A reverse genetics system for avian coronavirus infectious bronchitis virus based on targeted RNA recombination

Steven J van Beurden; Alinda J Berends; Annika Krämer-Kühl; Dieuwertje Spekreijse; Gilles Chénard; Hans-Christian Philipp; Egbert Mundt; Peter J M Rottier; M Hélène Verheije

doi:10.1186/s12985-017-0775-8

A reverse genetics system for avian coronavirus infectious bronchitis virus based on targeted RNA recombination

Virol J. 2017 Jun 12;14(1):109. doi: 10.1186/s12985-017-0775-8.

Authors

Steven J van Beurden¹, Alinda J Berends¹, Annika Krämer-Kühl², Dieuwertje Spekreijse³, Gilles Chénard³, Hans-Christian Philipp², Egbert Mundt², Peter J M Rottier¹, M Hélène Verheije⁴

Affiliations

¹ Faculty of Veterinary Medicine, Department of Pathobiology, Utrecht University, Yalelaan 1, 3584 CL, Utrecht, The Netherlands.
² Boehringer Ingelheim Veterinary Research Center GmbH & Co. KG, Bemeroder Str. 31, 30559, Hannover, Germany.
³ Boehringer Ingelheim Animal Health Operations, C.J. van Houtenlaan 36, 1381 CP, Weesp, The Netherlands.
⁴ Faculty of Veterinary Medicine, Department of Pathobiology, Utrecht University, Yalelaan 1, 3584 CL, Utrecht, The Netherlands. m.h.verheije@uu.nl.

Abstract

Background: Avian coronavirus infectious bronchitis virus (IBV) is a respiratory pathogen of chickens that causes severe economic losses in the poultry industry worldwide. Major advances in the study of the molecular biology of IBV have resulted from the development of reverse genetics systems for the highly attenuated, cell culture-adapted, IBV strain Beaudette. However, most IBV strains, amongst them virulent field isolates, can only be propagated in embryonated chicken eggs, and not in continuous cell lines.

Methods: We established a reverse genetics system for the IBV strain H52, based on targeted RNA recombination in a two-step process. First, a genomic and a chimeric synthetic, modified IBV RNA were co-transfected into non-susceptible cells to generate a recombinant chimeric murinized (m) IBV intermediate (mIBV). Herein, the genomic part coding for the spike glycoprotein ectodomain was replaced by that of the coronavirus mouse hepatitis virus (MHV), allowing for the selection and propagation of recombinant mIBV in murine cells. In the second step, mIBV was used as the recipient. To this end a recombination with synthetic RNA comprising the 3'-end of the IBV genome was performed by introducing the complete IBV spike gene, allowing for the rescue and selection of candidate recombinants in embryonated chicken eggs.

Results: Targeted RNA recombination allowed for the modification of the 3'-end of the IBV genome, encoding all structural and accessory genes. A wild-type recombinant IBV was constructed, containing several synonymous marker mutations. The in ovo growth kinetics and in vivo characteristics of the recombinant virus were similar to those of the parental IBV strain H52.

Conclusions: Targeted RNA recombination allows for the generation of recombinant IBV strains that are not able to infect and propagate in continuous cell lines. The ability to introduce specific mutations holds promise for the development of rationally designed live-attenuated IBV vaccines and for studies into the biology of IBV in general.

Keywords: Avian coronavirus; Chicken; Embryonated eggs; Infectious bronchitis virus; Mouse hepatitis virus; Poultry; Reverse genetics system; Targeted RNA recombination; Vaccine development.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cell Line
Chickens
Gene Targeting / methods
Infectious bronchitis virus / genetics*
Infectious bronchitis virus / growth & development*
Mice
RNA, Viral / genetics*
Recombination, Genetic*
Reverse Genetics / methods*

Substances

RNA, Viral