Whole Genome Sequencing Analysis of Cellulose-degrading Bacterium DC11 Isolated from Silkworm Excrement and Characterization of Its Key Cellulase Gene ytoP

IF 1.1 3区 农林科学 Q3 ENTOMOLOGY Journal of Asia-pacific Entomology Pub Date : 2024-07-06 DOI:10.1016/j.aspen.2024.102285
Yuanhao Zhang , Hao Li , Minqi Zhang , Xueping Jiang , Chen Chen , Xiaohui Zhang , Ran Zhang , Gaiqun Huang , Gang Liu , Zhongzheng Gui
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Abstract

In recent years, the microbial degradation of cellulose has emerged in addressing environmental pollution and acting as a substitute for scarce animal feeds. This study conducted a whole-genome sequencing analysis of a cellulose-degrading bacterium known as Bacillus subtilis DC11, previously isolated from the silkworm excrement. A critical cellulase gene was identified, namely ytoP. The ytoP gene was successfully cloned and expressed in E.coli using genetic engineering. ytoP is a segment of the endoglucanase gene in Bacillus subtilis DC11 and was found to be 1074 bp in size and encoded 357 amino acids. This study effectively constructed the cellulase expression vector and achieved successful expression of the ytoP gene from strain DC11 in E. coli BL21 (DE3). SDS-PAGE electrophoresis revealed that the protein had an approximate size range of 40–50 KDa and a concentration of around 3.675 mg/mL. An assay of enzyme activity demonstrated that the purified protein, with a concentration of approximately 100 μg/mL, exhibited a maximum activity of 12.980 U/mL. Through the integration of whole-genome sequencing and genetic engineering techniques, the critical cellulase gene ytoP from Bacillus subtilis DC11 has been successfully cloned and expressed, achieving highly efficient cellulase production. This study lays the foundation for large-scale applications of microbial cellulose degradation in the future.

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纤维素降解菌 DC11 的全基因组测序分析及其关键纤维素酶基因 ytoP 的特性分析
近年来,微生物降解纤维素在解决环境污染和替代稀缺动物饲料方面崭露头角。本研究对一种名为枯草芽孢杆菌 DC11 的纤维素降解菌进行了全基因组测序分析。研究发现了一个关键的纤维素酶基因,即 ytoP。ytoP 是枯草芽孢杆菌 DC11 内切葡聚糖酶基因的一个片段,大小为 1074 bp,编码 357 个氨基酸。本研究有效地构建了纤维素酶表达载体,并成功地在大肠杆菌 BL21 (DE3) 中表达了菌株 DC11 的 ytoP 基因。SDS-PAGE 电泳显示,该蛋白的大小范围约为 40-50 KDa,浓度约为 3.675 mg/mL。酶活性测定表明,纯化蛋白的浓度约为 100 μg/mL,最大活性为 12.980 U/mL。通过整合全基因组测序和基因工程技术,成功克隆并表达了枯草芽孢杆菌 DC11 的关键纤维素酶基因 ytoP,实现了纤维素酶的高效生产。这项研究为今后微生物降解纤维素的大规模应用奠定了基础。
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来源期刊
Journal of Asia-pacific Entomology
Journal of Asia-pacific Entomology Agricultural and Biological Sciences-Insect Science
CiteScore
2.70
自引率
6.70%
发文量
152
审稿时长
69 days
期刊介绍: The journal publishes original research papers, review articles and short communications in the basic and applied area concerning insects, mites or other arthropods and nematodes of economic importance in agriculture, forestry, industry, human and animal health, and natural resource and environment management, and is the official journal of the Korean Society of Applied Entomology and the Taiwan Entomological Society.
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