Engineered phage with antibacterial CRISPR-Cas selectively reduce E. coli burden in mice.

Yılmaz Emre Gençay ,Joana Carvalho,Džiuginta Jasinskytė,Katja Chandelle Johansen,Eric Van Der Helm,Iszabela Cristiana Turcu,Ricardo Pascal,Lene Jessen,Jasper Clube,Frenk Smrekar,Alice Troy,Anders Østergaard Petersen,Jonas Hink,Aurelie Gram,Mette Grove,Ana De Santiago Torio,Thea Staffeldt Schou,Morten Otto Alexander Sommer,Lone Bayer,Virginia Martínez,Michael J Satlin,Lev Koval,Szabolcs Semsey,Tina Bryde,Emilie Glad Bak,Melissa Kviesgaard Eriksen,K T Brunner ,Björn M Hallström ,C Grøndahl ,Timothy B Doyle ,Jakob Haaber ,Birgitte Bentz Damholt ,Milan Zdravković ,Adam M Takos ,Alex N Salazar ,Caroline Robert

doi:10.1038/s41587-023-01759-y

Yılmaz Emre Gençay , Joana Carvalho + Show 34 more

Open Access

https://doi.org/10.1038/s41587-023-01759-y

Copy DOI

Abstract

Antibiotic treatments have detrimental effects on the microbiome and lead to antibiotic resistance. To develop a phage therapy against a diverse range of clinically relevant Escherichia coli, we screened a library of 162 wild-type (WT) phages, identifying eight phages with broad coverage of E. coli, complementary binding to bacterial surface receptors, and the capability to stably carry inserted cargo. Selected phages were engineered with tail fibers and CRISPR-Cas machinery to specifically target E. coli. We show that engineered phages target bacteria in biofilms, reduce the emergence of phage-tolerant E. coli and out-compete their ancestral WT phages in coculture experiments. A combination of the four most complementary bacteriophages, called SNIPR001, is well tolerated in both mouse models and minipigs and reduces E. coli load in the mouse gut better than its constituent components separately. SNIPR001 is in clinical development to selectively kill E. coli, which may cause fatal infections in hematological cancer patients.

Full Text