中国生物防治学报
中國生物防治學報
중국생물방치학보
CHINESE JOURNAL OF BIOLOGICAL CONTROL
2014年
6期
828-833
,共6页
周洁%张艳军%谢明%贾开志
週潔%張豔軍%謝明%賈開誌
주길%장염군%사명%가개지
蜡蚧轮枝菌%DNA提取%PCR%虫生真菌
蠟蚧輪枝菌%DNA提取%PCR%蟲生真菌
사개륜지균%DNA제취%PCR%충생진균
Verticillium lecanii%DNA extraction%PCR%entomopathogenic fungi
土壤真菌分子生态学研究需要大量和高效地提取真菌的 DNA。应用市售的一般试剂盒提取土壤虫生真菌DNA,常常存在得率和质量低的问题,甚至根本提取不到土壤真菌的DNA样品。针对这一问题,本研究对细胞破碎方式及后续DNA提取参数进行了一系列的改进和优化,建立了一套针对性的提取方法。该提取法对虫生真菌—蜡蚧轮枝菌纯培养物的灵敏度极高,可在10个孢子的条件下提取到DNA,而市售的试剂盒则不能提取到(试剂盒在107个孢子条件仍提不到DNA);该提取法对人工投菌土样的DNA提取灵敏度达到102个孢子/克土,所得的DNA纯度高,无明显抑制后续PCR扩增的物质;施用过蜡蚧轮枝菌的田间土样所得 DNA 样品可成功扩增出蜡蚧轮枝菌特异片段,而未施用过蜡蚧轮枝菌的田间土样所得DNA 样品不能扩增出蜡蚧轮枝菌特异片段。本提取方法具有灵敏度和纯度高的特点,适用于土壤虫生真菌的分子生态学样品制备。
土壤真菌分子生態學研究需要大量和高效地提取真菌的 DNA。應用市售的一般試劑盒提取土壤蟲生真菌DNA,常常存在得率和質量低的問題,甚至根本提取不到土壤真菌的DNA樣品。針對這一問題,本研究對細胞破碎方式及後續DNA提取參數進行瞭一繫列的改進和優化,建立瞭一套針對性的提取方法。該提取法對蟲生真菌—蠟蚧輪枝菌純培養物的靈敏度極高,可在10箇孢子的條件下提取到DNA,而市售的試劑盒則不能提取到(試劑盒在107箇孢子條件仍提不到DNA);該提取法對人工投菌土樣的DNA提取靈敏度達到102箇孢子/剋土,所得的DNA純度高,無明顯抑製後續PCR擴增的物質;施用過蠟蚧輪枝菌的田間土樣所得 DNA 樣品可成功擴增齣蠟蚧輪枝菌特異片段,而未施用過蠟蚧輪枝菌的田間土樣所得DNA 樣品不能擴增齣蠟蚧輪枝菌特異片段。本提取方法具有靈敏度和純度高的特點,適用于土壤蟲生真菌的分子生態學樣品製備。
토양진균분자생태학연구수요대량화고효지제취진균적 DNA。응용시수적일반시제합제취토양충생진균DNA,상상존재득솔화질량저적문제,심지근본제취불도토양진균적DNA양품。침대저일문제,본연구대세포파쇄방식급후속DNA제취삼수진행료일계렬적개진화우화,건립료일투침대성적제취방법。해제취법대충생진균—사개륜지균순배양물적령민도겁고,가재10개포자적조건하제취도DNA,이시수적시제합칙불능제취도(시제합재107개포자조건잉제불도DNA);해제취법대인공투균토양적DNA제취령민도체도102개포자/극토,소득적DNA순도고,무명현억제후속PCR확증적물질;시용과사개륜지균적전간토양소득 DNA 양품가성공확증출사개륜지균특이편단,이미시용과사개륜지균적전간토양소득DNA 양품불능확증출사개륜지균특이편단。본제취방법구유령민도화순도고적특점,괄용우토양충생진균적분자생태학양품제비。
It is required to efficiently extract large quantity and high quality of fungal DNA for the soil fungal molecular ecological study. However, the yield and quality of DNA are often insufficient or even no any product can be produced by the commercial DNA extraction kit. To solve these problems, the cell lysis and subsequent DNA extraction parameters were optimized in this study, and then an efficient method of extracting soil fungal DNA was established. The results showed this method was very sensitive to entomopathogenic fungi Verticillium lecanii. DNA could be extracted from the pure culture samples which contained more than 10 spores, and the artificial soil samples which contained more than 100 spores per gram soil. However commercial DNA extraction kits are unable to extract DNA from the pure culture samples which contained 107 spores. The DNA product from our method did not show any obvious inhibition in the subsequent PCR amplification, and was proved to be high-pure by the OD260/280 value. DNA could be also extracted from - two natural soil samples,but the target sequence fragment specific for V. lecanii was only amplified from one natural soil sample applied with V. lecanii. In conclusion, this soil DNA extraction method is sensitive to entomopathogenic fungi and DNA products were high-pure, so it was suitable for the DNA preparation in soil entomopathogenic fungal molecular ecological research.
