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Featured researches published by Cruz Avila-Adame.


Plant Disease | 2004

A Two-Phase Resistance Response of Venturia inaequalis Populations to the QoI Fungicides Kresoxim-Methyl and Trifloxystrobin

Wolfram Köller; Diana M. Parker; William W. Turechek; Cruz Avila-Adame; D. Keith Cronshaw

The class of fungicides acting as respiration inhibitors by binding to the Qo center of cyto-chrome b (QoIs) are in wide use for the management of apple scab caused by Venturia inaequalis. In order to assess responses of V. inaequalis populations to treatments with QoIs, sensitivities of isolates were determined for germinating conidia or for mycelial colonies developing from germinating conidia. Under both test conditions, inhibitory potencies of kresoxim-methyl and trifloxystrobin were largely equivalent. V. inaequalis populations treated with QoIs in a commercial and an experimental orchard both responded with significant shifts toward declining QoI sensitivities. However, the population responses were quantitative in nature, and highly resistant isolates indicative of a cytochrome b target site mutation were not detected. V. inaequalis populations from both orchards investigated also were fully resistant to sterol de-methylation-inhibiting fungicides (DMIs) such as fenarimol and myclobutanil, but isolate sensitivities to QoIs and DMIs were largely unrelated. Performance tests with kresoxim-methyl and trifloxystrobin at the experimental orchard diagnosed as DMI-resistant revealed that the quantitative shift toward declining QoI sensitivities did not constitute the status of practical QoI resistance. In contrast to these quantitative responses, emergence of qualitative QoI resistance was documented for V. inaequalis in an orchard in North Germany, which had been treated intensively with a total of 25 QoI applications over four consecutive seasons. Isolates retrieved from the orchard were highly resistant to both kresoxim-methyl and trifloxystrobin and were characterized as G143A cytochrome b mutants. The results indicated that the paths of QoI resistance can be both quantitative and qualitative in nature. A similar phenomenon has not been described before. Circumstantial evidence suggests that the quantitative phase of V. inaequalis population responses to QoIs might be succeeded by a quantitative selection of highly resistant G143A target-site mutants.


Plant Disease | 2003

Characterization of Colletotrichum graminicola Isolates Resistant to Strobilurin-Related QoI Fungicides

Cruz Avila-Adame; Gilberto Olaya; Wolfram Köller

Isolates of Colletotrichum graminicola were collected from annual bluegrass or bent grass turf in Japan and the United States, and their sensitivities to QoI fungicides (QoIs) as well as their cytochrome b sequences were characterized. Five isolates sampled from turf treated repeatedly with azoxystrobin were highly QoI resistant under both in vivo and in vitro test conditions. The nucleotide sequences of a large cytochrome b gene segment involving the binding site of QoIs were fully homologous for all resistant isolates and contained the G143A target site mutation known to confer QoI resistance in other pathogens. QoI-sensitive isolates collected prior to treatments with QoIs were more diverse with regard to their cytochrome b gene sequences and their phenotype responses to QoIs. All wild-type isolates retained a glycine in position 143 of cytochrome b. Three of the four QoI-sensitive isolates were, in addition, distinguished by leucines in positions 95, 130, and 141, which were exchanged to threonine in all resistant but also in one of the sensitive isolates. In addition to a more pronounced divergence of cytochrome b sequences, the sensitive wild-type isolates also were diverse with regard to the induction of alternative respiration in response to QoI action, as indicated by comparisons of QoI sensitivities displayed in the absence or presence of the alternative oxidase inhibitor salicylhydroxamic acid. These different phenotype responses expressed under in vitro test conditions had no or only a slight impact on anthracnose control in protective applications of azoxystrobin. Isolate responses in vitro were very similar for trifloxystrobin, indicating cross-resistance among the class of QoIs. Our results imply that C. graminicola falls into the class of pathogens with a potential for rapid selection of highly QoI-resistant phenotypes. Frequent monitoring of population sensitivities will be required to determine the status of population responses toward practical QoI resistance.


Molecular Plant-microbe Interactions | 2002

Disruption of the alternative oxidase gene in Magnaporthe grisea and its impact on host infection.

Cruz Avila-Adame; Wolfram Köller

Plants and numerous fungi including Magnaporthe grisea protect mitochondria from interference by respiration inhibitors by expressing alternative oxidase, the enzymatic core of alternative respiration. The alternative oxidase gene AOXMg of M. grisea was disrupted. Several lines of evidence suggested that the disruption of AOXMg was sufficient to completely curb the expression of alternative respiration. In the infection of barley leaves, several AOXMg-minus and, thus, alternative respiration-deficient mutants of M. grisea retained their pathogenicity without significant impairment of virulence. However, differences between the wild-type strain and an AOXMg-minus mutant were apparent under oxidative stress conditions generated by the treatment of infected barley leaves with the commercial respiration inhibitor azoxystrobin. Symptom development was effectively suppressed on leaves infected with the alternative respiration-deficient mutant, while lesions on leaves infected with the wild-type strain continued to develop at much higher inhibitor doses. However, respective lesions rarely developed to the stage of full maturity. The results did not conform to a previous model implying that expression of alternative respiration is silenced during pathogenesis by the presence of constitutive plant antioxidants. Rather, alternative respiration provided protection from azoxystrobin during both saprophytic and infectious stages of the pathogen. The nature of similar oxidative stress conditions in the ecology of M. grisea remains an open question.


Pest Management Science | 2018

Characterization of the mechanism of action of the fungicide fenpicoxamid and its metabolite UK-2A: Mechanism of action of fenpicoxamid

David Young; Nick X. Wang; Stacy T Meyer; Cruz Avila-Adame

Abstract BACKGROUND Fenpicoxamid is a new fungicide for control of Zymoseptoria tritici, and is a derivative of the natural product UK‐2A. Its mode of action and target site interactions have been investigated. RESULTS UK‐2A strongly inhibited cytochrome c reductase, whereas fenpicoxamid was much less active, consistent with UK‐2A being the fungicidally active species generated from fenpicoxamid by metabolism. Both compounds caused rapid loss of mitochondrial membrane potential in Z. tritici spores. In Saccharomyces cerevisiae, amino acid substitutions N31K, G37C and L198F at the Qi quinone binding site of cytochrome b reduced sensitivity to fenpicoxamid, UK‐2A and antimycin A. Activity of fenpicoxamid was not reduced by the G143A exchange responsible for strobilurin resistance. A docking pose for UK‐2A at the Qi site overlaid that of antimycin A. Activity towards Botrytis cinerea was potentiated by salicylhydroxamic acid, showing an ability of alternative respiration to mitigate activity. Fungitoxicity assays against Z. tritici field isolates showed no cross‐resistance to strobilurin, azole or benzimidazole fungicides. CONCLUSION Fenpicoxamid is a Qi inhibitor fungicide that provides a new mode of action for Z. tritici control. Mutational and modeling studies suggest that the active species UK‐2A binds at the Qi site in a similar, but not identical, fashion to antimycin A.


Journal of General Plant Pathology | 2003

Insertional mutagenesis of Magnaporthe grisea toward decreased responsiveness of alternative respiration to inhibition by azoxystrobin

Cruz Avila-Adame; Wolfram Köller

Abstract Inhibitors of respiration with high affinity to the Qo site of cytochrome b constitute a major class of modern agricultural fungicides. Many fungal organisms, including plant pathogens, can circumvent this inhibition site by expressing alternative respiration, a pathway dependent on alternative oxidase and other unidentified gene products. The restriction enzyme-mediated insertion (REMI) technique was employed in this study to disrupt genes involved in the expression of fully functional alternative respiration of Magnaporthe grisea. In one of the REMI mutants obtained, the rescue response mediated by alternative respiration was completely abolished. In two other mutants, the response was diminished but not entirely silenced. For all three mutants, phenotype changes were not explained by an altered structure of the alternative oxidase gene AOXMg or by a decreased level of gene expression in response to the Qo inhibitor azoxystrobin. The gene potentially affected in one of the REMI mutants was a homolog of the ABC1 family of genes encoding chaperone-like proteins with roles in the optimal assembly of mitochondrial membrane complexes.


Current Genetics | 2003

Characterization of spontaneous mutants of Magnaporthe grisea expressing stable resistance to the Qo-inhibiting fungicide azoxystrobin

Cruz Avila-Adame; Wolfram Köller


Pest Management Science | 2003

Impact of alternative respiration and target-site mutations on responses of germinating conidia of Magnaporthe grisea to Qo-inhibiting fungicides

Cruz Avila-Adame; Wolfram Köller


Archive | 2001

Resistance to Strobilurin Fungicides

Wolfram Köller; Cruz Avila-Adame; Gilberto Olaya; Desen Zheng


Archive | 2017

composições fungicidas incluindo derivados de hidrazona e cobre

Cruz Avila-Adame; David H. Young; James Ruiz; Jeffrey Dale Webster; Nneka Breaux; Steven Howard Shaber; Thomas L. Siddall


Archive | 2016

composições algicidas sinergísticas incluindo derivados de hidrazona e cobre

Cruz Avila-Adame; David Young; James Ruiz; Jeffery Webster; Nneka Breaux; Steven Howard Shaber; Thomas L. Siddall

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David H. Young

United States Forest Service

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