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检测及其在其昆虫媒介烟盲蝽(半翅目:盲蝽科)中变化的 aster yellows 植原体浓度。

Detection and variability of aster yellows phytoplasma titer in its insect vector, Macrosteles quadrilineatus (Hemiptera: Cicadellidae).

机构信息

Department of Plant Pathology, University of Wisconsin-Madison, 1630 Linden Drive, Madison, WI 53706, USA.

出版信息

J Econ Entomol. 2011 Dec;104(6):1800-15. doi: 10.1603/ec11183.

DOI:10.1603/ec11183
PMID:22299339
Abstract

The aster yellows phytoplasma (AYp) is transmitted by the aster leafhopper, Macrosteles quadrilineatus Forbes, in a persistent and propagative manner. To study AYp replication and examine the variability of AYp titer in individual aster leafhoppers, we developed a quantitative real-time polymerase chain reaction assay to measure AYp concentration in insect DNA extracts. Absolute quantification of AYp DNA was achieved by comparing the amplification of unknown amounts of an AYp target gene sequence, elongation factor TU (tuf), from whole insect DNA extractions, to the amplification of a dilution series containing known quantities of the tuf gene sequence cloned into a plasmid. The capabilities and limitations of this method were assessed by conducting time course experiments that varied the incubation time of AYp in the aster leafhopper from 0 to 9 d after a 48 h acquisition access period on an AYp-infected plant. Average AYp titer was measured in 107 aster leafhoppers and, expressed as Log10 (copies/insect), ranged from 3.53 (+/- 0.07) to 6.26 (+/- 0.11) occurring at one and 7 d after the acquisition access period. AYp titers per insect and relative to an aster leafhopper chromosomal reference gene, cp6 wingless (cp6), increased approximately 100-fold in insects that acquired the AYp. High quantification cycle values obtained for aster leafhoppers not exposed to an AYp-infected plant were interpreted as background and used to define a limit of detection for the quantitative real-time polymerase chain reaction assay. This method will improve our ability to study biological factors governing AYp replication in the aster leafhopper and determine if AYp titer is associated with frequency of transmission.

摘要

黄化曲叶植原体(AYp)通过蔓叶甲,Macrosteles quadrilineatus Forbes,以持久和增殖的方式传播。为了研究 AYp 的复制,并检查个体蔓叶甲中 AYp 滴度的变异性,我们开发了一种定量实时聚合酶链反应测定法,以测量昆虫 DNA 提取物中的 AYp 浓度。通过比较从整个昆虫 DNA 提取物中扩增未知数量的 AYp 靶基因序列伸长因子 TU(tuf),与包含克隆到质粒中的 tuf 基因序列的已知数量稀释系列的扩增,实现了 AYp DNA 的绝对定量。通过进行时间过程实验评估了该方法的能力和局限性,该实验改变了 AYp 在蔓叶甲中的孵育时间,从 48 小时获取访问期后在 AYp 感染植物上的 0 到 9 天不等。在 107 只蔓叶甲中测量了平均 AYp 滴度,以 Log10(拷贝/昆虫)表示,范围从 3.53(+/-0.07)到 6.26(+/-0.11),分别发生在获取访问期后 1 天和 7 天。每只昆虫的 AYp 滴度与蔓叶甲染色体参考基因 cp6 无翅(cp6)相比,在获得 AYp 的昆虫中增加了约 100 倍。未暴露于 AYp 感染植物的蔓叶甲获得的高定量循环值被解释为背景,并用于定义定量实时聚合酶链反应测定法的检测限。该方法将提高我们研究 AYp 在蔓叶甲中复制的生物学因素的能力,并确定 AYp 滴度是否与传播频率相关。

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