4.6 Article

Identification of Helicoverpa armigera promoters for biotechnological applications

Journal

INSECT BIOCHEMISTRY AND MOLECULAR BIOLOGY
Volume 142, Issue -, Pages -

Publisher

PERGAMON-ELSEVIER SCIENCE LTD
DOI: 10.1016/j.ibmb.2022.103725

Keywords

Midgut promoters; U6 promoters; RNAi; CRISPR

Funding

  1. Institute of Molecular Biology and Biotechnology (IMBB/FORTH)
  2. Bayer Crop Sciences (Monheim, Germany)
  3. European Union (European Social Fund-ESF) through the Operational Programme 'Human Resources Development, Education and Lifelong Learning' [MIS-5000432]
  4. State Scholarships Foundation (IKY)

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This study identified functional RNA polymerase II and III promoters in Helicoverpa zea, which can be used for genetic manipulation in the context of agricultural biotechnology. Furthermore, four U6 promoters of H. armigera were also identified and evaluated, showing their potential for methodologies such as RNAi and CRISPR/Cas9.
Helicoverpa armigera and Helicoverpa zea are highly polyphagous major agricultural pests with a global distribution. Their control is based on insecticides, however, new, effective, and environmentally friendly control tools are required to be developed and validated. In an effort to facilitate the development of advanced biotechnological tools in these species that will take advantage of new powerful molecular biology techniques like CRISPR/ Cas9, we used available transcriptomic data and literature resources, in order to identify RNA polymerase II and III promoters active in RP-HzGUT-AW1(MG), a midgut derived cell line from Helicoverpa zea. Following functional analysis in insect cell lines, four RNA polymerase II promoters from the genes HaLabial, HaTsp-2A, HaPtx-I and HaCaudal were found to exhibit high transcriptional activity in vitro. The HaTsp-2A promoter did not exhibit any activity in the non-midgut derived cell lines Sf-9 and Hi-5 despite high sequence conservation among Lepidoptera, suggesting that it may function in a gut specific manner. Furthermore, considering the utility of RNA polymerase III U6 promoters in methodologies such as RNAi and CRISPR/Cas9, we identified and evaluated four different U6 promoters of H. armigera. In vitro experiments based on luciferase and GFP reporter assays, as well as in vivo experiments targeting an essential gene of Helicoverpa, indicate that these U6 promoters are functional and can be used to experimentally silence or knockout target genes through the expression of shRNAs and sgRNAs respectively. Taking our findings together, we provide a set of promoters useful for the genetic manipulation of Helicoverpa species, that can be used in various applications in the context of agricultural biotechnology.

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