Grover A, Azmi W, Paul Khurana S M, Chakrabarti S K
Central Potato Research Institute, Shimla 171001, Himachal Pradesh, India.
Lett Appl Microbiol. 2009 Nov;49(5):539-43. doi: 10.1111/j.1472-765X.2009.02687.x. Epub 2009 Jul 15.
To develop a reliable and sensitive protocol for detection of Ralstonia solanacearum using MDA-PCR (Multiple displacement amplification-PCR amplification).
MDA-PCR technique was performed on pure cell lysates as well as soil samples. Pure cell lysate as well as that of soil DNA was used as template in MDA reaction. MDA of template DNA was carried out in the presence of sample buffer, reaction buffer and enzyme mix (Phi 29 DNA polymerase and random hexamers). The MDA amplified DNA was used for PCR amplification using R. solanacearum -specific PCR primers. MDA-PCR could detect as low as 1 colony forming unit (CFU ml(-1)) of bacteria within 8 h including DNA isolation.
MDA followed by standard PCR facilitated the detection of pathogen from very low count samples. The method is of great importance in managing the brown rot disease of potato.
The ultrasensitive detection technique developed in the present study is sensitive and speedy enough to be included into integrated wilt disease control programmes.
开发一种可靠且灵敏的使用多重置换扩增 - 聚合酶链反应(MDA - PCR)检测青枯雷尔氏菌的方法。
对纯细胞裂解物以及土壤样本进行MDA - PCR技术操作。纯细胞裂解物以及土壤DNA用作MDA反应的模板。模板DNA的MDA反应在样品缓冲液、反应缓冲液和酶混合物(Phi 29 DNA聚合酶和随机六聚体)存在的情况下进行。MDA扩增的DNA使用青枯雷尔氏菌特异性PCR引物进行PCR扩增。MDA - PCR在8小时内(包括DNA提取)能够检测到低至1个菌落形成单位(CFU ml(-1))的细菌。
MDA之后进行标准PCR有助于从极低数量的样本中检测病原体。该方法在马铃薯青枯病防治中具有重要意义。
本研究开发的超灵敏检测技术灵敏且快速,足以纳入枯萎病综合防治计划。
