, Arseniev AS. Cancer cell injury by cytotoxins from cobra venom is mediated through lysosomal damage. Biochem J. 2005 Aug 15;390(Pt 1):11-8.]. As discussed previously, CaTXs are classified into two types, denominated S and P, the main difference between them being in the structure of their loop 2 (Figure 1). It was shown earlier that both P- and S-type toxins interact similarly with the lipid bilayer, namely by penetrating membrane with their three loops. However, P-type CaTX inserts its hydrophobic loop II deeper into the membrane than S-type CaTX [33. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Konshina AG, Utkin YN, Efremov RG, Arseniev AS. Interaction of three-finger toxins with phospholipid membranes: comparison of S- and P-type cytotoxins. Biochem J. 2005 May 1;387(Pt 3):807-15., 1313. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Utkin YN, Arseniev AS. Interaction of the P-type cardiotoxin with phospholipid membranes. Eur J Biochem. 2003 May;270(9):2038-46.]. Recently it was demonstrated that NS-CTX and NK-CTX, being P-type and S-type CaTXs, respectively, exhibited concentration-dependent growth inhibitory effects on human lung (A549), prostate (PC-3), and breast (MCF-7) cancer cell lines [1717. Chong HP, Tan KY, Tan CH. Cytotoxicity of snake venoms and cytotoxins from two southeast Asian cobras (Naja sumatrana, Naja kaouthia): exploration of anticancer potential, selectivity, and cell death mechanism. Front Mol Biosci. 2020 Nov 11;7:583587.]. Interestingly, P-type NS-CTX was significantly more potent in inhibiting the growth of the cancer cells [1717. Chong HP, Tan KY, Tan CH. Cytotoxicity of snake venoms and cytotoxins from two southeast Asian cobras (Naja sumatrana, Naja kaouthia): exploration of anticancer potential, selectivity, and cell death mechanism. Front Mol Biosci. 2020 Nov 11;7:583587.].

The biological effects of CaTXs include tissue necrosis, cardiac arrest and several others [1818. Dufton MJ, Hider RC. The structure and pharmacology of Elapid cytotoxins. In: Harvey AL, editor. Snake toxins. Perganon Press; New York, USA. p. 259-302. 1991.]. It should be noted that the acute toxicities of CaTXs of S- and P-types do not differ significantly, being in the range of 1-2 mg/kg for intravenous injection in mice [1919. Kaneda N, Sasaki T, Hayashi K. Primary structures of cardiotoxin analogues II and IV from the venom of Naja naja atra. Biochim Biophys Acta. 1977 Mar 28;491(1):53-66., 2020. Joubert FJ. Snake venom toxin. The amino acid sequence of three toxins (CM-2h, CM-4b and CM-6) from Naja haje annulifera (Egyptian cobra) venom. Hoppe Seylers Z Physiol Chem. 1977 Jan;358(1):79-96.]. An earlier study on the effect of some cardiotoxic cobra venom fractions on the isolated rat heart provided no data on the structure of toxins comprising these fractions [55. Sun JJ, Walker MJ. Actions of cardiotoxins from the southern Chinese cobra (Naja naja atra) on rat cardiac tissue. Toxicon. 1986;24(3):233-45.]. So far, there is no data about similarity or difference in the effects of the two types of CaTXs on the whole heart.

To compare the effects of the S- and P-type CaTXs on the isolated rat heart, we applied two individual toxins, CTX-1 and CTX-2, purified from Naja oxiana cobra venom. Our experiments showed that, in general, the development of the effects of both CaTXs on the whole rat heart proceeded as described in the literature for preparations of various types of myocardial tissue - the initial increase in contraction is followed by suppression with a simultaneous increase in the resting tension [99. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6., 2121. Wang HX, Lau SY, Huang SJ, Kwan CY, Wong TM. Cobra venom cardiotoxin induces perturbations of cytosolic calcium homeostasis and hypercontracture in adult rat ventricular myocytes. J Mol Cell Cardiol. 1997 Oct;29(10):2759-70.]. The available data indicate that CaTXs increase the concentrations of calcium ions in cardiomyocytes [2121. Wang HX, Lau SY, Huang SJ, Kwan CY, Wong TM. Cobra venom cardiotoxin induces perturbations of cytosolic calcium homeostasis and hypercontracture in adult rat ventricular myocytes. J Mol Cell Cardiol. 1997 Oct;29(10):2759-70., 2222. Wang CH, Wu WG. Amphiphilic beta-sheet cobra cardiotoxin targets mitochondria and disrupts its network. FEBS Lett. 2005 Jun 6;579(14):3169-74.], vascular smooth muscle cells [2323. Kwan CY, Kwan TK, Huang SJ. Effect of calcium on the vascular contraction induced by cobra venom cardiotoxin. Clin Exp Pharmacol Physiol. 2002 Sep;29(9):823-8.], and in vascular endothelial cells [2424. Ou YJ, Leung YM, Huang SJ, Kwan CY. Dual effects of extracellular Ca2+ on cardiotoxin-induced cytotoxicity and cytosolic Ca2+ changes in cultured single cells of rabbit aortic endothelium. Biochim Biophys Acta. 1997 Nov 13;1330(1):29-38.]. The observed initial increase in the heart contractility may be explained by the rise in the intracellular concentration of Ca²⁺ ions due to increase of the extracellular Ca²⁺ influx [2121. Wang HX, Lau SY, Huang SJ, Kwan CY, Wong TM. Cobra venom cardiotoxin induces perturbations of cytosolic calcium homeostasis and hypercontracture in adult rat ventricular myocytes. J Mol Cell Cardiol. 1997 Oct;29(10):2759-70.]. As CTX-2 induces a stronger increase in the heart contractility than CTX-1, the intracellular rise in the concentration of Ca²⁺ ions is probably higher in the presence of this toxin. However, it should be noted that due to the positive force-frequency correlation of the rat myocardium in the range of physiological frequencies [2525. Endoh M. Force-frequency relationship in intact mammalian ventricular myocardium: physiological and pathophysiological relevance. Eur J Pharmacol. 2004 Oct 1;500(1-3):73-86.], an increase in the heart rate can also result in LVDP elevation.

In our experiments, the heart rate does not increase in the presence of CaTXs (Figure 3) and, therefore, cannot account for LVDP growth. The observed subsequent diminution in LVDP and elevation in LVEDP may be a consequence of multiple processes leading to an overload of myocardial cells with Ca²⁺ and Na⁺ ions. These processes may include the activation of ion channels [2626. Tzeng WF, Chen YH. Suppression of snake-venom cardiotoxin-induced cardiomyocyte degeneration by blockage of Ca2+ influx or inhibition of non-lysosomal proteinases. Biochem J. 1988 Nov 15;256(1):89-95.], formation of a nonselective ion channel [2727. Wu PL, Chiu CR, Huang WN, Wu WG. The role of sulfatide lipid domains in the membrane pore-forming activity of cobra cardiotoxin. Biochim Biophys Acta. 2012 May;1818(5):1378-85.], and a change in the activity of ion pumps [2828. Huang JL, Trumble WR. Cardiotoxin from cobra venom affects the Ca-Mg-ATPase of cardiac sarcolemmal membrane vesicles. Toxicon. 1991;29(1):31-41., 2929. Bougis PE, Khélif A, Rochat H. On the inhibition of [Na+,K+]-ATPases by the components of Naja mossambica mossambica venom: evidence for two distinct rat brain [Na+,K+]-ATPase activities. Biochemistry. 1989 Apr 4;28(7):3037-43.], ultimately leading to the irreversible cell damage and death. Recently it has been shown that CaTXs are able to penetrate plasma membrane and outer mitochondrial membrane of the cell to target anionic cardiolipin and disrupt inner mitochondrial membrane structure and bioenergetics, which may result in cardiomyocyte death [3030. Gasanov SE, Shrivastava IH, Israilov FS, Kim AA, Rylova KA, Zhang B, Dagda RK. Naja naja oxiana cobra venom cytotoxins CTI and CTII disrupt mitochondrial membrane integrity: implications for basic three-fingered cytotoxins. PLoS One. 2015 Jun 19;10(6):e0129248., 3131. Li F, Shrivastava IH, Hanlon P, Dagda RK, Gasanoff ES. Molecular mechanism by which cobra venom cardiotoxins interact with the outer mitochondrial membrane. Toxins (Basel). 2020 Jun 27;12(7):425.]. All these processes are dependent on the integrity of the cell or mitochondrial membrane. P-type CTX-2 disrupts the membrane more strongly than S-type CXT-1 [33. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Konshina AG, Utkin YN, Efremov RG, Arseniev AS. Interaction of three-finger toxins with phospholipid membranes: comparison of S- and P-type cytotoxins. Biochem J. 2005 May 1;387(Pt 3):807-15.] and thus may more severely influence each of these processes.

Some differences between CTX-1 and CTX-2 in interaction with phospholipids were observed previously [3030. Gasanov SE, Shrivastava IH, Israilov FS, Kim AA, Rylova KA, Zhang B, Dagda RK. Naja naja oxiana cobra venom cytotoxins CTI and CTII disrupt mitochondrial membrane integrity: implications for basic three-fingered cytotoxins. PLoS One. 2015 Jun 19;10(6):e0129248.]. While both CTX-1 and CTX-2 exhibit similar biophysical effects on model membranes composed of phosphatidylcholine and cardiolipin for forming non-bilayer structures, only CTX-2 was able to form non-bilayer structures in large unilamellar membranes composed of phosphatidylcholine and phosphatidylserine [3030. Gasanov SE, Shrivastava IH, Israilov FS, Kim AA, Rylova KA, Zhang B, Dagda RK. Naja naja oxiana cobra venom cytotoxins CTI and CTII disrupt mitochondrial membrane integrity: implications for basic three-fingered cytotoxins. PLoS One. 2015 Jun 19;10(6):e0129248.]. Indeed, in our experiments, CTX-2 is more effective in contributing to the overload of cells with Ca²⁺ and Na⁺ ions as the increase in LVEDP is much stronger and the time to fully develop the effects is significantly shorter in the case of CTX-2. Overall, our results indicate that CTX-2 possesses a higher potency than CTX-1 in relation to damaging effects on the whole rat heart. Thus, the higher activity of CTX-2 as compared to CTX-1 demonstrated in the frog heart [88. Grishin EV, Sukhikh AP, Adamovich TB, Ovchinnikov YA. Isolation, properties, and amino acid sequence of two cytotoxins from the venom of the Central Asian cobra Naja naja oxiana. Bioorg Khim. 1976;2(8):1018-34.] and the papillary muscle of the rat right ventricle [99. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6.] is retained for the whole rat heart.

Conclusion

Therefore, for the first time, we have compared the effects of two types of CaTXs on the isolated mammalian heart. Both toxins showed a similar profile of action; however, the P-type toxin CTX-2 has a higher potency. Apparently, the previously shown greater ability of this toxin to disrupt the lipid bilayer in vitro leads to its greater toxicity ex vivo.

Abbreviations

CaTXs: cardiotoxins; CTX-1: cytotoxin (cardiotoxin) 1; CTX-2: cytotoxin (cardiotoxin) 2; LVDP: left ventricular developed pressure; LVEDP: left ventricle end-diastolic pressure; LVP: left ventricular pressure.

References

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6. Chen KM, Guan YY, Sun JJ. Effects of direct lytic factors from southern Chinese cobra venom on Ca2+ movement in rabbit aorta strip. Zhongguo Yao Li Xue Bao. 1993 Nov;14(6):500-4.
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10. Wang CH, Monette R, Lee SC, Morley P, Wu WG. Cobra cardiotoxin-induced cell death in fetal rat cardiomyocytes and cortical neurons: different pathway but similar cell surface target. Toxicon. 2005 Sep 15;46(4):430-40.
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» https://doi.org/10.1590/1678-9199-JVATITD-2020-0005
13. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Utkin YN, Arseniev AS. Interaction of the P-type cardiotoxin with phospholipid membranes. Eur J Biochem. 2003 May;270(9):2038-46.
14. Minasian SM, Galagudza MM, Dmitriev YV, Kurapeev DI, Vlasov TD. Myocardial protection against global ischemia with Krebs-Henseleit buffer-based cardioplegic solution. J Cardiothorac Surg. 2013 Apr 2;8:60.
15. Huang SJ, Kwan CY. Inhibition by multivalent cations of contraction induced by Chinese cobra venom cardiotoxin in guinea pig papillary muscle. Life Sci. 1996;59(4):PL55-60.
16. Feofanov AV, Sharonov GV, Astapova MV, Rodionov DI, Utkin YN, Arseniev AS. Cancer cell injury by cytotoxins from cobra venom is mediated through lysosomal damage. Biochem J. 2005 Aug 15;390(Pt 1):11-8.
17. Chong HP, Tan KY, Tan CH. Cytotoxicity of snake venoms and cytotoxins from two southeast Asian cobras (Naja sumatrana, Naja kaouthia): exploration of anticancer potential, selectivity, and cell death mechanism. Front Mol Biosci. 2020 Nov 11;7:583587.
18. Dufton MJ, Hider RC. The structure and pharmacology of Elapid cytotoxins. In: Harvey AL, editor. Snake toxins. Perganon Press; New York, USA. p. 259-302. 1991.
19. Kaneda N, Sasaki T, Hayashi K. Primary structures of cardiotoxin analogues II and IV from the venom of Naja naja atra Biochim Biophys Acta. 1977 Mar 28;491(1):53-66.
20. Joubert FJ. Snake venom toxin. The amino acid sequence of three toxins (CM-2h, CM-4b and CM-6) from Naja haje annulifera (Egyptian cobra) venom. Hoppe Seylers Z Physiol Chem. 1977 Jan;358(1):79-96.
21. Wang HX, Lau SY, Huang SJ, Kwan CY, Wong TM. Cobra venom cardiotoxin induces perturbations of cytosolic calcium homeostasis and hypercontracture in adult rat ventricular myocytes. J Mol Cell Cardiol. 1997 Oct;29(10):2759-70.
22. Wang CH, Wu WG. Amphiphilic beta-sheet cobra cardiotoxin targets mitochondria and disrupts its network. FEBS Lett. 2005 Jun 6;579(14):3169-74.
23. Kwan CY, Kwan TK, Huang SJ. Effect of calcium on the vascular contraction induced by cobra venom cardiotoxin. Clin Exp Pharmacol Physiol. 2002 Sep;29(9):823-8.
24. Ou YJ, Leung YM, Huang SJ, Kwan CY. Dual effects of extracellular Ca2+ on cardiotoxin-induced cytotoxicity and cytosolic Ca2+ changes in cultured single cells of rabbit aortic endothelium. Biochim Biophys Acta. 1997 Nov 13;1330(1):29-38.
25. Endoh M. Force-frequency relationship in intact mammalian ventricular myocardium: physiological and pathophysiological relevance. Eur J Pharmacol. 2004 Oct 1;500(1-3):73-86.
26. Tzeng WF, Chen YH. Suppression of snake-venom cardiotoxin-induced cardiomyocyte degeneration by blockage of Ca2+ influx or inhibition of non-lysosomal proteinases. Biochem J. 1988 Nov 15;256(1):89-95.
27. Wu PL, Chiu CR, Huang WN, Wu WG. The role of sulfatide lipid domains in the membrane pore-forming activity of cobra cardiotoxin. Biochim Biophys Acta. 2012 May;1818(5):1378-85.
28. Huang JL, Trumble WR. Cardiotoxin from cobra venom affects the Ca-Mg-ATPase of cardiac sarcolemmal membrane vesicles. Toxicon. 1991;29(1):31-41.
29. Bougis PE, Khélif A, Rochat H. On the inhibition of [Na+,K+]-ATPases by the components of Naja mossambica mossambica venom: evidence for two distinct rat brain [Na+,K+]-ATPase activities. Biochemistry. 1989 Apr 4;28(7):3037-43.
30. Gasanov SE, Shrivastava IH, Israilov FS, Kim AA, Rylova KA, Zhang B, Dagda RK. Naja naja oxiana cobra venom cytotoxins CTI and CTII disrupt mitochondrial membrane integrity: implications for basic three-fingered cytotoxins. PLoS One. 2015 Jun 19;10(6):e0129248.
31. Li F, Shrivastava IH, Hanlon P, Dagda RK, Gasanoff ES. Molecular mechanism by which cobra venom cardiotoxins interact with the outer mitochondrial membrane. Toxins (Basel). 2020 Jun 27;12(7):425.

Funding

This work was supported by the Russian Science Foundation, project № 21-14-00316.
Ethics approval

This study did not involve endangered or protected species. All animal procedures were performed on male Sprague-Dawley rats (obtained from the Laboratory of experimental animals, Pushchino, Russia), and were approved by the Biological Safety and Ethics Committee of the Institute of Cellular Biophysics (Instruction for the use of laboratory animals in the Institute of Cellular Biophysics № 57 of 30.12.2011). All handling of animals were carried out in accordance with Directive 2010/63/EU of the European Parliament.
Consent for publication

Not applicable

Publication Dates

Publication in this collection
04 Apr 2022
Date of issue
2022

History

Received
19 Oct 2021
Accepted
15 Dec 2021

© The Author(s). 2022 Open Access This article is distributed under the terms of the Creative Commons Attribution 4.0 International License (https://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The Creative Commons Public Domain Dedication waiver (https://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.

[1] 1. Dubovskii PV, Konshina AG, Efremov RG. Cobra cardiotoxins: membrane interactions and pharmacological potential. Curr Med Chem. 2014;21(3):270-87.

[2] 2. Dubovskii PV, Utkin YN. Antiproliferative activity of cobra venom cytotoxins. Curr Top Med Chem. 2015;15(7):638-48.

[3] 3. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Konshina AG, Utkin YN, Efremov RG, Arseniev AS. Interaction of three-finger toxins with phospholipid membranes: comparison of S- and P-type cytotoxins. Biochem J. 2005 May 1;387(Pt 3):807-15.

[4] 4. Harvey AL, Marshall RJ, Karlsson E. Effects of purified cardiotoxins from the Thailand cobra (Naja naja siamensis) on isolated skeletal and cardiac muscle preparations. Toxicon. 1982;20(2):379-96.

[5] 5. Sun JJ, Walker MJ. Actions of cardiotoxins from the southern Chinese cobra (Naja naja atra) on rat cardiac tissue. Toxicon. 1986;24(3):233-45.

[6] 6. Chen KM, Guan YY, Sun JJ. Effects of direct lytic factors from southern Chinese cobra venom on Ca2+ movement in rabbit aorta strip. Zhongguo Yao Li Xue Bao. 1993 Nov;14(6):500-4.

[7] 7. Ho KH, Kwan CY, Huang SJ, Bourreau JP. Dual effect of cobra cardiotoxin on vascular smooth muscle and endothelium. Zhongguo Yao Li Xue Bao. 1998 May;19(3):197-202.

[8] 8. Grishin EV, Sukhikh AP, Adamovich TB, Ovchinnikov YA. Isolation, properties, and amino acid sequence of two cytotoxins from the venom of the Central Asian cobra Naja naja oxiana Bioorg Khim. 1976;2(8):1018-34.

[9] 9. Averin AS, Astashev ME, Andreeva TV, Tsetlin VI, Utkin YN. Cardiotoxins from Cobra Naja oxiana change the force of contraction and the character of rhythmoinotropic phenomena in the rat myocardium. Dokl Biochem Biophys. 2019 Jul;487(1):282-6.

[10] 10. Wang CH, Monette R, Lee SC, Morley P, Wu WG. Cobra cardiotoxin-induced cell death in fetal rat cardiomyocytes and cortical neurons: different pathway but similar cell surface target. Toxicon. 2005 Sep 15;46(4):430-40.

[11] 11. Lee SC, Lin CC, Wang CH, Wu PL, Huang HW, Chang CI, Wu WG. Endocytotic routes of cobra cardiotoxins depend on spatial distribution of positively charged and hydrophobic domains to target distinct types of sulfated glycoconjugates on cell surface. J Biol Chem. 2014 Jul 18;289(29):20170-81.

[12] 12. Lertwanakarn T, Suntravat M, Sanchez EE, Boonhoh W, Solaro RJ, Wolska BM, Martin JL, de Tombe PP, Tachampa K. Suppression of cardiomyocyte functions by β-CTX isolated from the Thai king cobra (Ophiophagus hannah) venom via an alternative method. J Venom Anim Toxins incl Trop Dis. 2020 Jul 17;26:e20200005. doi: 10.1590/1678-9199-JVATITD-2020-0005.
» https://doi.org/10.1590/1678-9199-JVATITD-2020-0005

[13] 13. Dubovskii PV, Lesovoy DM, Dubinnyi MA, Utkin YN, Arseniev AS. Interaction of the P-type cardiotoxin with phospholipid membranes. Eur J Biochem. 2003 May;270(9):2038-46.

[14] 14. Minasian SM, Galagudza MM, Dmitriev YV, Kurapeev DI, Vlasov TD. Myocardial protection against global ischemia with Krebs-Henseleit buffer-based cardioplegic solution. J Cardiothorac Surg. 2013 Apr 2;8:60.

[15] 15. Huang SJ, Kwan CY. Inhibition by multivalent cations of contraction induced by Chinese cobra venom cardiotoxin in guinea pig papillary muscle. Life Sci. 1996;59(4):PL55-60.

[16] 16. Feofanov AV, Sharonov GV, Astapova MV, Rodionov DI, Utkin YN, Arseniev AS. Cancer cell injury by cytotoxins from cobra venom is mediated through lysosomal damage. Biochem J. 2005 Aug 15;390(Pt 1):11-8.

[17] 17. Chong HP, Tan KY, Tan CH. Cytotoxicity of snake venoms and cytotoxins from two southeast Asian cobras (Naja sumatrana, Naja kaouthia): exploration of anticancer potential, selectivity, and cell death mechanism. Front Mol Biosci. 2020 Nov 11;7:583587.

[18] 18. Dufton MJ, Hider RC. The structure and pharmacology of Elapid cytotoxins. In: Harvey AL, editor. Snake toxins. Perganon Press; New York, USA. p. 259-302. 1991.

[19] 19. Kaneda N, Sasaki T, Hayashi K. Primary structures of cardiotoxin analogues II and IV from the venom of Naja naja atra Biochim Biophys Acta. 1977 Mar 28;491(1):53-66.

[20] 20. Joubert FJ. Snake venom toxin. The amino acid sequence of three toxins (CM-2h, CM-4b and CM-6) from Naja haje annulifera (Egyptian cobra) venom. Hoppe Seylers Z Physiol Chem. 1977 Jan;358(1):79-96.

[21] 21. Wang HX, Lau SY, Huang SJ, Kwan CY, Wong TM. Cobra venom cardiotoxin induces perturbations of cytosolic calcium homeostasis and hypercontracture in adult rat ventricular myocytes. J Mol Cell Cardiol. 1997 Oct;29(10):2759-70.

[22] 22. Wang CH, Wu WG. Amphiphilic beta-sheet cobra cardiotoxin targets mitochondria and disrupts its network. FEBS Lett. 2005 Jun 6;579(14):3169-74.

[23] 23. Kwan CY, Kwan TK, Huang SJ. Effect of calcium on the vascular contraction induced by cobra venom cardiotoxin. Clin Exp Pharmacol Physiol. 2002 Sep;29(9):823-8.

[24] 24. Ou YJ, Leung YM, Huang SJ, Kwan CY. Dual effects of extracellular Ca2+ on cardiotoxin-induced cytotoxicity and cytosolic Ca2+ changes in cultured single cells of rabbit aortic endothelium. Biochim Biophys Acta. 1997 Nov 13;1330(1):29-38.

[25] 25. Endoh M. Force-frequency relationship in intact mammalian ventricular myocardium: physiological and pathophysiological relevance. Eur J Pharmacol. 2004 Oct 1;500(1-3):73-86.

[26] 26. Tzeng WF, Chen YH. Suppression of snake-venom cardiotoxin-induced cardiomyocyte degeneration by blockage of Ca2+ influx or inhibition of non-lysosomal proteinases. Biochem J. 1988 Nov 15;256(1):89-95.

[27] 27. Wu PL, Chiu CR, Huang WN, Wu WG. The role of sulfatide lipid domains in the membrane pore-forming activity of cobra cardiotoxin. Biochim Biophys Acta. 2012 May;1818(5):1378-85.

[28] 28. Huang JL, Trumble WR. Cardiotoxin from cobra venom affects the Ca-Mg-ATPase of cardiac sarcolemmal membrane vesicles. Toxicon. 1991;29(1):31-41.

[29] 29. Bougis PE, Khélif A, Rochat H. On the inhibition of [Na+,K+]-ATPases by the components of Naja mossambica mossambica venom: evidence for two distinct rat brain [Na+,K+]-ATPase activities. Biochemistry. 1989 Apr 4;28(7):3037-43.

[30] 30. Gasanov SE, Shrivastava IH, Israilov FS, Kim AA, Rylova KA, Zhang B, Dagda RK. Naja naja oxiana cobra venom cytotoxins CTI and CTII disrupt mitochondrial membrane integrity: implications for basic three-fingered cytotoxins. PLoS One. 2015 Jun 19;10(6):e0129248.

[31] 31. Li F, Shrivastava IH, Hanlon P, Dagda RK, Gasanoff ES. Molecular mechanism by which cobra venom cardiotoxins interact with the outer mitochondrial membrane. Toxins (Basel). 2020 Jun 27;12(7):425.

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