Nature Communications (Jul 2024)

Engineered reversible inhibition of SpyCatcher reactivity enables rapid generation of bispecific antibodies

  • Christian Hentrich,
  • Mateusz Putyrski,
  • Hanh Hanuschka,
  • Waldemar Preis,
  • Sarah-Jane Kellmann,
  • Melissa Wich,
  • Manuel Cavada,
  • Sarah Hanselka,
  • Victor S. Lelyveld,
  • Francisco Ylera

DOI
https://doi.org/10.1038/s41467-024-50296-y
Journal volume & issue
Vol. 15, no. 1
pp. 1 – 15

Abstract

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Abstract The precise regulation of protein function is essential in biological systems and a key goal in chemical biology and protein engineering. Here, we describe a straightforward method to engineer functional control into the isopeptide bond-forming SpyTag/SpyCatcher protein ligation system. First, we perform a cysteine scan of the structured region of SpyCatcher. Except for two known reactive and catalytic residues, none of these mutations abolish reactivity. In a second screening step, we modify the cysteines with disulfide bond-forming small molecules. Here we identify 8 positions at which modifications strongly inhibit reactivity. This inhibition can be reversed by reducing agents. We call such a reversibly inhibitable SpyCatcher “SpyLock”. Using “BiLockCatcher”, a genetic fusion of wild-type SpyCatcher and SpyLock, and SpyTagged antibody fragments, we generate bispecific antibodies in a single, scalable format, facilitating the screening of a large number of antibody combinations. We demonstrate this approach by screening anti-PD-1/anti-PD-L1 bispecific antibodies using a cellular reporter assay.