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绿僵菌在感染昆虫表皮中产生的两种细胞外胰蛋白酶的生化特性及超微结构定位

Biochemical characterization and ultrastructural localization of two extracellular trypsins produced by Metarhizium anisopliae in infected insect cuticles.

作者信息

St Leger R J, Joshi L, Bidochka M J, Rizzo N W, Roberts D W

机构信息

Boyce Thompson Institute, Cornell University, Ithaca, New York 14853, USA.

出版信息

Appl Environ Microbiol. 1996 Apr;62(4):1257-64. doi: 10.1128/aem.62.4.1257-1264.1996.

Abstract

Proteinase 2 (Pr2) is a fungal (Metarhizium anisopliae) serine proteinase which has a tryptic specificity for basic residues and which may be involved in entomopathogenicity. Analytical and preparative isoelectric focusing methods were used to separate two trypsin components, produced during growth on cockroach cuticle, with isoelectric points of 4.4 (molecular mass, 30 kDa) and 4.9 (27 kDa). The catalytic properties of the proteases were analyzed by their kinetic constants and by a combination of two-dimensional gelatin-sodium dodecyl sulfate-polyacrylamide gel electrophoresis and enzyme overlay membranes. Both Pr2 isoforms preferentially cleave at the carboxyl sides of positively charged amino acids, preferring arginine; the pI 4.4 Pr2 isoform also possessed significant activity against lysine. Compared with the pathogen's subtilisin-like enzyme (Pr1), the pI 4.4 Pr2 isoform shows low activity against insoluble proteins in a host (Manduca sexta) cuticle. However, it degrades most cuticle proteins when they are solubilized, with high-molecular-weight basic proteins being preferentially hydrolyzed. Polyclonal antibodies raised against each Pr2 isoform were isotype specific. This allowed us to use ultrastructural immunocytochemistry to independently visualize each isoform during penetration of the host (M. sexta) cuticle. Both isoforms were secreted by infection structures (appressoria) on the cuticle surface and by the penetrant hyphae within the cuticle. The extracellular sheath, which is commonly observed around fungal cells, often contained Pr2 molecules. Intracellular labelling was sparse.

摘要

蛋白酶2(Pr2)是一种真菌(绿僵菌)丝氨酸蛋白酶,对碱性残基具有胰蛋白酶特异性,可能参与昆虫致病性。采用分析型和制备型等电聚焦方法分离了在蟑螂表皮上生长过程中产生的两种胰蛋白酶成分,其等电点分别为4.4(分子量30 kDa)和4.9(27 kDa)。通过动力学常数以及二维明胶-十二烷基硫酸钠-聚丙烯酰胺凝胶电泳和酶覆盖膜相结合的方法分析了蛋白酶的催化特性。两种Pr2同工型均优先在带正电荷氨基酸的羧基侧切割,更倾向于精氨酸;pI 4.4的Pr2同工型对赖氨酸也具有显著活性。与病原体的枯草杆菌蛋白酶样酶(Pr1)相比,pI 4.4的Pr2同工型对宿主(烟草天蛾)表皮中的不溶性蛋白质活性较低。然而,当表皮蛋白溶解时,它会降解大多数表皮蛋白,高分子量碱性蛋白优先被水解。针对每种Pr2同工型产生的多克隆抗体具有同种型特异性。这使我们能够利用超微结构免疫细胞化学在宿主(烟草天蛾)表皮穿透过程中独立观察每种同工型。两种同工型均由表皮表面的侵染结构(附着胞)和表皮内的穿透菌丝分泌。通常在真菌细胞周围观察到的细胞外鞘中常含有Pr2分子。细胞内标记很少。

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