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一种用于测定小菜蛾酯酶活性的连续分光光度法测定。

A continuous spectrophotometric assay for the determination of diamondback moth esterase activity.

作者信息

He Xiaodun

机构信息

Beneficial Insects Research Unit, KSARC, Agricultural Research Service, U. S. Department of Agriculture, Weslaco, Texas 78596, USA.

出版信息

Arch Insect Biochem Physiol. 2003 Oct;54(2):68-76. doi: 10.1002/arch.10103.

Abstract

Conventional methods to determine esterase activity from insects are composed of a three-step process where the enzyme is allowed to hydrolyze a 1-naphthyl acetate substrate, that reaction is quenched by a SDS detergent, and then a Fast Blue B dye complex is formed with 1-naphthol, the product of 1-naphthyl acetate hydrolysis. These methods measure dye-product complex rather than the product, 1-naphthol. A new assay is presented that continuously monitors the formation of 1-naphthol with the hydrolysis of an esterase substrate. The esterase activity was determined as the slope of the linear regression change in absorbance over time at 320 nm. The continuous assay provides a simple, rapid, and sensitive method for measuring esterases extracted from a single diamondback moth in 1-10 min. The detection limit of the assay is approximately 0.6 microM 1-naphthol. The 1-naphthol product from the esterase reaction was confirmed by HPLC analysis. According to the assay, the K(m) and V(max) values of the esterase were 28 +/- 2 microM and 6.0 +/- 0.1 microM/min, respectively, at 37 degrees C for 1-naphthyl acetate. The K(i) value was 9 +/- 2 microM using azadirachtin, an insecticide from neem tree, Azadirachta indica (A.Juss). Azadirachtin was a reversible competitive inhibitor of the esterase activity.

摘要

测定昆虫酯酶活性的传统方法由三个步骤组成

首先让酶水解乙酸 - 1 - 萘酯底物,然后用SDS去污剂终止该反应,接着乙酸 - 1 - 萘酯水解产物1 - 萘酚与固蓝B染料形成复合物。这些方法测量的是染料 - 产物复合物而非产物1 - 萘酚。本文介绍了一种新的测定方法,该方法可随着酯酶底物的水解持续监测1 - 萘酚的形成。酯酶活性通过在320 nm处吸光度随时间的线性回归变化斜率来确定。这种连续测定法为测量从单只小菜蛾中提取的酯酶提供了一种简单、快速且灵敏的方法,可在1 - 10分钟内完成。该测定法的检测限约为0.6微摩尔/升1 - 萘酚。酯酶反应产生的1 - 萘酚产物通过高效液相色谱分析得到证实。根据该测定法,在37℃下,酯酶对乙酸 - 1 - 萘酯的米氏常数(K(m))和最大反应速度(V(max))分别为28±2微摩尔/升和6.0±0.1微摩尔/(升·分钟)。使用印楝树(Azadirachta indica (A.Juss))中的杀虫剂印楝素时,其抑制常数(K(i))为9±2微摩尔/升。印楝素是酯酶活性的可逆竞争性抑制剂。

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