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农业环境科学学报 2005

土壤微生物分子生态学研究中总DNA的提取

Keywords: 土壤DNA提取,DNA质量,PCR扩增,限制性片段长度多态性分析,温度梯度凝胶电泳分析

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Abstract:

建立了一种土壤DNA提取方法。根据DNA产量和纯度2个评价指标,从3种手提土壤DNA方法中优选出方法B为手提DNA方法(Labmethod),它包括样品预处理,细胞裂解,粗DNA纯化,其中细胞裂解组合了玻璃珠击打,SDS裂解,溶菌酶裂解。进一步应用PCR-限制性片段长度多态性(Restrictionfragmentlengthpolymorphism,RFLP)技术及PCR-温度梯度凝胶电泳(Temperaturegradientgelelectrophoresis,TGGE)技术,结合DNA产量、纯度、片段大小以及所反映的微生物群落结构特性等指标评价了手提方法(Labmethod)得到的总DNA质量,并将这些结果与2种应用较广的商业试剂盒(MoBioUltraCleanSoilDNAKit和Bio101FastDNASPINKit(ForSoil))所得DNA的各种指标进行了比较。结果表明,手提方法(Labmethod)的粗DNA产量低于Bio101Kit的,但高于MoBioKit的。这些方法所得DNA的长度都在21kb左右,Labmethod提取的DNA没有严重被剪切现象,而2种试剂盒提取的DNA都有不同程度的剪切。手提方法得到的DNA经纯化后,应用细菌及真菌特异引物进行PCR扩增,均能获得目的片段,表明该方法能从土壤中同时有效提取细菌和真菌总基因组DNA。并且,手提方法所得DNA的细菌16SrDNA和真菌18SrDNA的PCR-RFLP图谱与两种商业试剂盒的图谱基本相似,但3种方法提取

References

[1]	Amann R I, Ludwig W, Schleifer K H. Phylogenetic identification and in situ detection of individual microbial cells without cultivation [J]. Microbiol Rev, 1995, 59: 143-169.
[2]	Pace N R. A molecular view of microbial diversity and the biosphere[J].Science, 1997, 276: 734-740.
[3]	Frostegard A, Courtois S, Ramisse V, et al. Quantification of bias related to the extraction of DNA directly from soils [J]. Appl Envir Microbiol,1999, 65: 5409-5420.
[4]	Krsek M, Wellington E M H. Comparison of different methods for the isolation and purification of total community DNA from soil[J]. J Microbiol Meth, 1999, 39: 1-16.
[5]	Martin-Laurent F, Philippot L, Hallet S, et al. DNA extraction from soils: Old bias for new microbial diversity analysis methods [J]. Appl Envir Microbiol, 2001, 67: 2354-2359.
[6]	Di Cello F, Bevivino A, Chiarini L, et al. Biodiversity of a Burkholderia cepacia population isolated from the maize rhizosphere at different plant growth stages[J]. Appl Envir Microbiol, 1997, 63: 4485-4493.
[7]	Muyzer G, De Waal E C, Uitterlinden A G. Profiling of complex microbial populations by denaturing gradient gel electrophoresis analysis of polymerase chain reaction-amplified genes coding for 16S rRNA [J].Appl Environ Microbiol, 1993, 59: 695-700.
[8]	Vainio E J, Hantula J. Direct analysis of wood-inhabiting fungi using denaturing gradient gel electrophoresis of amplified ribosomal DNA [J].Mycol Res, 2000, 104: 927-936.
[9]	Sandhu G S, Kline B C, Stockman L, et al. Molecular probes for diagnosis of fungal infections[J]. J Clin Microbiol, 1995, 33: 2913-2919.
[10]	陈敏,赵立平.焦化废水处理系统中用不同培养基分离的细菌种群多样性[J].微生物学报,2003,43(3):366-371.
[11]	Zhou J, Brouns M A, Tiedje J M. DNA recovery from soils of diverse composition[J]. Appl Envir Microbiol, 1996, 62:316-322.
[12]	Lamontagne M G, Michel F C, Holden P A, et al. Evaluation of extraction and purification methods for obtaining PCR-ampli-fiable DNA from compost for microbial community analysis [J]. J Microbiol Meth,2002, 49: 255-264.
[13]	Miller D N, Bryant J E, Madsen E L, et al. Evaluation and optimization of DNA extraction and purification procedures for soil and sediment samples[J]. Appl Envir Microbiol, 1999, 65: 4715-4724.

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