Direct effects of interleukin-8 on growth and functional activity of T lymphocytes

CD3⁺ T-lymphocytes were isolated from the normal donors by positive magnetic separation. Activation of the T cells with particles conjugated with antibodies to CD3, СD28 and СD2 molecules led to a marked increase in T-cell production of interleukine-8 (IL-8). We present evidence that IL-8 receptor α-chain (CXCR1, CD181) is expressed on the cell surface of 13.3% T cells. Activation of T-lymphocytes resulted in significant enhancement of CD181⁺ cells both in naive CD4⁺ T cell and terminally differentiated effector CD4⁺ T cell compartments with concomitant reduction of CD181⁺ cells in effector memory CD4⁺ T cell subset. The level of T cell activation was assessed judging from the surface expression of CD25 (IL-2 receptor α-chain). We demonstrate that IL-8 treatment (0.01–10.0 ng/ml concentration range) reduced the activation status of both CD4⁻ and CD4⁺ effector memory T cells, as well as terminally differentiated effector T cells, without significantly affecting the activation of naive T cells or central memory T cells. In addition, IL-8 up-regulated IL-2 and down-regulated IL-10 production by activated T cells, with no effect on interferon-gamma (IFN-γ) and IL-4 production. Data obtained suggests the importance of IL-8 in the direct regulation of adaptive T cell reactivity.     

Antibodies against Tityus discrepans venom do not abolish the effect of Tityus serrulatus venom on the rat sodium and potassium channels.

Anti-(Tityus serrulatus + Tityus bahiensis) and anti-Tityus discrepans venom polyclonal antisera were used to investigate whether antigenic differences exist between the venoms of the Brazilian T. serrulatus and the Venezuelan T. discrepans scorpions. Both antisera recognised the toxin-containing electrophoretic fractions of their cognate venoms and also those from Tityus zulianus and Tityus trinitatis venoms on Western blots. The anti-T. discrepans antiserum reacted only weakly with T. serrulatus toxic polypeptides. The effect of T. serrulatus alpha- or beta-toxins on rat skeletal muscle Na+ channels expressed in Xenopus laevis oocytes was abolished by pre-incubating the venom with anti-(T. serrulatus + T. bahiensis) serum but not with anti-T. discrepans serum. Nor did the Brazilian or the Venezuelan sera prevent the reduction in K+ currents by T. serrulatus venom in X. laevis oocytes expressing the rat brain delayed rectifying Shaker K+ channel (Kv1.2). These results indicate that toxins from T. serrulatus and T. discrepans venoms, which primarily target mammalian Na+ channels, are antigenically distinct, although they probably share common epitopes. Our results also suggest that Na+ channel-active toxins are the immunodominant antigens of the T. serrulatus venom.     

Antigenic relationships of fractionated western diamondback rattlesnake (Crotalus atrox) hemorrhagic toxins and other rattlesnake venoms as indicated by monoclonal antibodies

Seven hemorrhagic factors have been isolated from Crotalus atrox venom, but their antigenic relationships have not been well studied. In this study, two different monoclonal antibodies, C. atrox peak 8 (CA-P-8) and C. atrox subclone 5 (CA-5+), were produced against two C. atrox venom hemorrhagic fractions and used in an ELISA (enzyme-linked immunosorbent assay) to determine if the hemorrhagic factors in C. atrox venom are antigenically related. The same ELISA test was used to determine cross-reactivity of seven other crude Crotalidae venoms. The two monoclonal antibodies were tested for their ability to neutralize each hemorrhagic HPLC fraction separated from C. atrox venom. C. atrox venom was fractionated into 22 fractions using HPLC analytical DEAE ion exchange. Fractions 4-17 were hemorrhagic. The CA-P-8 monoclonal antibody reacted strongly with hemorrhagic fraction 8; CA-5+ had a broader reactivity and reacted with several HPLC hemorrhagic and non-hemorrhagic fractions. Crude venoms of C. adamanteus, C. scutulatus scutulatus and C. viridis lutosus reacted with CA-P-8, while C. viridis lutosus, C. viridis oreganus, C. scutulatus scutulatus and C. horridus horridus reacted with CA-5+. C. molossus molossus and C. lepidus lepidus did not react with CA-P-8 and CA-5+. Hemorrhagic HPLC fractions 6, 7, 8, were completely neutralized by monoclonal antibody CA-P-8; fraction 9 was partially neutralized. The present study indicated that some C. atrox venom HPLC hemorrhagic fractions have both common and unique epitopes. Antigenic determinants were also found to be shared among different Crotalus species.(ABSTRACT TRUNCATED AT 250 WORDS)     

Isolation and characterization of two novel scorpion toxins: The α-toxin-like CeII8, specific for Nav1.7 channels and the classical anti-mammalian CeII9, specific for Nav1.4 channels

Scorpion β-toxins represent a particular pharmacological group of voltage-gated sodium channel (VGSC) neurotoxins. They typically shift the voltage dependence of activation to more hyperpolarizing potentials and reduce the peak current amplitude by binding to receptor-site 4. Here, we report the purification and functional characterization of the first voltage-gated sodium channel toxins, CeII8 and CeII9, isolated from the scorpion Centruroides elegans (Thorell, 1876), which is responsible for deadly cases of intoxication in Mexico. The soluble venom was fractionated by gel filtration and ion-exchange chromatography, followed by reversed-phase HPLC. The toxins CeII8 and CeII9 were further purified and both their amino acid sequence and molecular weight were determined. Both toxins were electrophysiologically characterized on four mammalian VGSCs (rNa_v1.2, rNa_v1.4, hNa_v1.5 and rNa_v1.7) expressed heterologously in Xenopus laevis oocytes, using the two-electrode voltage-clamp technique. Although CeII8 has the highest sequence similarity with scorpion α-toxins, inhibiting the inactivation of VGSCs, 300 nM toxin had a clear β-toxin effect and was selective towards Na_v1.7, involved in short-term and inflammatory pain. To the best of our knowledge, CeII8 is the first β-toxin active on Na_v1.7. CeII9, a typical anti-mammalian β-toxin, selectively modulated Na_v1.4 at a concentration of 700 nM and was, in contrast to CeII8, found to be lethal to mice. Interestingly, both toxins, despite their differences in amino acid sequence, only altered the biophysical properties of a fraction of the expressed sodium channels. Since these effects have also been reported for the β-toxin CssIV, the bioactive surfaces of the toxins have been compared to each other.     

Experimental immunization with Thalassophryne nattereri fish venom: striking IL-5 production and impaired of B220+ cells.

Murine experimental model have been useful to understanding the toxic as well as the pharmacological properties of the Thalassophryne nattereri venom. However, the specific immune response to T. nattereri venom in mice is yet unclear. Our results showed that the venom elicited in BALB/c mice high levels of specific IgG1 and total IgE isotype with high affinity, accompanied by a striking IL-5 production, what point out to a Th2-like response. Meanwhile, the production of IFN-gamma by lymphocytes pool expanded upon mitogen stimulus, suggests that the venom was also able to activate Th1 clones. Elevated number of antigen-presenting cells expressing CD11c or CD11b from day 4 to 6 supported ongoing antigen presentation process in the primary response and efficient T-cell expansion (increase of CD4(+) cells). In contrast, decreased B220 expression was observed, suggesting that the formation of memory long lived cell compartment. In conclusion, T. natterri venom stimulates an association of cytokine of both Th1 and Th2 profile, with a notable IL-5 production and specific IgG1 and total IgE isotypes secretion. Furthermore, our finding showed that T. natterri venom can affect the B cell fate and induce a memory antibody response through the secretion of protective IgG subclasses. Further studies with the venom protein toxins may provide clues to molecular mechanism regulating proliferation and differentiation of antibody-secreting cells in our model. A better understating of how T. natterri venom can modulate immune response could be useful in therapeutic strategies.     

In vitro and in vivo inhibitory effects of Tabernaemontana alternifolia against Naja naja venom

BackgroundTabernaemontana alternifolia root is traditionally used and practiced among few Indian tribes as an antidote for snakebites.ObjectiveTo combat and neutralize Naja naja venom using methanolic root extract of Tabernaemontana alternifolia and to explore its efficacy on venom biomarkers in search of newer herbal antidote or first-aid-point of care for therapeutics.Materialization.Pharmacological activities such as fibrinogenolytic, direct and indirect hemolytic activities for the neutralization of the venom were evaluated. Lethal toxicity annulation studies were performed using the murine model by pre-incubation and post-treatment protocols. Further, the neutralization of edema and myotoxicity were also evaluated.ResultsElectrophoretic analysis revealed that the complete neutralization of fibrinogen degradation was observed at 1:10 (w/w) (venom to extract). T. alternifolia exhibited an effective dose (ED₅₀) value of 87.20 µg/mL for venom-induced hemolysis. Venom at 2 µg concentration produced 11 mm of hemolytic radiance and was neutralized at 1:20 (w/w) venom to extract concentration. The survival time and the neurotoxic symptoms in mice were concluded to be delayed by both the methods of lethal toxicity inhibition using methanol extract. The edema ratio reduced the venom to extract ratio of 1:20 (w/w) from 173 ± 45% to 133.61% when subjected to 5 µg of venom concentration. The plant extract significantly neutralized the myotoxic activity.ConclusionT. alternifolia methanolic root extract could be a potent contributor in the effective treatment of N. naja venom-induced toxicity.     

Purification and characterization of a mammalian toxin from venom of the Mexican scorpion,Centruroides limpidus tecomanus Hoffmann

The venom from the scorpion Centruroides limpidus tecomanus Hoffmann was obtained by homogenization of entire telsons and electrical stimulation of anaesthetized animals. Both venom preparations contain toxic proteins to mice and were separated in a Sephadex G-50 column followed by carboxymethyl-cellulose chromatography. At least two toxic fractions were resolved from the homogenized telsons and three toxic fractions from the venom obtained by electrical stimulation. Rechromatography of the latter fractions on an ion exchange column (Aminex A-5) gave a homogeneous toxin called II.9.3, which on amino acid analysis was shown to be composed of 65 residues with a calculated mol. wt of 7335. The N-terminal sequence is H-Lys-Glx-Gly-X-Leu-Val-Asx-His-X-Thr-Gly-Cys-…, homologous to other scorpion toxins. The venom obtained by electrical stimulation was further characterized; the fraction I from the Sephadex G-50 chromatography shows hyaluronidase activity, although the fraction III shows at least 15 different components positive to ninhydrin, after separation by peptide mapping techniques.     

芋螺镇痛多肽研究进展

芋螺多肽由芋螺毒液管和毒囊内壁的毒腺所分泌,大多数芋螺多肽由10～40个氨基酸残基组成,且富含二硫键,能特异性作用于乙酰胆碱受体 (nAChR),及钙、钠、钾等多种离子通道亚型。目前已发现作用于N-型钙通道、nAChR的α9α10亚基、TTX-R钠通道、NMDA受体的芋螺多肽具有很强的镇痛活性,其中N-型钙通道抑制剂ω-MVIIA已于2004年上市。该类镇痛多肽具有相对分子质量小、结构稳定、活性及选择性高等特点。芋螺镇痛多肽不仅会成为镇痛机制等相关神经生物学研究的重要工具,也会为开发新一代无致瘾镇痛药起到重要作用。本文对芋螺镇痛多肽研究的最新进展予以评述,着重介绍芋螺镇痛多肽的作用靶位、构效关系及其应用进展。     

In vitro effects of an immunostimulating bacterial lysate on human lymphocyte function

MLBL is an oral immunostimulating vaccine consisting of bacterial standardized lysates obtained by mechanical lysis of different strains of Gram-positive and Gram-negative bacteria that can cause acute and chronic infections of the respiratory tract. Previous studies suggested a stimulating effect of MLBL both on humoral and cellular immune responses. In the present study, the in vitro effects of MLBL on human lymphocyte effector functions and its mechanisms of action were evaluated. The results show that the most remarkable effects of MLBL on the immune system are: i) activation of the IL-2 receptor (IL-2Ralpha) on different lymphocyte subsets (B, CD4+ T and CD8+ T cells) involved both in humoral and cellular immune responses; ii) induction of cytokine synthesis (IL-2, IL-10, IL-12, IFNgamma) in the immune competent cells that induce and regulate immune responses; iii) generation of CD4+ and CD8+ effector T cells. Overall, these results suggest that the therapeutic effect of MLBL on acute and recurrent infections of the respiratory tract is related to its ability to activate the responses of different subsets of immune competent cells both for humoral and cellular immunity. Moreover, these effects can be induced either by direct immune cell activation or through the generation and activation of immune effector cells.     

Erythropoietin exerts direct immunomodulatory effects on the cytokine production by activated human T-lymphocytes

The effect of erythropoietin-β (Epo-β) on the functional profile of activated human T-lymphocytes remains largely unknown, which hinders clinical application of Epo as an immunomodulatory agent. We studied the direct impact of Epo on the activation status of human T lymphocytes following activation by particles loaded with antibodies (Abs) against human CD2, CD3, and CD28. T cell activation was assessed by the surface expression of CD38 activation marker. Epo did not significantly affect activation status of both CD4⁺ and CD4⁻ T cells, as well as of naive (CD45RA⁺ CD197⁺), central memory (CD45RA⁻ CD197⁺), effector memory (CD45RA⁻ CD197⁻), and terminally-differentiated (CD45RA⁺ CD197⁻) T cells. However, Epo markedly augmented production of IL-2, IL-4 and IL10 by activated T cells with concomitant reduction in IFN-γ secretion. Taken together, our data showed that Epo could directly down-regulate pro-inflammatory T cell responses without affecting T cell activation status.     

An Overview of The Three Dimensional Structure of Short Spider Toxins

Arthropods are one of the most diverse animal groups on the Earth. Spiders belong to this phylum and they are ancient animals with a history going back some three hundred million years. They are abundant, widespread, and natural controllers of insect populations. They use their venom to capture prey or to fight against predators. This venom is constituted of various peptides and enzymes with different activities. Among these proteins, toxic peptides are responsible for the macroscopic effect of the venom.

Most of the toxins are known to interact with ion channels (mainly potassium channels, sodium channels, and calcium channels). These transmembrane molecules are ubiquitous in the cells. They underlie a broad range of the most basic biological processes, from excitation and signaling to secretion and absorption. Like enzymes they are diverse and ubiquitous macromolecular catalysts with high substrate specificity and subject to strong regulation. Animal toxins and, more specifically, spider toxins are effectors of these channels. Depending on the peptide, they have ability to block the channel by plugging into its pore of conduction, or by modifying the opening and closing capacity of the channels, binding on a few specific sites along the structure of the channel.

Most of these peptides fold according to the overall same pattern, the inhibitor cystine knot (ICK) scaffold. Basically, it consists of a ring formed by a part of the backbone of the peptide and two disulfide bridges, penetrated by a third disulfide bridge. An additional disulfide bridge might be found in some toxins. Another fold has been found in a few toxins and has been described as the DDH scaffold. This motif lacks the knot and comprises an antiparallel β -hairpin stabilized by two conserved disulfide bridges.

This paper will try to summarize the structural characteristics of the spider toxins for which the fold has been described in the literature.     

Biosynthesis,secretion and in vivo isotopic labelling of venom of the Egyptian cobra, Naja haje annulifera

The venom glands of Elapidae differ from those of the Viperidae by lacking an expanded central lumen; the venom is stored in the tubular lumina as well as inside the cells in densely packed secretion granules. Using isotope tracer techniques, it was found that in the Egyptian cobra (Naja haje annulifera) venom is secreted both from pre-existing and from newly-formed granules. The rate of protein biosynthesis peaks at 4–9 days after venom was extracted (milked) from the glands. Highly labelled toxins (1–10 mCi/mmole protein) were isolated in good yield from the venom of snakes chronically intubated and infused i.p. with (³H)-amino acids. Repeated Fluothane (Halothane) anaesthesias and venom collections had no ill effect on venom yield. The radioactive venom and its component toxins retained full biological potency.     

Cytokine regulation by MAPK activated kinase 2 in keratinocytes exposed to sulfur mustard

Uncontrolled inflammation contributes to cutaneous damage following exposure to the warfare agent bis(2-chloroethyl) sulfide (sulfur mustard, SM). Activation of the p38 mitogen activated protein kinase (MAPK) precedes SM-induced cytokine secretion in normal human epidermal keratinocytes (NHEKs). This study examined the role of p38-regulated MAPK activated kinase 2 (MK2) during this process. Time course analysis studies using NHEK cells exposed to 200 μM SM demonstrated rapid MK2 activation via phosphorylation that occurred within 15 min. p38 activation was necessary for MK2 phosphorylation as determined by studies using the p38 inhibitor SB203580. To compare the role of p38 and MK2 during SM-induced cytokine secretion, small interfering RNA (siRNA) targeting these proteins was utilized. TNF-α, IL-1β, IL-6 and IL-8 secretion was evaluated 24 h postexposure, while mRNA changes were quantified after 8 h. TNF-α, IL-6 and IL-8 up regulation at the protein and mRNA level was observed following SM exposure. IL-1β secretion was also elevated despite unchanged mRNA levels. p38 knockdown reduced SM-induced secretion of all the cytokines examined, whereas significant reduction in SM-induced cytokine secretion was only observed with TNF-α and IL-6 following MK2 knockdown. Our observations demonstrate potential activation of other p38 targets in addition to MK2 during SM-induced cytokine secretion.     

核潜艇长航对艇员T淋巴细胞凋亡及肿瘤坏死因子-α白细胞介素-8白细胞介素-2的影响

目的了解核潜艇长航前后艇员T淋巴细胞凋亡率及血清肿瘤坏死因子(TNF)-ɑ、白细胞介素(IL)-8和IL-2含量的变化,探讨核潜艇长航对艇员免疫功能的影响。方法分别采集核潜艇艇员出航前后外周血标本,分离T淋巴细胞,经细胞凋亡分析仪检测比较长航前后T淋巴细胞凋亡率的变化;应用专用放身免疫试剂盒检测并比较长航前后艇员血液内TNF-α、IL-2、IL-8含量的变化。结果①长航后,核潜艇艇员外周血T淋巴细胞凋亡率增高(P<0.01);②长航后血液内细胞因子TNF-α、IL-8含量降低(P<0.05),IL-2含量则升高(P<0.05)。结论核潜艇长航后艇员外周血T淋巴细胞寿命缩短,凋亡率升高;机体内细胞因子的含量也受影响,舱室复杂环境因素可影响艇员免疫功能。     

Stejnihagin, a novel snake metalloproteinase from Trimeresurus stejnegeri venom, inhibited L-type Ca channels

Snake venom metalloproteinases (SVMPs) mainly distribute in Crotalid and Viperid snake venom and are classified into the Reprolysin subfamily of the M12 family of metalloproteinases. Previous function investigations have suggested that SVMPs are the key toxins involved in a variety of snake venom-induced pathogenesis including systemic injury, local damage, hemorrhage, edema, hypotension, hypovolemia, inflammation and necrosis. However, up to now, there is no report on ion channels blocking activity about SVMPs. Here, from Trimeresurus stejnegeri venom we purified a component Stejnihagin containing a mixture of Stejnihagin-A and -B, with 86% sequences identity, both as members of SVMPs. In the study, whole-cell patch clamp and vessel tension measurement were employed to identify the effect of Stejnihagin on L-type Ca²⁺ channels and vessel contraction. The results show that Stejnihagin inhibited L-type Ca²⁺channels in A7r5 cells with an IC₅₀ about 37 nM and simultaneously blocked 60 mM K⁺-induced vessel contraction. Besides, the inhibitory effect of Stejnihagin on L-type Ca²⁺ channels was also independent of the enzymatic activity. This finding offers new insight into the snake venom metalloproteinase functions and provides a novel pathogenesis of T. stejnegeri venom. Furthermore, it may also provide a clue to study the structure-function relationship of animal toxins and voltage-gated Ca²⁺ channel.     

Bothrops moojeni venom and BmooLAAO-I downmodulate CXCL8/IL-8 and CCL2/MCP-1 production and oxidative burst response,and upregulate CD11b expression in human neutrophils

Bothrops snake venoms contain biologically active components, including L-amino acid oxidases (LAAO) that induce significant leukocyte accumulation at inflammatory sites characterized by early neutrophil infiltration. As it remains unclear how snake venoms modulate neutrophil activation and chemokine production, here we examined whether Bothrops moojeni crude venom (BmV) and its LAAO (BmooLAAO-I) affect expression of the surface activation markers CD11b and CD66b, production of the chemokines CCL2/MCP-1, CCL5/RANTES, CXCL8/IL-8, CXCL9/MIG, and CXCL-10/IP-10, and activation of oxidative burst in human neutrophils. Cell viability, expression of activation markers, and chemokine production were assessed by flow cytometry, while the oxidative burst response was measured by chemiluminescence. BmV at 50 and 75 µg/mL reduced CXCL8/IL-8 (p < 0.001 and p < 0.01, respectively) and CCL2/MCP-1 production (p < 0.05), while BmooLAAO-I at the same concentrations reduced only CCL2/MCP-1 production (p < 0.01). These effects were accompanied by CD11b upregulation (p < 0.05 for 50 and 75 µg/mL BmV; p < 0.01 for 50 and 75 µg/mL BmooLAAO-I) and CD66b downregulation (p < 0.05 for 50 and 75 µg/mL BmV). Both BmV and BmooLAAO-I at concentrations ranging from 0.625 to 5 µg/mL suppressed the oxidative burst of neutrophils stimulated with phorbol 12-myristate 13-acetate, while BmooLAAO-I at 2.5 and 5 µg/mL also suppressed the neutrophil response stimulated with opsonized zymosan. Considering that neutrophils participate in the pathogenesis of autoimmune and inflammatory diseases, the findings reported herein indicate that BmV and BmooLAAO-I are potential immunomodulating agents.     

Effects of the venom of the Brazilian scorpion Tityus serrulatus and two of its fractions on the isolated diaphragm of the rat

1. The effects of Tityus serrulatus venom and of two of its toxic fractions, toxin gamma (Tx gamma) and T2III1, on the rat isolated diaphragm were examined. 2. The crude venom (5 ng) facilitated the neuromuscular transmission and increased the twitch tension evoked by retrograde injection of Ach. 3. Tx gamma (25-100 ng) and fraction T2III1 (2.5 ng) also facilitated the neuromuscular transmission but only fraction T2III1 increased the twitch tension evoked by retrograde injection of Ach. 4. Tx gamma (50 ng) and fraction T2III1 (2.5 ng) produced a tetrodotoxin-sensitive increase in the frequency of miniature endplate potentials (m.e.p.p.) and a transitory reduction of the resting potential. The latter effect of the fractions was prevented by treating muscles with tetrodotoxin or D-tubocurarine. Fraction T2III1 also produced a tetrodotoxin-resistance increase of m.e.p.p. amplitude. 5. These results suggest that Tx gamma enhances Ach output through the activation of Na+ channels in the motor nerve terminals. Fraction T2III1 produced effects similar to those induced by Tx gamma but also acted at postjunctional sites, probably by increasing subsynaptic membrane sensitivity to the neurotransmitter.