首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Characterization and Ultrastructural Localization of Chitinases from Metarhizium anisopliae M. flavoviride and Beauveria bassiana during Fungal Invasion of Host (Manduca sexta) Cuticle
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Characterization and Ultrastructural Localization of Chitinases from Metarhizium anisopliae M. flavoviride and Beauveria bassiana during Fungal Invasion of Host (Manduca sexta) Cuticle

机译:寄主(Manduca sexta)角质层真菌侵染过程中金属异形体黄萎病杆菌和球孢白僵菌的几丁质酶的表征和超微结构定位

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摘要

Extracellular chitinases have been suggested to be virulence factors in fungal entomopathogenicity. We employed isoelectric focusing and a set of three fluorescent substrates to investigate the numbers and types of chitinolytic enzymes produced by the entomopathogenic fungi Metarhizium anisopliae, Metarhizium flavoviride, and Beauveria bassiana. Each species produced a variety of N-acetyl-(beta)-d-glucosaminidases and endochitinases during growth in media containing insect cuticle. M. flavoviride also produced 1,4-(beta)-chitobiosidases. The endochitinases could be divided according to whether they had basic or acidic isoelectric points. In contrast to those of the other two species, the predominant endochitinases of M. anisopliae were acidic, with isoelectric points of about 4.8. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis resolved the acidic chitinases of M. anisopliae into two major bands (43.5 and 45 kDa) with identical N-terminal sequences (AGGYVNAVYFY TNGLYLSNYQPA) similar to an endochitinase from the mycoparasite Trichoderma harzianum. Use of polyclonal antibodies to the 45-kDa isoform and ultrastructural immunocytochemistry enabled us to visualize chitinase production during penetration of the host (Manduca sexta) cuticle. Chitinase was produced at very low levels by infection structures on the cuticle surface and during the initial penetration of the cuticle, but much greater levels of chitinase accumulated in zones of proteolytic degradation, which suggests that the release of the chitinase is dependent on the accessibility of its substrate.
机译:已经提出细胞外几丁质酶是真菌昆虫致病性中的毒力因子。我们采用等电聚焦和一组三个荧光底物来研究昆虫病原真菌金属假单胞菌,黄萎病杆菌和球孢白僵菌产生的几丁质分解酶的数量和类型。在含有昆虫角质层的培养基中生长期间,每个物种都产生各种N-乙酰基-β-d-氨基葡萄糖苷酶和内切质酶。黄病毒分枝杆菌还产生1,4-β-壳聚糖酶。内切壳多糖酶可以根据它们具有碱性或酸性等电点来区分。与其他两个物种相反,无芒分枝杆菌的主要内切壳蛋白酶是酸性的,等电点约为4.8。十二烷基硫酸钠-聚丙烯酰胺钠凝胶电泳将酸性支链霉菌的几丁质酶分解成两个主要带(43.5和45 kDa),它们具有相同的N端序列(AGGYVNAVYFY TNGLYLSNYQPA),类似于支原体木霉菌的内切几丁质酶。使用针对45 kDa亚型的多克隆抗体和超微结构免疫细胞化学技术,我们可以观察到宿主(Manduca sexta)表皮的渗透过程中几丁质酶的产生。几丁质酶是由表皮表面和表皮的初始渗透过程中的感染结构以极低的水平产生的,但是几丁质酶的水平在蛋白水解降解区域中积聚得多,这表明几丁质酶的释放取决于甲壳素的可及性。它的底物。

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