Karla A Oliveira, Ricardo J S Torquato, Daniela C G Garcia Lustosa, Tales Ribeiro, Bruno W L Nascimento, Lilian C G de Oliveira, Maria A Juliano, Thaysa Paschoalin, Virginia S Lemos, Ricardo N Araujo, Marcos H Pereira, Aparecida S Tanaka
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The cleavage activity of triapsin on PAR peptides was investigated based on FRET technology. Mass spectrometry was used to analyze the sites of PAR-2 peptide cleaved by triapsin. NO measurements were performed using the DAN assay (2,3-diaminonapthalene). The vasorelaxant activity of triapsin was measured in vessels with or without functional endothelium pre-contracted with phenylephrine (3 µM). Intravital microscopy was used to assess the effect of triapsin on mouse skin microcirculation.</p><p><strong>Results: </strong>Triapsin was able to induce hydrolysis of PAR peptides and showed a higher preference for cleavage of the PAR-2 peptide. Analysis by mass spectrometry confirmed a single cleavage site, which corresponds to the activation site of the PAR-2 receptor. Triapsin induced dose-dependent NO release in cultured human umbilical vein endothelial cells (HUVECs), reaching a maximum effect at 17.58 nM. Triapsin purified by gel-filtration chromatography (10<sup>-16</sup> to 10<sup>-9</sup> M) was applied cumulatively to mouse mesenteric artery rings and showed a potent endothelium-dependent vasodilator effect (EC<sub>30</sub> = 10<sup>-12</sup> M). Nitric oxide seems to be partially responsible for this vasodilator effect because L-NAME (L-NG-nitroarginine methyl ester 300 µM), a nitric oxide synthetase inhibitor, did not abrogate the vasodilation activated by triapsin. Anti-PAR-2 antibody completely inhibited vasodilation observed in the presence of triapsin activity. Triapsin activity also induced an increase in the mouse ear venular diameter.</p><p><strong>Conclusion: </strong>Data from this study suggest a plausible association between triapsin activity mediated PAR-2 activation and vasodilation caused by <i>T. infestans</i> saliva.</p>","PeriodicalId":520810,"journal":{"name":"The journal of venomous animals and toxins including tropical diseases","volume":" ","pages":"e20200098"},"PeriodicalIF":0.0000,"publicationDate":"2021-03-08","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7939238/pdf/","citationCount":"3","resultStr":"{\"title\":\"Proteolytic activity of <i>Triatoma infestans</i> saliva associated with PAR-2 activation and vasodilation.\",\"authors\":\"Karla A Oliveira, Ricardo J S Torquato, Daniela C G Garcia Lustosa, Tales Ribeiro, Bruno W L Nascimento, Lilian C G de Oliveira, Maria A Juliano, Thaysa Paschoalin, Virginia S Lemos, Ricardo N Araujo, Marcos H Pereira, Aparecida S Tanaka\",\"doi\":\"10.1590/1678-9199-JVATITD-2020-0098\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><strong>Background: </strong><i>Triatoma infestans</i> (Hemiptera: Reduviidae) is a hematophagous insect and the main vector of <i>Trypanosoma cruzi</i> (Kinetoplastida: Trypanosomatidae). 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引用次数: 3
摘要
背景:红三角虫(半翅目:红三角虫科)是一种吸血昆虫,是克氏锥虫的主要传播媒介。在本研究中,作者研究了从疟原虫唾液中提取的丝氨酸蛋白酶活性是否在血管舒缩调节中起作用,并通过切割和激活蛋白酶激活受体(PARs)来调节昆虫的血液摄食。方法:采用先前报道的方法,对大肠杆菌唾液进行层析,纯化丝氨酸蛋白酶triapsin。利用FRET技术研究了triapsin在PAR多肽上的裂解活性。质谱法分析了三肽裂解PAR-2肽的位点。采用DAN法(2,3-二氨基萘)测定NO。用苯肾上腺素(3µM)预收缩血管内皮,分别在有或无功能内皮的血管中测定triapsin的血管松弛活性。采用活体显微镜观察triapsin对小鼠皮肤微循环的影响。结果:Triapsin能够诱导PAR肽的水解,并且对PAR-2肽的裂解表现出更高的偏好。质谱分析证实了一个单一的裂解位点,该位点对应于PAR-2受体的激活位点。Triapsin诱导培养的人脐静脉内皮细胞(HUVECs)释放剂量依赖性NO,在17.58 nM处达到最大效果。经凝胶过滤层析纯化的Triapsin(10-16至10-9 M)累积应用于小鼠肠系膜动脉环,显示出有效的内皮依赖性血管扩张作用(EC30 = 10-12 M)。一氧化氮似乎是这种血管扩张作用的部分原因,因为一氧化氮合成酶抑制剂L-NAME (l- ng -硝基精氨酸甲酯300µM)并没有消除Triapsin激活的血管扩张作用。抗par -2抗体完全抑制血管舒张观察到存在triapsin活性。Triapsin活性也诱导小鼠耳静脉直径增加。结论:本研究的数据表明,triapsin活性介导的PAR-2激活与感染T.菌唾液引起的血管舒张之间可能存在关联。
Proteolytic activity of Triatoma infestans saliva associated with PAR-2 activation and vasodilation.
Background: Triatoma infestans (Hemiptera: Reduviidae) is a hematophagous insect and the main vector of Trypanosoma cruzi (Kinetoplastida: Trypanosomatidae). In the present study, the authors investigated whether a serine protease activity from the saliva of T. infestans has a role in vasomotor modulation, and in the insect-blood feeding by cleaving and activating protease-activated receptors (PARs).
Methods: T. infestans saliva was chromatographed as previously reported for purification of triapsin, a serine protease. The cleavage activity of triapsin on PAR peptides was investigated based on FRET technology. Mass spectrometry was used to analyze the sites of PAR-2 peptide cleaved by triapsin. NO measurements were performed using the DAN assay (2,3-diaminonapthalene). The vasorelaxant activity of triapsin was measured in vessels with or without functional endothelium pre-contracted with phenylephrine (3 µM). Intravital microscopy was used to assess the effect of triapsin on mouse skin microcirculation.
Results: Triapsin was able to induce hydrolysis of PAR peptides and showed a higher preference for cleavage of the PAR-2 peptide. Analysis by mass spectrometry confirmed a single cleavage site, which corresponds to the activation site of the PAR-2 receptor. Triapsin induced dose-dependent NO release in cultured human umbilical vein endothelial cells (HUVECs), reaching a maximum effect at 17.58 nM. Triapsin purified by gel-filtration chromatography (10-16 to 10-9 M) was applied cumulatively to mouse mesenteric artery rings and showed a potent endothelium-dependent vasodilator effect (EC30 = 10-12 M). Nitric oxide seems to be partially responsible for this vasodilator effect because L-NAME (L-NG-nitroarginine methyl ester 300 µM), a nitric oxide synthetase inhibitor, did not abrogate the vasodilation activated by triapsin. Anti-PAR-2 antibody completely inhibited vasodilation observed in the presence of triapsin activity. Triapsin activity also induced an increase in the mouse ear venular diameter.
Conclusion: Data from this study suggest a plausible association between triapsin activity mediated PAR-2 activation and vasodilation caused by T. infestans saliva.
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