Identification and recombinant expression of an antimicrobial peptide (cecropin B-like) from soybean pest Anticarsia gemmatalis

被引:0
作者
Costa Ramos, Luis Felipe [1 ]
de Oliveira Rangel, Joao Henrique [1 ]
Andrade, Guilherme Caldas [1 ]
Lixa, Carolina [1 ]
Araujo de Castilho, Livia Vieira [1 ,2 ]
Sousa Nogueira, Fabio Cesar [1 ]
Pinheiro, Anderson S. [1 ]
Gomes, Fabio Mendonca [3 ]
AnoBom, Cristiane Dinis [1 ]
Perpetua de Oliveira, Danielle Maria [1 ]
Almeida, Rodrigo Volcan [1 ]
机构
[1] Fed Univ Rio de Janeiro UFRJ, Ctr Math & Nat Sci, Inst Chem, Dept Biochem, Rio De Janeiro, RJ, Brazil
[2] Fed Univ Rio de Janeiro UFRJ, Alberto Luiz Coimbra Inst Grad Studies & Res COPP, Rio De Janeiro, RJ, Brazil
[3] Fed Univ Rio de Janeiro UFRJ, Carlos Chagas Filho Inst Biophys, Rio De Janeiro, RJ, Brazil
关键词
Antimicrobial peptides; Cecropin B; Heterologous expression; Anticarsia gemmatalis; Agricultural pest; ESCHERICHIA-COLI; CDNA CLONING; PLUTELLA-XYLOSTELLA; BOMBYX-MORI; PROTEINS; INSECT; PURIFICATION; LARVAE; SUSCEPTIBILITY; MECHANISMS;
D O I
10.1590/1678-9199-JVATITD-2020-0127
中图分类号
R99 [毒物学(毒理学)];
学科分类号
100405 ;
摘要
Background: Insects can be found in numerous diverse environments, being exposed to pathogenic organisms like fungi and bacteria. Once these pathogens cross insect physical barriers, the innate immune system operates through cellular and humoral responses. Antimicrobial peptides are small molecules produced by immune signaling cascades that develop an important and generalist role in insect defenses against a variety of microorganisms. In the present work, a cecropin B-like peptide (AgCecropB) sequence was identified in the velvetbean caterpillar Anticarsia gemmatalis and cloned in a bacterial plasmid vector for further heterologous expression and antimicrobial tests. Methods: AgCecropB sequence (without the signal peptide) was cloned in the plasmid vector pET-M30-MBP and expressed in the Escherichia coli BL21(DE3) expression host. Expression was induced with IPTG and a recombinant peptide was purified using two affinity chromatography steps with Histrap column. The purified peptide was submitted to high-resolution mass spectrometry (HRMS) and structural analyses. Antimicrobial tests were performed using gram-positive (Bacillus thuringiensis) and gram-negative (Burkholderia kururiensis and E. coli) bacteria. Results: AgCecropB was expressed in E. coli BL21 (DE3) at 28 degrees C with IPTG 0.5 mM. The recombinant peptide was purified and enriched after purification steps. HRMS confirmed AgCrecropB molecular mass (4.6 kDa) and circular dichroism assay showed alpha-helix structure in the presence of SDS. AgCrecropB inhibited almost 50% of grampositive B. thuringiensis bacteria growth. Conclusions: The first cecropin B-like peptide was described in A. gemmatalis and a recombinant peptide was expressed using a bacterial platform. Data confirmed tertiary structure as predicted for the cecropin peptide family. AgCecropB was capable to inhibit B. thuringiensis growth in vitro.
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页数:12
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