Characterization of emergent toxigenic M1UK Streptococcus pyogenes and associated sublineages

Author:

Li Ho Kwong12ORCID,Zhi Xiangyun12ORCID,Vieira Ana12ORCID,Whitwell Harry J.34,Schricker Amelia5,Jauneikaite Elita67,Li Hanqi2,Yosef Ahmed2,Andrew Ivan8,Game Laurence8,Turner Claire E.9,Lamagni Theresa107,Coelho Juliana107,Sriskandan Shiranee172ORCID

Affiliation:

1. MRC Centre for Molecular Bacteriology & Infection (CMBI), Imperial College London, London, UK

2. Department of Infectious Disease, Imperial College London, London, UK

3. Department of Metabolism, Digestion and Reproduction, Imperial College London, London, UK

4. National Phenome Centre and Imperial Clinical Phenotyping Centre, Department of Metabolism, Digestion and Reproduction, Imperial College London, London, UK

5. UK Dementia Research Institute, Department of Brain Sciences, Imperial College London, London, UK

6. School of Public Health, Imperial College London, London, UK

7. NIHR Health Protection Unit in Healthcare-associated Infection and Antimicrobial Resistance, Imperial College London, London, UK

8. Genomics Facility, UKRI-MRC London Institute for Medical Sciences (LMS), Imperial College London, London, UK

9. The Florey Institute, School of Biosciences, University of Sheffield, South Yorkshire, UK

10. Centre for Infections, UK Health Security Agency, London, UK

Abstract

Streptococcus pyogenes genotype emm1 is a successful, globally distributed epidemic clone that is regarded as inherently virulent. An emm1 sublineage, M1UK, that produces increased levels of SpeA toxin was associated with increased scarlet fever and invasive infections in England in 2015/2016. Defined by 27 SNPs in the core genome, M1UK is now dominant in England. To more fully characterize M1UK, we undertook comparative transcriptomic and proteomic analyses of M1UK and contemporary non-M1UK emm1 strains (M1global). Just seven genes were differentially expressed by M1UK compared with contemporary M1global strains. In addition to speA, five genes in the operon that includes glycerol dehydrogenase were upregulated in M1UK (gldA, mipB/talC, pflD, and phosphotransferase system IIC and IIB components), while aquaporin (glpF2) was downregulated. M1UK strains have a stop codon in gldA. Deletion of gldA in M1global abrogated glycerol dehydrogenase activity, and recapitulated upregulation of gene expression within the operon that includes gldA, consistent with a feedback effect. Phylogenetic analysis identified two intermediate emm1 sublineages in England comprising 13/27 (M113SNPs) and 23/27 SNPs (M123SNPs), respectively, that had failed to expand in the population. Proteomic analysis of invasive strains from the four phylogenetic emm1 groups highlighted sublineage-specific changes in carbohydrate metabolism, protein synthesis and protein processing; upregulation of SpeA was not observed in chemically defined medium. In rich broth, however, expression of SpeA was upregulated ~10-fold in both M123SNPs and M1UK sublineages, compared with M113SNPs and M1global. We conclude that stepwise accumulation of SNPs led to the emergence of M1UK. While increased expression of SpeA is a key indicator of M1UK and undoubtedly important, M1UK strains have outcompeted M123SNPs and other emm types that produce similar or more superantigen toxin. We speculate that an accumulation of adaptive SNPs has contributed to a wider fitness advantage in M1UK on an inherently successful emm1 streptococcal background.

Funder

Medical Research Council

Publisher

Microbiology Society

Subject

General Medicine

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