Development of simplified and rapid nucleic acid release protocol for PCR based detection of Potato viruses

被引:4
|
作者
Raigond, Baswaraj [1 ]
Verma, Ambika [1 ]
Kochhar, Tarvinder [1 ]
Roach, Shivani [1 ]
Sharma, Sanjeev [1 ]
Chakrabarti, S. K. [1 ]
机构
[1] ICAR Cent Potato Res Inst, Shimla 171001, India
关键词
Potato virus; Detection; Nucleic acid; Buffer; RT-PCR; Validation; PLANT-SAMPLES;
D O I
10.1007/s12600-018-0650-1
中图分类号
S3 [农学(农艺学)];
学科分类号
0901 ;
摘要
A simple, cost-effective and rapid viral nucleic acid release (NAR) buffer suitable for RT-PCR based diagnostic assay was developed for the detection of potato viruses. The NAR buffer and commercially available RNA isolation kit were compared for RT-PCR based assay, where an amplicon of expected size (similar to 380 bp) targeting PVY was observed in both isolations indicating that it can be used in RT-PCR based diagnostic assays. The same was further validated for its repeatability by running across more than hundred suspected potato leaf samples collected from different sources where, it showed consistent results for the presence of PVY indicating its reliability. The NAR buffer assay was examined for its sensitivity in comparison with the kit based isolation where both the assays were able to detect even up to 10(-5) dilution without affecting the sensitivity. NAR buffer was found stable up to 28 days at -20 degrees C and for 14 days at 4 degrees C without losing PCR sensitivity. The assay was also found effective to release the nucleic acid from potato leaves, thrips and aphids for PCR and RT-PCR based detection of DNA viruses like ToLCNDV-potato and other RNA viruses. The developed protocol is simple, less laborious, time-saving (10-15 min) and economical (1/100th of kit) as compared to kit based protocol. The assay can be adopted in diagnostic laboratories for detection of RNA/DNA viruses from potato plants and in thrips as well.
引用
收藏
页码:255 / 262
页数:8
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