Trinucleotide cap analogs with triphosphate chain modifications: synthesis, properties, and evaluation as mRNA capping reagents

Author:

Warminski Marcin1,Depaix Anais2,Ziemkiewicz Kamil2,Spiewla Tomasz13,Zuberek Joanna1,Drazkowska Karolina2ORCID,Kedzierska Hanna3,Popielec Agnieszka3,Baranowski Marek R3,Sklucka Marta3,Bednarczyk Marcelina3,Smietanski Miroslaw3,Wolosewicz Karol3,Majewski Bartosz3,Serwa Remigiusz A4,Nowis Dominika35,Golab Jakub36,Kowalska Joanna13ORCID,Jemielity Jacek23ORCID

Affiliation:

1. Division of Biophysics, Institute of Experimental Physics, Faculty of Physics, University of Warsaw , Pasteura 5, 02-093 Warsaw , Poland

2. Centre of New Technologies, University of Warsaw , Banacha 2C, 02-097 Warsaw , Poland

3. Explorna Therapeutics sp. z o.o , Zwirki i Wigury 93/2157, 02-089 Warsaw , Poland

4. Proteomics Core Facility, IMol Polish Academy of Sciences , 02-247 Warsaw , Poland

5. Laboratory of Experimental Medicine, Faculty of Medicine, Medical University of Warsaw , Nielubowicza 5, 02-097 Warsaw , Poland

6. Department of Immunology, Medical University of Warsaw , Nielubowicza 5, 02-097 Warsaw , Poland

Abstract

Abstract The recent COVID-19 pandemics have demonstrated the great therapeutic potential of in vitro transcribed (IVT) mRNAs, but improvements in their biochemical properties, such as cellular stability, reactogenicity and translational activity, are critical for further practical applications in gene replacement therapy and anticancer immunotherapy. One of the strategies to overcome these limitations is the chemical modification of a unique mRNA 5′-end structure, the 5′-cap, which is responsible for regulating translation at multiple levels. This could be achieved by priming the in vitro transcription reaction with synthetic cap analogs. In this study, we combined a highly efficient trinucleotide IVT capping technology with several modifications of the 5′ cap triphosphate bridge to synthesize a series of 16 new cap analogs. We also combined these modifications with epigenetic marks (2′-O-methylation and m6Am) characteristic of mRNA 5′-ends in higher eukaryotes, which was not possible with dinucleotide caps. All analogs were compared for their effect on the interactions with eIF4E protein, IVT priming, susceptibility to decapping, and mRNA translation efficiency in model cell lines. The most promising α-phosphorothiolate modification was also evaluated in an in vivo mouse model. Unexpected differences between some of the analogs were analyzed using a protein cell extract pull-down assay.

Funder

National Science Centre, Poland

European Union

National Centre for Research and Development

Publisher

Oxford University Press (OUP)

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