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六氯丁二烯降解菌株粘质沙雷氏菌HL1的鉴定及降解特性研究

Identification and degradation characterization of hexachlorobutadiene degrading strain Serratia marcescens HL1.

作者信息

Li M T, Hao L L, Sheng L X, Xu J B

机构信息

Department of Environmental Science and Engineering, Northeast Normal University, Changchun 130024, PR China.

出版信息

Bioresour Technol. 2008 Oct;99(15):6878-84. doi: 10.1016/j.biortech.2008.01.048. Epub 2008 Mar 11.

DOI:10.1016/j.biortech.2008.01.048
PMID:18337093
Abstract

A bacterium (strain HL1) capable of growing with hexachlorobutadiene (HCBD) as sole carbon and energy sources was isolated from a mixture of soil contaminated with HCBD and activated sludge obtained from petrochemical plant wastewater treatment plant by using enrichment culture. Biochemical characteristics and phylogenetic analysis based on 16S rDNA sequence indicate that strain HL1 clearly belongs to Serratia marcescens sp. Resting cells of strain HL1 were found to remove HCBD from culture fluids with the concomitant release of chloride ion under aerobic conditions. The ranges of pH value and temperature for satisfactory growth of strain HL1 cells were from 7.0 to 8.0 and 25 to 30 degrees C, respectively. Capability of resting cells to degrade HCBD was induced by HCBD in the culture fluids. HCBD (20mg/l) was removed from culture fluids by resting cells in 4 d without lag phase, but for 50mg/l and 80mg/l HCBD 7 days were needed with lag phase. Growth of strain HL1 cells was inhibited by HCBD at the concentration up to 160mg/l. First order kinetics could be fitted to the biodegradation of HCBD by HL1 cells after lag phase at initial concentrations of 20, 50, and 80mg/l. Strain HL1 also showed strong capacity to degrade chloroprene, trichloroethylene, tetrachloroethylene, and vinyl chloride at solely initial concentration of 50mg/l. Results could offer useful information for the application of strain HL1 in bioremediation or control of HCBD-polluted environment.

摘要

通过富集培养,从受六氯丁二烯(HCBD)污染的土壤与石化厂废水处理厂活性污泥的混合物中分离出一种能够以六氯丁二烯作为唯一碳源和能源生长的细菌(菌株HL1)。基于16S rDNA序列的生化特性和系统发育分析表明,菌株HL1明显属于粘质沙雷氏菌。发现在有氧条件下,菌株HL1的静止细胞能够从培养液中去除HCBD,并伴随氯离子的释放。菌株HL1细胞生长的适宜pH值范围为7.0至8.0,适宜温度范围为25至30摄氏度。培养液中的HCBD可诱导静止细胞降解HCBD的能力。静止细胞在4天内可从培养液中去除20mg/l的HCBD,无延迟期,但对于50mg/l和80mg/l的HCBD,需要7天且有延迟期。浓度高达160mg/l的HCBD会抑制菌株HL1细胞的生长。在初始浓度为20、50和80mg/l时,延迟期后HL1细胞对HCBD的生物降解符合一级动力学。菌株HL1在初始浓度仅为50mg/l时,对氯丁二烯、三氯乙烯、四氯乙烯和氯乙烯也表现出很强的降解能力。这些结果可为菌株HL1在生物修复或控制HCBD污染环境中的应用提供有用信息。

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