Literature DB >> 26131741

Co-selection and replacement of resistance alleles to Lysinibacillus sphaericus in a Culex quinquefasciatus colony.

Karlos Diogo de Melo Chalegre1, Daniella A Tavares1, Tatiany P Romão1, Heverly Suzany G de Menezes1, Nathaly A Nascimento1, Cláudia Maria F de Oliveira1, Osvaldo P de-Melo-Neto2, Maria Helena N L Silva-Filha1.   

Abstract

The Cqm1 α-glucosidase, expressed within the midgut of Culex quinquefasciatus mosquito larvae, is the receptor for the Binary toxin (Bin) from the entomopathogen Lysinibacillus sphaericus. Mutations of the Cqm1 α-glucosidase gene cause high resistance levels to this bacterium in both field and laboratory populations, and a previously described allele, cqm1REC, was found to be associated with a laboratory-resistant colony (R2362). This study described the identification of a novel resistance allele, cqm1REC-2, that was co-selected with cqm1REC within the R2362 colony. The two alleles display distinct mutations but both generate premature stop codons that prevent the expression of midgut-bound Cqm1 proteins. Using a PCR-based assay to monitor the frequency of each allele during long-term maintenance of the resistant colony, cqm1REC was found to predominate early on but later was replaced by cqm1REC-2 as the most abundant resistance allele. Homozygous larvae for each allele were then generated that displayed similar high-resistance phenotypes with equivalent low levels of transcript and lack of protein expression for both cqm1REC and cqm1REC-2. In progeny from a cross of homozygous individuals for each allele at a 1 : 1 ratio, analyzed for ten subsequent generations, cqm1REC showed a higher frequency than cqm1REC-2. The replacement of cqm1REC by cqm1REC -2 observed in the R2362 colony, kept for 210 generations, indicates changes in fitness related to traits that are unknown but linked to these two alleles, and constitutes a unique example of evolution of resistance within a controlled laboratory environment.
© 2015 FEBS.

Entities:  

Keywords:  Binary toxin; allele replacement; cqm1 alleles; receptors; α-glucosidases

Mesh:

Substances:

Year:  2015        PMID: 26131741     DOI: 10.1111/febs.13364

Source DB:  PubMed          Journal:  FEBS J        ISSN: 1742-464X            Impact factor:   5.542


  4 in total

1.  Functional Bacillus thuringiensis Cyt1Aa Is Necessary To Synergize Lysinibacillus sphaericus Binary Toxin (Bin) against Bin-Resistant and -Refractory Mosquito Species.

Authors:  Nathaly Alexandre Nascimento; Mary Carmen Torres-Quintero; Samira López Molina; Sabino Pacheco; Tatiany Patrícia Romão; Antonio Pereira-Neves; Mario Soberón; Alejandra Bravo; Maria Helena Neves Lobo Silva-Filha
Journal:  Appl Environ Microbiol       Date:  2020-03-18       Impact factor: 4.792

2.  A differential transcriptional profile by Culex quinquefasciatus larvae resistant to Lysinibacillus sphaericus IAB59 highlights genes and pathways associated with the resistance phenotype.

Authors:  Tatiana Maria Teodoro Rezende; Antonio Mauro Rezende; Gabriel Luz Wallau; Crhisllane Rafaele Santos Vasconcelos; Osvaldo Pompílio de-Melo-Neto; Maria Helena Neves Lobo Silva-Filha; Tatiany Patrícia Romão
Journal:  Parasit Vectors       Date:  2019-08-20       Impact factor: 3.876

Review 3.  Bacterial Toxins Active against Mosquitoes: Mode of Action and Resistance.

Authors:  Maria Helena Neves Lobo Silva-Filha; Tatiany Patricia Romão; Tatiana Maria Teodoro Rezende; Karine da Silva Carvalho; Heverly Suzany Gouveia de Menezes; Nathaly Alexandre do Nascimento; Mario Soberón; Alejandra Bravo
Journal:  Toxins (Basel)       Date:  2021-07-27       Impact factor: 4.546

4.  A new allele conferring resistance to Lysinibacillus sphaericus is detected in low frequency in Culex quinquefasciatus field populations.

Authors:  Heverly Suzany Gouveia Menezes; Karlos Diogo de Melo Chalegre; Tatiany Patrícia Romão; Cláudia Maria Fontes Oliveira; Osvaldo Pompílio de-Melo-Neto; Maria Helena Neves Lobo Silva-Filha
Journal:  Parasit Vectors       Date:  2016-02-04       Impact factor: 3.876

  4 in total

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