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筛选非丝状细菌生产角质降解酶。

Screening of nonfilamentous bacteria for production of cutin-degrading enzymes.

机构信息

Plant Science Research Unit, Eastern Regional Research Center, Agricultural Research Service, U.S. Department of Agriculture, Philadelphia, Pennsylvania 19118.

出版信息

Appl Environ Microbiol. 1992 Jul;58(7):2123-30. doi: 10.1128/aem.58.7.2123-2130.1992.

Abstract

Two hundred thirty-two nonfilamentous bacterial strains, including saprophytes, plant pathogens, and opportunistic plant and human pathogens, were screened for the ability to produce cutinases (cutin-degrading esterases). Initially, esterase activity of culture filtrates of strains grown in nutrient broth-yeast extract medium supplemented with 0.4% apple or tomato cutin was determined by a spectrophotometric assay utilizing the model substrate p-nitrophenyl butyrate. The culture filtrates of the 10 Pseudomonas aeruginosa strains tested exhibited the highest esterase activity, with values of >500 nmol/min/ml. Of these 10 strains, 3 (K799, 1499A, and DAR41352) demonstrated significant induction (10-fold or above) of esterase activity by addition of cutin to nutrient broth-yeast extract medium. The ability of culture filtrates of the three strains to cause release of apple cutin monomers was confirmed by a novel high-performance liquid chromatography technique. Monomer identification was confirmed by gas chromatography-mass spectroscopy analyses. Addition of the nonionic detergent n-octylglucoside stimulated cutinase activity of culture filtrates from strains K799 and DAR41352, but not that of filtrates from strain 1499A. Time course studies in nutrient broth-yeast extract medium supplemented with apple cutin indicated maximal levels of cutinase in the culture fluids after cultures entered stationary phase. Incubation temperatures below the optimal temperature for growth (37 degrees C) led to maximal production of cutinase.

摘要

二百三十二株非丝状细菌菌株,包括腐生菌、植物病原体和机会性植物和人类病原体,被筛选出产生角质酶(角质降解酯酶)的能力。最初,通过利用模型底物对硝基苯丁酸酯的分光光度测定法,测定在补充有 0.4%苹果或番茄角质的营养肉汤-酵母提取物培养基中生长的菌株的培养滤液中的酯酶活性。测试的 10 株铜绿假单胞菌菌株的培养滤液表现出最高的酯酶活性,其值> 500 nmol/min/ml。在这 10 株菌株中,有 3 株(K799、1499A 和 DAR41352)通过在营养肉汤-酵母提取物培养基中添加角质显著诱导(10 倍或更高)酯酶活性。通过新型高效液相色谱技术证实了这三株菌株的培养滤液能够引起苹果角质单体的释放。通过气相色谱-质谱分析确认了单体的鉴定。添加非离子洗涤剂辛基葡萄糖苷刺激了 K799 和 DAR41352 菌株的培养滤液中的角质酶活性,但不刺激 1499A 菌株的滤液中的角质酶活性。在补充有苹果角质的营养肉汤-酵母提取物培养基中的时间过程研究表明,在培养物进入静止期后,培养物中的角质酶达到最高水平。低于生长最佳温度(37 摄氏度)的孵育温度导致角质酶的最大产量。

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