Upregulation of virulence genes promotes Vibrio cholerae biofilm hyperinfectivity
Abstract
Vibrio cholerae remains a major global health threat, disproportionately impacting parts of the world without adequate infrastructure and sanitation resources. In aquatic environments, V. cholerae exists both as planktonic cells and as biofilms, which are held together by an extracellular matrix. V. cholerae biofilms have been shown to be hyperinfective, but the mechanism of hyperinfectivity is unclear. Here we show that biofilm-grown cells, irrespective of the surfaces on which they are formed, are able to markedly outcompete planktonic-grown cells in the infant mouse. Using an imaging technique designed to render intestinal tissue optically transparent and preserve the spatial integrity of infected intestines, we reveal and compare three-dimensional V. cholerae colonization patterns of planktonic-grown and biofilm-grown cells. Quantitative image analyses show that V. cholerae colonizes mainly the medial portion of the small intestine and that both the abundance and localization patterns of biofilm-grown cells differ from that of planktonic-grown cells. In vitro biofilm-grown cells activate expression of the virulence cascade, including the toxin coregulated pilus (TCP), and are able to acquire the cholera toxin-carrying CTXФ phage. Overall, virulence factor gene expression is also higher in vivo when infected with biofilm-grown cells, and modulation of their regulation is sufficient to cause the biofilm hyperinfectivity phenotype. Together, these results indicate that the altered biogeography of biofilm-grown cells and their enhanced production of virulence factors in the intestine underpin the biofilm hyperinfectivity phenotype.
Additional Information
© 2020 National Academy of Sciences. Published under the PNAS license. Edited by John J. Mekalanos, Harvard University, Boston, MA, and approved March 11, 2020 (received for review September 23, 2019). PNAS first published April 30, 2020. We thank Benjamin Abrams, University of California, Santa Cruz (UCSC) Life Sciences Microscopy Center, for technical support during confocal imaging, which is supported by grant S10 OD023528 (to F.H.Y.) from the National Institutes of Health. We thank Ron Taylor and Karen Skorupski for the TcpA antibody. We thank Adam Alpine for his assistance with Fig. 2 A and B. We thank Molecular Technologies (Caltech) for assistance with HCR probe design. We would also like to acknowledge the members of the F.H.Y. laboratory and Karla J. F. Satchell for their useful input and contributions. This work was supported by NIH grants RO1 AI102584, RO1 AI114261, and RO1 AI055987 (to F.H.Y.); NIH grants 5R01HL117328-03 and 1R01AI127850-01A1 (to D.K.N.); and the DEPAS17F0 fellowship from the Cystic Fibrosis Foundation (to W.H.D.), as well as the European Research Council StG-716734, the Human Frontier Science Program CDA00084/2015-C, and the Deutsche Forschungsgemeinschaft SFB987 (to K.D.). A.L.G.-H. was supported by the University of California Institute for Mexico and the United States (UC MEXUS) and El Consejo Nacional de Ciencia y Tecnología (CONACYT) Postdoctoral Research fellowship. Data Availability: RNA-seq data are available through NCBI GEO with series number GSE135887. Author contributions: A.L.G.-H., W.H.D., J.H.P., J.K.T., K.D., D.K.N., and F.H.Y. designed research; A.L.G.-H., W.H.D., J.H.P., and J.K.T. performed research; R.H. contributed new reagents/analytic tools; A.L.G.-H., W.H.D., J.H.P., J.K.T., R.H., H.J., K.D., S.B., D.K.N., and F.H.Y. analyzed data; and A.L.G.-H., W.H.D., J.H.P., J.K.T., K.D., D.K.N., and F.H.Y. wrote the paper. The authors declare no competing interest. This article is a PNAS Direct Submission. Data deposition: RNA-seq data are available through National Center for Biotechnology Information (NCBI) Gene Expression Omnibus (GEO) (series number GSE135887). This article contains supporting information online at https://www.pnas.org/lookup/suppl/doi:10.1073/pnas.1916571117/-/DCSupplemental.Attached Files
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Additional details
- PMCID
- PMC7245069
- Eprint ID
- 102971
- DOI
- 10.1073/pnas.1916571117
- Resolver ID
- CaltechAUTHORS:20200504-083728290
- S10 OD023528
- NIH
- RO1 AI102584
- NIH
- RO1 AI114261
- NIH
- RO1 AI055987
- NIH
- 5R01HL117328-03
- NIH
- 1R01AI127850-01A1
- NIH
- DEPAS17F0
- Cystic Fibrosis Foundation
- 716734
- European Research Council (ERC)
- CDA00084/2015-C
- Human Frontier Science Program
- SFB987
- Deutsche Forschungsgemeinschaft (DFG)
- University of California Institute for Mexico and the United States (UC MEXUS)
- Consejo Nacional de Ciencia y Tecnología (CONACYT)
- Created
-
2020-05-04Created from EPrint's datestamp field
- Updated
-
2021-11-16Created from EPrint's last_modified field
- Caltech groups
- Division of Geological and Planetary Sciences, Division of Biology and Biological Engineering