Identification and immobilization of a novel cold-adapted esterase, and its potential for bioremediation of pyrethroid-contaminated vegetables

Xinjiong Fan; Weiqu Liang; Yanfang Li; He Li; Xiaolong Liu

doi:10.1186/s12934-017-0767-9

Identification and immobilization of a novel cold-adapted esterase, and its potential for bioremediation of pyrethroid-contaminated vegetables

Microb Cell Fact. 2017 Sep 11;16(1):149. doi: 10.1186/s12934-017-0767-9.

Authors

Xinjiong Fan¹, Weiqu Liang², Yanfang Li², He Li³, Xiaolong Liu⁴

Affiliations

¹ School of Basic Medical Sciences, Anhui Medical University, 81 Meishan Rd, Hefei, 230032, Anhui, People's Republic of China.
² Dongguan Agriculture Research Center, Dongguan, 523079, Guangdong, People's Republic of China.
³ School of Basic Courses, Guangdong Pharmaceutical University, 280 E. Outer Ring Rd., Guangzhou, 510006, Guangdong, People's Republic of China.
⁴ School of Basic Medical Sciences, Anhui Medical University, 81 Meishan Rd, Hefei, 230032, Anhui, People's Republic of China. liuxiaolong85@126.com.

Abstract

Background: Pyrethroids are potentially harmful to living organisms and ecosystems. Thus, concerns have been raised about pyrethroid residues and their persistence in agricultural products. To date, although several pyrethroid-hydrolyzing enzymes have been cloned, very few reports are available on pyrethroid-hydrolyzing enzymes with cold adaptation, high hydrolytic activity and good reusability, indispensable properties in practical bioremediation of pyrethroid-contaminated vegetables.

Results: Here, a novel gene (est684) encoding pyrethroid-hydrolyzing esterase was isolated from the Mao-tofu metagenome for the first time. Est684 encoded a protein of 227 amino acids and was expressed in Escherichia coli BL21 (DE3) in soluble form. The optimum temperature was 18 °C. It maintained 46.1% of activity at 0 °C and over 50% of its maximal activity at 4-35 °C. With the goal of enhancing stability and recycling biocatalysts, we used mesoporous silica SBA-15 as a nanometer carrier for the efficient immobilization of Est684 by the absorption method. The best conditions were an esterase-to-silica ratio of 0.96 mg/g (w/w) and an adsorption time of 30 min at 10 °C. Under these conditions, the recovery of enzyme activity was 81.3%. A large improvement in the thermostability of Est684 was achieved. The half-life (T_1/2) of the immobilized enzyme at 35 °C was 6 h, 4 times longer than the soluble enzyme. Interestingly, the immobilized Est684 had less loss in enzyme activity up to 12 consecutive cycles, and it retained nearly 54% of its activity after 28 cycles, indicating excellent operational stability. Another noteworthy characteristic was its high catalytic activity. It efficiently hydrolyzed cyhalothrin, cypermethrin, and fenvalreate in pyrethroid-contaminated cucumber within 5 min, reaching over 85% degradation efficiency after four cycles.

Conclusions: A novel cold-adapted pyrethroid-hydrolyzing esterase was screened from the Mao-tofu metagenome. This report is the first on immobilizing pyrethroid-hydrolyzing enzyme on mesoporous silica. The immobilized enzyme with high hydrolytic activity and outstanding reusability has a remarkable potential for bioremediation of pyrethroid-contaminated vegetables, and it is proposed as an industrial enzyme.

Keywords: Bioremediation; Esterase; Immobilization; Pyrethroid; Reusability; Vegetables.

MeSH terms

Biodegradation, Environmental*
Cloning, Molecular
Cold Temperature
Cucumis sativus
Enzyme Stability
Enzymes, Immobilized / chemistry
Enzymes, Immobilized / metabolism*
Esterases / chemistry
Esterases / genetics
Esterases / metabolism*
Food Contamination*
Half-Life
Hydrogen-Ion Concentration
Hydrolysis
Pesticide Residues / metabolism*
Pyrethrins / metabolism*
Silicon Dioxide
Substrate Specificity
Temperature
Vegetables*

Substances

Enzymes, Immobilized
Pesticide Residues
Pyrethrins
SBA-15
cypermethrin
Silicon Dioxide
Esterases