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在培养过程中添加蛋白酶 K 会改变苏云金芽孢杆菌培养物的生理学特性以及 cry1Ac、nprX、nprA 和 spo0A 基因的转录。

Addition of proteinase K during the culture alter the physiology of Bacillus thuringiensis culture and the cry1Ac, nprX, nprA, and spo0A gene transcription.

机构信息

Instituto de Biotecnología, Universidad del Papaloapan, Circuito Central 200, Parque Industrial, 68301, Tuxtepec, Oaxaca, México.

División de Estudios de Posgrado, Doctorado en Biotecnología, Universidad del Papaloapan, Circuito Central 200, Parque Industrial, 68301, Tuxtepec, Oaxaca, México.

出版信息

Antonie Van Leeuwenhoek. 2022 Jan;115(1):89-102. doi: 10.1007/s10482-021-01683-8. Epub 2021 Nov 19.

Abstract

Bacillus thuringiensis is the major bioinsecticide worldwide produced due to the Cry protein activity. Several studies have been done to improve the cost-productivity relation. The neutral protease A (NprA) is the major extracellular protein massively produced during the stationary phase by this bacterium, contributing to the Cry proteins' degradation. Also, the deletion of aprA and nprA genes enhanced the yield of Cry protein, stabilizing it. Therefore, to increase Cry production, one possibility is to degrade the NprA protease in the culture media. In the present study, proteinase K was used to hydrolyze the NprA to increase Cry production. Proteinase K was added during the exponential growth of B. thuringiensis culture. The bacilli and endospores were measured along all culture, while the Cry protein was measured at the end of the culture. The addition of PK affects the bacilli and spore kinetics positively but negatively to the Cry protein (there is no Cry protein detection). Therefore, the gene expression of the cry1Ac, nprX, nprA, and spo0A was measured. The expression of each gene was followed along all culture. Results demonstrated that PK alters both the transcriptional levels and the expression order of the genes.

摘要

苏云金芽孢杆菌是世界上主要的生物杀虫剂,因其 Cry 蛋白活性而产生。已经进行了多项研究来提高成本效益关系。中性蛋白酶 A(NprA)是该细菌在静止期大量产生的主要细胞外蛋白,有助于 Cry 蛋白的降解。此外,aprA 和 nprA 基因的缺失提高了 Cry 蛋白的产量,使其稳定。因此,为了增加 Cry 蛋白的产量,可以将 NprA 蛋白酶在培养基中降解。在本研究中,使用蛋白酶 K 水解 NprA 以增加 Cry 蛋白的产量。在苏云金芽孢杆菌培养物的指数生长期添加蛋白酶 K。在整个培养过程中测量杆菌和芽孢,在培养结束时测量 Cry 蛋白。PK 的添加对杆菌和芽孢动力学有积极影响,但对 Cry 蛋白有负面影响(未检测到 Cry 蛋白)。因此,测量了 cry1Ac、nprX、nprA 和 spo0A 的基因表达。在整个培养过程中都跟踪了每个基因的表达情况。结果表明,PK 改变了基因的转录水平和表达顺序。

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