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作 者:崔凯杰 侯瑞[2] 袁大祥 周然[2] 葛艳辉[3] 王晓丽[3] 胡杰辉
机构地区:[1]天津市滨海新区环境保护监测站,天津300457 [2]交通运输部天津水运工程科学研究所水路交通环境保护技术交通行业重点实验室,天津300456 [3]天津理工大学环境科学与安全工程学院,天津300384
出 处:《天津理工大学学报》2017年第3期55-60,共6页Journal of Tianjin University of Technology
基 金:国家国际科技合作专项项目(2015DFA90250);国家自然科学青年基金(21307045);天津市滨海新区塘沽科技发展资金(2012STHB04-03)
摘 要:采集天津渤海湾滩涂沉积物,以原油为唯一碳源富集原油降解菌群.采用三种不同细菌DNA提取试剂盒提取原油降解菌总DNA,结果显示New Probe细菌基因组DNA小量提取试剂盒提取出的细菌总DNA质量和纯度最理想.通过对PCR体系中引物量、模板量和PCR程序中退火温度、循环数的优化,确定优化的PCR条件为:25μL Master、3μL DNA模板、1μL Primer-1、1μL Primer-2、20μLdd H_2O.扩增程序为:94℃预变性4 min;94℃变性1 min、55℃退火1 min、72℃延伸1 min,25个循环;72℃延伸6 min.原油降解菌的DGGE指纹图谱分析表明原油降解菌群的群落结构相对稳定,没有出现明显的减弱趋势.As the sole carbon source, crude oil was used to enrich oil-degrading bacteria from the sediment in Tianjin Habor. Total oil-degrading bacteriaDNA was extracted by three kinds of DNA extraction kits. The results demonstrated that the most ideal quality and purity of total DNA were obtained by New Probe bacterial genome DNA extraction kit. Optimized condition of polymerase chain reaction ( PCR ), which ensured via the optimization of primer quantity, template quantity, annealing temperature,and cycles in PCR program,was as the following. 25μL Master,3 μL DNA template, 1 μL Primer-1, 1 μL Primer-2,20 μLddH20. PCR amplification contain the initial denaturation at 94 ℃ for 4 min, then 25 cycles were executed: denaturation at 94 ℃ for 1 min,anneal at 55 ℃ for 1 min,elongation at 72 ℃ for lmin. After the 25 cycles,a final elongation was excuted at 72 ℃ for 6min. The analysis to PCR-DGGE fingerprintingof oil-degrading bacteria revealed that the community structure of oil-degrading bacteria was relatively stable and showed no significantly reducing tendency.
关 键 词:石油降解菌群 原油 DNA提取 PCR—DGGE
分 类 号:X55[环境科学与工程—环境工程]
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