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Engineering Agrobacterium tumefaciens adhesion to target cells

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Abstract Agrobacterium tumefaciens is a plant pathogen commonly repurposed for genetic modification of crops. Despite its versatility, it remains inefficient at transferring DNA to many hosts, including to animal cells. Like many pathogens, physical contact between A. tumefaciens and host cells promotes infection efficacy. Thus, improving the strength and specificity of A. tumefaciens to target cells has the potential for enhancing DNA transfer for biotechnological and therapeutic purposes. Here we demonstrate a methodology for engineering genetically-encoded exogeneous adhesins at the surface of A. tumefaciens . We identified an autotransporter gene we named Aat, that is predicted to show canonical β-barrel and passenger domains. We engineered the β-barrel scaffold and linker (Aat β ) to display synthetic adhesins susceptible to rewire A. tumefaciens to alternative host targets. As a proof of concept, we leveraged the versatility of a VHH domain to rewire A. tumefaciens adhesion to yeast and mammalian hosts displaying a GFP target receptor. Finally, to demonstrate how synthetic A. tumefaciens adhesion can improve transfer to host cells, we showed improved protein translocation into HeLa cells using a sensitive split luciferase reporter system. Engineering A. tumefaciens adhesion has therefore a strong potential in generating complex heterogeneous cellular assemblies and in improving DNA transfer efficiency against non-natural hosts.
Title: Engineering Agrobacterium tumefaciens adhesion to target cells
Description:
Abstract Agrobacterium tumefaciens is a plant pathogen commonly repurposed for genetic modification of crops.
Despite its versatility, it remains inefficient at transferring DNA to many hosts, including to animal cells.
Like many pathogens, physical contact between A.
tumefaciens and host cells promotes infection efficacy.
Thus, improving the strength and specificity of A.
tumefaciens to target cells has the potential for enhancing DNA transfer for biotechnological and therapeutic purposes.
Here we demonstrate a methodology for engineering genetically-encoded exogeneous adhesins at the surface of A.
tumefaciens .
We identified an autotransporter gene we named Aat, that is predicted to show canonical β-barrel and passenger domains.
We engineered the β-barrel scaffold and linker (Aat β ) to display synthetic adhesins susceptible to rewire A.
tumefaciens to alternative host targets.
As a proof of concept, we leveraged the versatility of a VHH domain to rewire A.
tumefaciens adhesion to yeast and mammalian hosts displaying a GFP target receptor.
Finally, to demonstrate how synthetic A.
tumefaciens adhesion can improve transfer to host cells, we showed improved protein translocation into HeLa cells using a sensitive split luciferase reporter system.
Engineering A.
tumefaciens adhesion has therefore a strong potential in generating complex heterogeneous cellular assemblies and in improving DNA transfer efficiency against non-natural hosts.

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