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定量聚合酶链反应(QPCR)分析和RNA干扰(RNAi)确定了大豆胞囊线虫与宿主初始相互作用所需的咽腺细胞表达基因。

QPCR analysis and RNAi define pharyngeal gland cell-expressed genes of Heterodera glycines required for initial interactions with the host.

作者信息

Bakhetia M, Urwin P E, Atkinson H J

机构信息

Centre for Plant Sciences, University of Leeds, Leeds LS2 9JT, UK.

出版信息

Mol Plant Microbe Interact. 2007 Mar;20(3):306-12. doi: 10.1094/MPMI-20-3-0306.

Abstract

Changes in transcript abundance of genes expressed in the three pharyngeal gland cells of Heterodera glycines after host invasion were monitored by quantitative polymerase chain reaction (qPCR) and the consequences of disrupting their expression studied by RNAi treatment prior to invasion. Two transcripts were known to be expressed in the two subventral gland cells (hg-pel and hg-eng-1), a further two in the single dorsal gland cell only (hg-gp and hg-syv46), and a fifth transcript (hg-cm) was expressed by both gland cell types. The qPCR study established that transcripts of hg-syv46 and hg-gp increased in abundance by 2 days postinfection (dpi), with the former remaining the most abundant. The hg-cm transcript level showed minor changes from 0 to 14 dpi but did fall by 21 dpi. In contrast, hg-eng-1 and hg-eng-2 messenger (m)RNA declined by 7 dpi and hg-pel by 14 dpi before it increased at 21 dpi. RNAi-targeting of hg-eng-1 reduced the number of females present on the plants at 10 days. Targeting of hg-gp, hg-cm, and hg-pel caused a change in sexual fate favoring male development on roots. Both effects were evident after targeting hg-syv46. Suppression of hg-eng-1 mRNA levels in second-stage juveniles (J2i) by RNAi was transient, with a recovery by 15 days of incubation in water after treatment. Presoaking H. glycines J2 with double-stranded RNA has value for studying gene function during the nematode's early interaction with a plant.

摘要

通过定量聚合酶链反应(qPCR)监测大豆胞囊线虫(Heterodera glycines)宿主入侵后在三个咽腺细胞中表达的基因转录本丰度变化,并在入侵前通过RNA干扰处理研究破坏其表达的后果。已知两个转录本在两个亚腹侧腺细胞中表达(hg-pel和hg-eng-1),另外两个仅在单个背侧腺细胞中表达(hg-gp和hg-syv46),第五个转录本(hg-cm)由两种腺细胞类型表达。qPCR研究表明,感染后2天(dpi),hg-syv46和hg-gp的转录本丰度增加,前者仍是最丰富的。hg-cm转录本水平在0至14 dpi之间变化较小,但在21 dpi时确实下降。相比之下,hg-eng-1和hg-eng-2信使(m)RNA在7 dpi时下降,hg-pel在14 dpi时下降,然后在21 dpi时增加。靶向hg-eng-1的RNA干扰在10天时减少了植物上的雌虫数量。靶向hg-gp、hg-cm和hg-pel导致性命运发生变化,有利于根上的雄性发育。靶向hg-syv46后,这两种效应都很明显。通过RNA干扰抑制二期幼虫(J2i)中hg-eng-1 mRNA水平是短暂的,处理后在水中孵育15天可恢复。用双链RNA预浸泡大豆胞囊线虫J2对于研究线虫与植物早期相互作用期间的基因功能具有价值。

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