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使用蛋白水解酶作为锥虫鉴定的额外工具。

Use of proteolytic enzymes as an additional tool for trypanosomatid identification.

作者信息

Santos A L S, Abreu C M, Alviano C S, Soares R M A

机构信息

Laboratório de Biologia de Protistas, Departamento de Microbiologia Geral, Instituto de Microbiologia Prof Paulo de Góes, Centro de Ciências da Saúde, Universidade Federal do Rio de Janeiro, Rio de Janeiro, RJ 21941-590, Brazil.

出版信息

Parasitology. 2005 Jan;130(Pt 1):79-88. doi: 10.1017/s0031182004006353.

Abstract

The expression of proteolytic activities in the Trypanosomatidae family was explored as a potential marker to discriminate between the morphologically indistinguishable flagellates isolated from insects and plants. We have comparatively analysed the proteolytic profiles of 19 monoxenous trypanosomatids (Herpetomonas anglusteri, H. samuelpessoai, H. mariadeanei, H. roitmani, H. muscarum ingenoplastis, H. muscarum muscarum, H. megaseliae, H. dendoderi, Herpetomoas sp., Crithidia oncopelti, C. deanei, C. acanthocephali, C. harmosa, C. fasciculata, C. guilhermei, C. luciliae, Blastocrithidia culicis, Leptomonas samueli and Lept. seymouri) and 4 heteroxenous flagellates (Phytomonas serpens, P. mcgheei, Trypanosoma cruzi and Leishmania amazonensis) by in situ detection of enzyme activities on sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE ) containing co-polymerized gelatine as substrate, in association with specific proteinase inhibitors. All 23 trypanosomatids expressed at least 1 acidic proteolytic enzyme. In addition, a characteristic and specific pattern of cell-associated metallo and/or cysteine proteinases was observed, except for the similar profiles detected in 2 Herpetomonas (H. anglusteri and H. samuelpessoai) and 3 Crithidia (C. fasciculata, C. guilhermei and C. luciliae) species. However, these flagellates released distinct secretory proteinase profiles into the extracellular medium. These findings strongly suggest that the association of cellular and secretory proteinase pattern could represent a useful marker to help trypanosomatid identification.

摘要

对锥虫科中蛋白水解活性的表达进行了探索,将其作为一种潜在标记,用于区分从昆虫和植物中分离出的形态上难以区分的鞭毛虫。我们通过在含有共聚明胶作为底物的十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳(SDS - PAGE)上原位检测酶活性,并结合特定蛋白酶抑制剂,比较分析了19种单宿主锥虫(安氏赫氏鞭毛虫、塞缪尔佩索阿赫氏鞭毛虫、玛丽亚德内赫氏鞭毛虫、罗伊特曼赫氏鞭毛虫、食蚜蝇赫氏鞭毛虫无质体、食蚜蝇赫氏鞭毛虫、大蠊赫氏鞭毛虫、树栖赫氏鞭毛虫、赫氏鞭毛虫属、康氏克氏锥虫、德氏克氏锥虫、棘头克氏锥虫、哈莫萨克氏锥虫、束状克氏锥虫、吉尔赫梅克氏锥虫、卢西利亚克氏锥虫、库蚊芽生锥虫、塞缪尔利什曼原虫和西莫里利什曼原虫)和4种异宿主鞭毛虫(蛇形植鞭毛虫、麦吉植鞭毛虫、克氏锥虫和亚马逊利什曼原虫)的蛋白水解谱。所有23种锥虫都至少表达1种酸性蛋白水解酶。此外,观察到一种与细胞相关的金属蛋白酶和/或半胱氨酸蛋白酶的特征性和特异性模式,但在2种赫氏鞭毛虫(安氏赫氏鞭毛虫和塞缪尔佩索阿赫氏鞭毛虫)和3种克氏锥虫(束状克氏锥虫、吉尔赫梅克氏锥虫和卢西利亚克氏锥虫)中检测到相似的谱。然而,这些鞭毛虫向细胞外培养基中释放了不同的分泌蛋白酶谱。这些发现强烈表明,细胞和分泌蛋白酶模式的组合可能是有助于锥虫鉴定的有用标记。

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