AI Article Synopsis

  • The study investigates the presence of recombinant Spike protein in individuals vaccinated with mRNA-based SARS-CoV-2 vaccines, using a mass spectrometry approach to detect specific protein fragments.
  • Results showed that a specific Spike protein fragment was found in 50% of biological samples from vaccinated individuals, irrespective of antibody levels, with detection occurring between 69 and 187 days post-vaccination.
  • This novel proteomic method helps evaluate the half-life of Spike protein and supports ongoing monitoring of vaccine efficacy, especially concerning additional booster doses.

Article Abstract

Purpose: The SARS-CoV-2 pandemic prompted the development and use of next-generation vaccines. Among these, mRNA-based vaccines consist of injectable solutions of mRNA encoding for a recombinant Spike, which is distinguishable from the wild-type protein due to specific amino acid variations introduced to maintain the protein in a prefused state. This work presents a proteomic approach to reveal the presence of recombinant Spike protein in vaccinated subjects regardless of antibody titer.

Experimental Design: Mass spectrometry examination of biological samples was used to detect the presence of specific fragments of recombinant Spike protein in subjects who received mRNA-based vaccines.

Results: The specific PP-Spike fragment was found in 50% of the biological samples analyzed, and its presence was independent of the SARS-CoV-2 IgG antibody titer. The minimum and maximum time at which PP-Spike was detected after vaccination was 69 and 187 days, respectively.

Conclusions And Clinical Relevance: The presented method allows to evaluate the half-life of the Spike protein molecule "PP" and to consider the risks or benefits in continuing to administer additional booster doses of the SARS-CoV-2 mRNA vaccine. This approach is of valuable support to complement antibody level monitoring and represents the first proteomic detection of recombinant Spike in vaccinated subjects.

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Source
http://dx.doi.org/10.1002/prca.202300048DOI Listing

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