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利用携带潮霉素B抗性基因的微小盾壳霉研究核盘菌菌核在土壤中的存活和侵染情况。

Use of Coniothyrium minitans transformed with the hygromycin B resistance gene to study survival and infection of Sclerotinia sclerotiorum sclerotia in soil.

作者信息

Jones E Eirian, Stewart Alison, Whipps John M

机构信息

Horticulture Research International, Wellesbourne, Warwick, CV35 9EF, UK.

出版信息

Mycol Res. 2003 Mar;107(Pt 3):267-76. doi: 10.1017/s0953756203007457.

Abstract

A Coniothyrium minitans strain (T3) co-transformed with the genes for beta-glucuronidase (uidA) and hygromycin phosphotransferase (hph), the latter providing resistance to the antibiotic hygromycin B, was used to investigate the survival and infection of sclerotia of Sclerotinia sclerotiorum by C. minitans over time in four different soils. Infection of sclerotia was rapid in all cases, with the behaviour of transformant T3 and wild type parent A69 being similar. Differences were seen between the soils in the rate of infection of sclerotia by C. minitans and in their indigenous fungal populations. Amendment of agar with hygromycin B enabled the quantification of C. minitans in soil by dilution plating where there was a high background of other microorganisms. In Lincoln soil from New Zealand, which had a natural but low population of C. minitans, the hygromycin B resistance marker allowed the umambiguous discrimination of the applied transformed isolate from the indigenous hygromycin B sensitive one. In this soil, although the indigenous C. minitans population was detected from sclerotia, none were recovered on the dilution plates, indicating the increased sensitivity of C. minitans detection from soil using sclerotial baiting. C. minitans was a very efficient parasite, being able to infect a large proportion of sclerotia within a relatively short time from an initially low soil population. The addition of hygromycin B to agar also allowed the detection of C. minitans from decaying sclerotia by inhibiting secondary fungal colonisers. This is the first report to show that fungi colonising sclerotia already infected by C. minitans mask the detection of C. minitans from sclerotia rather than displacing the original parasite.

摘要

将编码β-葡萄糖醛酸酶(uidA)和潮霉素磷酸转移酶(hph)的基因共转化的微小盾壳霉菌株(T3)用于研究微小盾壳霉在四种不同土壤中随时间对核盘菌菌核的存活和侵染情况,其中潮霉素磷酸转移酶赋予对潮霉素B的抗性。在所有情况下,菌核的侵染都很快,转化体T3和野生型亲本A69的表现相似。不同土壤中微小盾壳霉对菌核的侵染率及其本地真菌种群存在差异。在其他微生物背景较高的情况下,用潮霉素B改良琼脂能够通过稀释平板法对土壤中的微小盾壳霉进行定量。在新西兰的林肯土壤中,微小盾壳霉的自然种群数量较低,潮霉素B抗性标记使得能够明确区分所施用的转化菌株和本地对潮霉素B敏感的菌株。在这种土壤中,虽然从菌核中检测到了本地微小盾壳霉种群,但在稀释平板上未分离到任何菌株,这表明使用菌核诱饵法从土壤中检测微小盾壳霉的灵敏度有所提高。微小盾壳霉是一种非常有效的寄生菌,能够在相对较短的时间内从最初较低土壤种群中侵染很大比例的菌核。向琼脂中添加潮霉素B还能通过抑制次生真菌定殖者从腐烂菌核中检测到微小盾壳霉。这是第一份表明定殖在已被微小盾壳霉感染的菌核上的真菌会掩盖从菌核中检测微小盾壳霉的现象,而不是取代原来的寄生菌的报告。

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