Plastidic <i>ACCase</i> Ile-1781-Leu is present in pinoxaden-resistant southern crabgrass (<i>Digitaria ciliaris</i>)

Basak, S. L.; McElroy, J. Scott; Brown, Austin M.; Gonçalves, Clebson Gomes; Patel, Jinesh; McCullough, Patrick E.

doi:10.1017/wsc.2019.56

Cited by 12 publications

(21 citation statements)

References 54 publications

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“…Both traditional Sanger sequencing from PCR and next generation sequencing are important for understanding the plant gene family. Previously, researchers have found that PCR‐based amplification may not be sufficient to reveal all target‐site resistance mutations 31, 32 . Here, we demonstrated that it is equally important to validate sequencing data from RNA‐seq by standard PCR, so that: (i) computational errors could be checked and corrected; and (ii) the nucleotide diversity of different individuals/populations, not limited to the few plants with transcriptome data, can be revealed.…”

Section: Discussionmentioning

confidence: 85%

Diversity of α‐tubulin transcripts in Lolium rigidum

Chen

Chu

Han

et al. 2020

Pest Management Science

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BACKGROUND Tubulin, the target site of dinitroaniline herbicides, is encoded by small gene families in plants. To better characterize the mechanisms of target‐site resistance to dinitroaniline herbicides in the globally important weedy species Lolium rigidum, attempts were made to amplify and sequence α‐tubulin transcripts. RESULTS Four α‐tubulin isoforms (TUA1, TUA2, TUA3 and TUA4) were identified in L. rigidum. Variations in the number and sequence of transcripts encoding these α‐tubulin proteins were found in individuals from the two L. rigidum populations examined. Within and among populations, differences in the 5′‐ and 3′‐untranslated regions of cDNA in TUA3 and TUA4 were identified. Furthermore, a novel double mutation, Arg‐390‐Cys+Asp‐442‐Glu, in the TUA3 transcript was identified and has the potential to confer dinitroaniline resistance. CONCLUSION This research reveals the complexity of the α‐tubulin gene family in individuals/populations of the cross‐pollinated weedy species L. rigidum, and highlights the need for better understanding of the molecular architecture of tubulin gene families for detecting resistance point mutations. Although TUA4 is a commonly expressed α‐tubulin isoform containing most frequently reported resistance mutations, other mutant tubulin isoforms may also have a role in conferring dinitroaniline resistance.

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Section: Discussionmentioning

confidence: 85%

Diversity of α‐tubulin transcripts in Lolium rigidum

Chen

Chu

Han

et al. 2020

Pest Management Science

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“…Basak et al. (2020) also reported difficulty with PCR‐based sequencing of the ACCase CT domain coding region in southern crabgrass. The application of more advanced approaches such as next generation sequencing may be required for these species.…”

Section: Resultsmentioning

confidence: 99%

Characterization of mutations conferring inherent resistance to acetyl coenzyme A carboxylase‐inhibiting herbicides in turfgrass and grassy weeds

Tate

McCullough

Harrison³

et al. 2021

Crop Science

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An herbicide‐resistant weed control system that utilizes naturally occurring mutations to acetyl‐coenzyme A carboxylase (ACCase)‐inhibiting herbicides could provide herbicide selectivity and improve control of grassy weeds in turf. Knowledge regarding the presence of these mutations in grasses is needed to guide development of this type of system. This research subjected 24 species of warm‐season, cool‐season, and grassy weed species to rates of 0, 400, and 1200 g a.i. ha−1 of fenoxaprop herbicide and surveyed these species for the presence of site‐of‐action mutations in ACCase at amino acid (aa) positions 1781, 1999, 2027, 2041, 2076, 2088, and 2096. Nine species including Agrostis capillaris L., Festuca ovina L., Festuca rubra L., Lolium multiflorum Lam., Lolium perenne L., Paspalum dilatatum Poir., Poa annua L., Zoysia japonica Steud., and Z. matrella [L.] Merr. were tolerant to fenoxaprop. Site of action point mutations conferring resistance to ACCase herbicides were found at aa position 1781 in only three of 24 species surveyed (Festuca ovina, Festuca rubra, and Poa annua). The information obtained from this study provide guidance for the development of ACCase resistant weed control systems for turfgrass.

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“…Previously collected seeds of two resistant biotypes (R1 and R2) of D. ciliaris with confirmed resistance to select ACCase-targeting herbicides and one susceptible (S) biotype were included in this study (Basak et al 2019;Yu et al 2017). To generate green plant material for enzyme extraction, seeds of resistant and susceptible D. ciliaris biotypes were sown in separate plastic flats containing commercial potting soil and peat moss (2:1 v/v).…”

Section: Seed Sample Collection and Growth Conditionsmentioning

confidence: 99%

“…This result can only be because of differential interaction with the ACCase substrate and the tested ACCase-targeting herbicide, as no absorption, translocation, or metabolism is at play as would be the case when screening whole plants. The ACCase carboxyl transferase domains were sequenced and reported for S, R1, and R2 previously (Basak et al 2019). No other amino acid substitutions except Ile-1781-Leu were observed between R1 or R2 that would explain the difference between these biotypes (Supplementary Data 2).…”

Section: Research Implicationsmentioning

confidence: 99%

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Detecting the effect of ACCase-targeting herbicides on ACCase activity utilizing a malachite green colorimetric functional assay

et al. 2021

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Research was conducted to evaluate acetyl-Coenzyme A carboxylase (ACCase) enzyme activity using a functional malachite green colorimetric assay previously identified as resistant to sethoxydim, and select aryloxyphenoxypropionate (FOPs) herbicides, fenoxaprop, and fluazifop. Two resistant southern crabgrass [Digitaria ciliaris (Retz.) Koeler] biotypes, R1 and R2, containing an Ile-1781-Leu amino acid substitution and previously identified as resistant to sethoxydim, pinoxaden, and fluazifop but not clethodim was utilized as the resistant chloroplastic ACCase source compared to known susceptible (S) ACCase. Dose-response studies with sethoxydim, clethodim, fluazifop-p-butyl, and pinoxaden (0.6 to 40 µM) were conducted to compare the ACCase enzyme-herbicides interaction of R1, R2, and S using the malachite green functional assay. Assay results indicated that R biotypes required more ACCase-targeting herbicides to inhibit ACCase activity compared to S. IC50 values of all four herbicides for R biotypes were consistently an order of magnitude greater than S. No sequencing differences in the carboxyltransferase domain was observed for R1 and R2, however, R2 IC50 values were greater across all herbicides. These results indicate the malachite green functional assay is effective in evaluating ACCase enzyme activity of R and S biotypes in the presence of ACCase-targeting herbicides, which can be used as a replacement for the 14C-based radiometric functional assay.

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Plastidic ACCase Ile-1781-Leu is present in pinoxaden-resistant southern crabgrass (Digitaria ciliaris)

Cited by 12 publications

References 54 publications

Diversity of α‐tubulin transcripts in Lolium rigidum

Diversity of α‐tubulin transcripts in Lolium rigidum

Characterization of mutations conferring inherent resistance to acetyl coenzyme A carboxylase‐inhibiting herbicides in turfgrass and grassy weeds

Detecting the effect of ACCase-targeting herbicides on ACCase activity utilizing a malachite green colorimetric functional assay

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