Detection and Practical Differentiation of Phytoplasmas from Several Host Plants Using PCR-RFLP

Kikin Mutaqin, Purnama Hidayat, Budi Tjahjono, Yayi Munara Kusumah, Rusmilah Suseno
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Abstract

Phytoplasma as a phytopathogenic prokaryote with a wide host range is a pathogen that needs more attention in Indonesia. This pathogen is relatively difficult to detect and identify due to its complicated biological properties. This study involved detection of phytoplasmas by polymerase chain reaction (PCR) technique with P1/P7 primers from seven symptomatic plants, i.e. Bermuda grass white leaf, bamboo yellows, witches’ broom of peanut, soybean, yard long bean, and cactus, and sweet potato little leaf. The phytoplasma DNA of the 16S rRNA gene resulting from PCR amplification was examined by digestion reaction using three endonuclease enzymes AluI, RSaI, and MSeI to generate restriction fragment length polymorphism (RFLP) profile. The seven diseased plants were confirmed positive to be associated with phytoplasma as indicated by the PCR product of 1800 bp. Based on the RFLP profiles of the three enzymes, the phytoplasmas were divided into two groups, namely group I (Bermuda grass and bamboo) and group II (peanuts, soybeans, yard long beans, cactus, and sweet potatoes). Cactus phytoplasma is a sub-group (strain) because it has a slightly different fragment of MSeI RFLP profile.
利用PCR-RFLP技术检测几种寄主植物的植物原体并进行实用分化
植物原体作为一种寄主范围广泛的植物致病性原核生物,在印度尼西亚是一种需要引起重视的病原体。由于其复杂的生物学特性,这种病原体的检测和鉴定相对困难。本研究利用P1/P7引物,采用聚合酶链反应(PCR)技术对百达草白叶、竹黄、花生、大豆、豇豆、仙人掌、甘薯小叶等7种对症植物的原体进行检测。采用三种酶切酶AluI、RSaI和MSeI对PCR扩增得到的植物原体16S rRNA基因进行酶切,得到限制性片段长度多态性(RFLP)图谱。结果表明,7株病株均与植物原体相关,PCR扩增结果为1800bp。根据三种酶的RFLP图谱,将植物原体分为两类,即I类(百达草和竹子)和II类(花生、大豆、豇豆、仙人掌和红薯)。仙人掌植原体是一个亚群(菌株),因为它具有稍微不同的MSeI RFLP片段。
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