Lycotoxin-1 insecticidal peptide optimized by amino acid scanning mutagenesis and expressed as a coproduct in an ethanologenic Saccharomyces cerevisiae strain

Hughes SR; Dowd PF; Hector RE; Panavas T; Sterner DE; Qureshi N; Bischoff KM; Bang SS; Mertens JA; Johnson ET

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Lycotoxin-1 insecticidal peptide optimized by amino acid scanning mutagenesis and expressed as a coproduct in an ethanologenic Saccharomyces cerevisiae strain

机译：Lycotoxin-1杀虫肽通过氨基酸扫描诱变法优化，并在产乙醇的酿酒酵母菌株中作为副产物表达

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New methods of safe biological pest control are required as a result of evolution of insect resistance to current biopesticides. Yeast strains being developed for conversion of cellulosic biomass to ethanol are potential host systems for expression of commercially valuable peptides, such as bioinsecticides, to increase the cost-effectiveness of the process. Spider venom is one of many potential sources of novel insect-specific peptide toxins. Libraries of mutants of the small amphipathic peptide lycotoxin-1 from the wolf spider were produced in high throughput using an automated integrated plasmid-based functional proteomic platform and screened for ability to kill fall armyworms, a significant cause of damage to corn (maize) and other crops in the United States. Using amino acid scanning mutagenesis (AASM) we generated a library of mutagenized lycotoxin-1 open reading frames (ORF) in a novel small ubiquitin-like modifier (SUMO) yeast expression system. The SUMO technology enhanced expression and improved generation of active lycotoxins. The mutants were engineered to be expressed at high level inside the yeast and ingested by the insect before being cleaved to the active form (so-called Trojan horse strategy). These yeast strains expressing mutant toxin ORFs were also carrying the xylose isomerase (XI) gene and were capable of aerobic growth on xylose. Yeast cultures expressing the peptide toxins were prepared and fed to armyworm larvae to identify the mutant toxins with greatest lethality. The most lethal mutations appeared to increase the ability of the toxin alpha-helix to interact with insect cell membranes or to increase its pore-forming ability, leading to cell lysis. The toxin peptides have potential as value-added coproducts to increase the cost-effectiveness of fuel ethanol bioproduction. Copyright (c) 2008 European Peptide Society and John Wiley & Sons, Ltd.

机译：由于昆虫对当前生物农药的抗性进化，需要安全的生物害虫防治新方法。正在开发用于将纤维素生物质转化为乙醇的酵母菌株是潜在的宿主系统，用于表达商业上有价值的肽（例如生物杀虫剂），以提高该方法的成本效益。蜘蛛毒是新型昆虫特异性肽毒素的许多潜在来源之一。使用自动整合的基于质粒的功能蛋白质组学平台，以高通量生产了来自狼蛛的小两亲性肽lycotoxin-1突变体的文库，并筛选了杀死秋季粘虫的能力，这是造成玉米（玉米）和玉米受损的重要原因。美国的其他农作物。使用氨基酸扫描诱变（AASM），我们在新型小型泛素样修饰子（SUMO）酵母表达系统中生成了诱变的lycotoxin-1开放阅读框（ORF）。 SUMO技术增强了活性核毒素的表达并改善了其产生。这些突变体经过改造后可以在酵母中高水平表达，并在被切割成活性形式之前被昆虫吸收（所谓的特洛伊木马策略）。这些表达突变毒素ORF的酵母菌株也携带木糖异构酶（XI）基因，并且能够在木糖上有氧生长。制备表达肽毒素的酵母培养物，并喂入粘虫幼虫中，以鉴定具有最大杀伤力的突变毒素。最致命的突变似乎增加了毒素α-螺旋与昆虫细胞膜相互作用的能力或增加了其致孔能力，从而导致细胞裂解。毒素肽具有增值副产品的潜力，可以提高燃料乙醇生物生产的成本效益。版权所有（c）2008欧洲肽协会和John Wiley＆Sons，Ltd.

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《Journal of peptide science: An official publication of the European Peptide Society》 |2008年第9期|共12页
作者
Hughes SR; Dowd PF; Hector RE; Panavas T; Sterner DE; Qureshi N; Bischoff KM; Bang SS; Mertens JA; Johnson ET;
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中图分类蛋白质的一级结构;
关键词
insecticidal peptide; amino acid scanning mutagenesis; SUMO high-level yeast expression system; fuel ethanol coproduct; ANAEROBIC XYLOSE FERMENTATION; CELL-PENETRATING PEPTIDES; BACILLUS-THURINGIENSIS; SPIDER NEUROTOXINS; CALCIUM-CHANNELS; YEAST; RESISTANCE; ISOMERASE; PLASMID; PROTEIN;

机译：杀虫肽;氨基酸扫描诱变;SUMO高级酵母表达系统;燃料乙醇副产物;厌氧木糖发酵;穿透细胞的肽;苏醒杆菌;蜘蛛神经毒素;钙离子通道;酵母;抗性;异构酶;血浆;蛋白质;

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1. Lycotoxin-1 insecticidal peptide optimized by amino acid scanning mutagenesis and expressed as a coproduct in an ethanologenic Saccharomyces cerevisiae strain [J] . Hughes SR, Dowd PF, Hector RE, Journal of peptide science: An official publication of the European Peptide Society . 2008,第9期

机译：Lycotoxin-1杀虫肽通过氨基酸扫描诱变法优化，并在产乙醇的酿酒酵母菌株中作为副产物表达
2. γ-Glutamyltransferase is not involved in the bulk uptake of amino acids, peptides or γ-glutamyl-amino acids in yeast (Saccharomyces cerevisiae) [J] . G M Payne, J W Payne The biochemical journal . 1984,第1期

机译：酵母（Saccharomyces cerevisiae）中氨基酸，肽或γ-谷氨酰胺基氨基酸的大量摄入不涉及γ-谷氨酰胺基转移酶
3. The permease homologue Ssy1p controls the expression of amino acid and peptide transporter genes in Saccharomyces cerevisiae. [J] . Didion T, Regenberg B, Jorgensen MU, Molecular Microbiology . 1998,第3期

机译：渗透酶同系物Ssy1p控制酿酒酵母中氨基酸和肽转运蛋白基因的表达。
4. Biosynthesis of amino acids sulfur in Saccharomyces cerevisiae is affected by fermentation conditions in beer production [C] . C.S. Leal-Guerra, E. Pérez-Ortega, L. Damas-Buenrostro, International Conference on Environmental, Industrial and Applied Microbiology . 2009

机译：酿酒酵母酿酒酵母中氨基酸硫的生物合成受到啤酒生产中发酵条件的影响
5. Molecular, genetic, and functional analysis of Ptr3p, a novel protein involved in amino acid and dipeptide regulation of di/tri-peptide transport system in Saccharomyces cerevisiae. [D] . Narita, Vanny. 2002

机译：Ptr3p的分子，遗传和功能分析，这是一种在酿酒酵母中涉及氨基酸和二/三肽转运系统的二肽调节的新型蛋白质。
6. gamma-Glutamyltransferase is not involved in the bulk uptake of amino acids peptides or gamma-glutamyl-amino acids in yeast (Saccharomyces cerevisiae). [O] . G M Payne, J W Payne 1984

机译：γ-谷氨酰胺基转移酶不参与酵母（酿酒酵母）中氨基酸肽或γ-谷氨酰胺基氨基酸的大量摄取。
7. The permease homologue Ssy1p controls the expression of amino acid and peptide transporter genes in Saccharomyces cerevisiae [O] . Thomas Didion, Birgitte Regenberg, Marianne U. Jorgensen, 1998

机译：允许同源物SSY1p控制酿酒酵母中氨基酸和肽转运蛋白基因的表达

Lycotoxin-1 insecticidal peptide optimized by amino acid scanning mutagenesis and expressed as a coproduct in an ethanologenic Saccharomyces cerevisiae strain

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