4.7 Article

Target-site and non-target-site-based resistance to tribenuron-methyl in multiply-resistant Myosoton aquaticum L.

Journal

PESTICIDE BIOCHEMISTRY AND PHYSIOLOGY
Volume 155, Issue -, Pages 8-14

Publisher

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.pestbp.2018.12.004

Keywords

Acetolactate synthase (ALS); Target-site-based resistance; Non-target-site-based resistance; Resistance mechanism; Multiple herbicide resistance; Myosoton aquaticum L. (water chickweed)

Funding

  1. National Natural Science Foundation of China [31601653]
  2. Project of Shandong Province Higher Educational Science and Technology Program [J18KA134]
  3. China Postdoctoral Science Foundation [2017M612311]
  4. National Key Research and Development Plan [2016YFD0300701]
  5. Hunan Provincial Key Laboratory for Biology and Control of Weeds [2015TP-1016]
  6. Funds of Shandong Double Tops Program [SYL2017XTTD11]

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Myosoton aquaricum L., a widespread and competitive winter weed of wheat in China, has evolved resistance to many classes of herbicides. In one M. aquaticum population (AH03), collected from Anhui Province, where tribenuron-methyl and florasulam had been used to control this weed resistance to both herbicides had evolved. Compared with the sensitive population, HNO3(S), the resistant (R) population, AH03, was highly resistant to tribenuron-methyl, flucarbazone-Na and pyroxsulam, moderately resistant to pyrithiobac-sodium, and florasulam, and had low resistance to diflufenican. AH03 was still controlled by imazethapyr, 2,4-D butylate, fluroxypyr-meptyl, and isoproturon. Pretreatment with the P450 inhibitor malathion reduced the GR50 value of tribenuron-methyl by 43% in the R population, and by 25% in the S population. This indicates that P450-mediated enhanced metabolism is one likely mechanism for tribenuron-methyl resistance in M. aquaticum. Glutathione-S-transferase (GST) activity could be induced by tribenuron-methyl in both the R and S populations. However, both the basal and induced GST activity of the R population was lower than that of the S population. The in vitro ALS assay confirmed that the ALS from the R plants showed a high resistance (52.93-fold) to tribenuron-methyl. ALS gene sequencing revealed a Pro197Ala substitution in the R plants. Based on the ALS gene sequence analysis, molecular markers were also developed to identify the specific Pro197Ala mutation. This population of M. aquaticum has multiple resistance and target-site (ALS Pro197A1a) and non-target-site resistance mechanisms contribute to tribenuron-methyl resistance.

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