A high-throughput, modified ALS activity assay for Cyperus difformis and Schoenoplectus mucronatus seedlings

Rafael M Pedroso; Kassim Al-Khatib; Bradley D Hanson; Albert J Fischer

doi:10.1016/j.pestbp.2016.06.001

A high-throughput, modified ALS activity assay for Cyperus difformis and Schoenoplectus mucronatus seedlings

Pestic Biochem Physiol. 2017 Jan:135:78-81. doi: 10.1016/j.pestbp.2016.06.001. Epub 2016 Jun 3.

Authors

Rafael M Pedroso¹, Kassim Al-Khatib², Bradley D Hanson¹, Albert J Fischer¹

Affiliations

¹ Department of Plant Sciences, University of California at Davis, Davis, CA 95616, United States.
² Department of Plant Sciences, University of California at Davis, Davis, CA 95616, United States. Electronic address: kalkhatib@ucdavis.edu.

PMID: 28043335
DOI: 10.1016/j.pestbp.2016.06.001

Abstract

Cyperus difformis L. (CYPDI) and Schoenoplectus mucronatus (L.) Palla (SCHMU) are major weeds of California (CA) rice, where resistance to acetolactate synthase (ALS)-inhibitors was identified in several CYPDI and SCHMU populations that have also evolved resistance to photosystem II (PSII)-inhibiting herbicides. The mechanism of ALS resistance in these populations remains to be clarified but this information is crucial in a weed management program, especially in a scenario where resistance to multiple herbicides has been identified. ALS activity assays are commonly used to diagnose resistance to ALS-inhibitors, but protocols currently available are burdensome for the study of CYPDI and SCHMU, as they require large amounts of plant material from young seedlings and have low yields. Our objective was to investigate the ALS resistance mechanism in suspected ALS-resistant (R) CYPDI and SCHMU biotypes using a modified ALS activity assay that requires less plant material. ALS enzymes from suspected R biotypes were at least 10,000-fold less sensitive to bensulfuron-methyl than susceptible (S) cohorts, indicating ALS resistance that is likely due to an altered target-site. Protein concentration (mgg^-1 tissue) did not differ between R and S biotypes within each species, suggesting that R biotypes do not over produce ALS enzymes. CYPDI biotypes had up to 4-fold more protein per mg of tissue than SCHMU biotypes, but up to 7-fold more acetoin per mg^-1 protein was quantified in SCHMU, suggesting greater ALS catalytic ability in SCHMU biotypes, regardless of their herbicide resistance status. Our optimized protocol to measure ALS activity allowed for up to a 3-fold increase in the number of assays performed per g of leaf tissue. The modified assay may be useful for measuring ALS activity in other weed species that also produce small amount of foliage in early growth stages when protein in tissue is most abundant.

Keywords: Acetolactate synthase; Bensulfuron-methyl; Cyperus difformis; Herbicide resistance; Oryza sativa; Schoenoplectus mucronatus.

MeSH terms

Acetolactate Synthase / metabolism*
Biological Assay
Cyperaceae / drug effects*
Cyperaceae / enzymology
Herbicide Resistance
Herbicides / toxicity*
Plant Proteins / metabolism*
Plant Weeds / drug effects
Plant Weeds / enzymology
Seedlings / drug effects*
Seedlings / enzymology
Sulfonylurea Compounds / toxicity*

Substances

Herbicides
Plant Proteins
Sulfonylurea Compounds
methyl bensulfuron
Acetolactate Synthase