Journal
ACS CHEMICAL BIOLOGY
Volume 16, Issue 5, Pages 844-856Publisher
AMER CHEMICAL SOC
DOI: 10.1021/acschembio.1c00013
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Funding
- Tri-Institutional Chemical Biology program through the NIH Chemistry-Biology Training Grant [T32 GM115327]
- NSF Graduate Research Fellowship
- NIH [P41GM066354]
- New York State Assembly
- National Natural Science Foundation of China [21778010]
- Shenzhen Science and Technology Innovation Committee [JCYJ20170412150832022]
- NSF [MCB-1810695]
- ORIP/NIH facility improvement grant [CO6RR015495]
- NIH-NIGMS [R01GM087544]
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Site-specific S-palmitoylation of IFITM3 enhances its antiviral activity by modulating its conformation and interaction with lipid membranes, demonstrating the direct impact of lipidation on the protein's biophysical properties and cellular activity to prevent virus infection.
Interferon-induced transmembrane proteins (IFITMs) are S-palmitoylated proteins in vertebrates that restrict a diverse range of viruses. S-palmitoylated IFITM3 in particular engages incoming virus particles, prevents their cytoplasmic entry, and accelerates their lysosomal clearance by host cells. However, how S-palmitoylation modulates the structure and biophysical characteristics of IFITM3 to promote its antiviral activity remains unclear. To investigate how site-specific S-palmitoylation controls IFITM3 antiviral activity, we employed computational, chemical, and biophysical approaches to demonstrate that site-specific lipidation of cysteine 72 enhances the antiviral activity of IFITM3 by modulating its conformation and interaction with lipid membranes. Collectively, our results demonstrate that site-specific S-palmitoylation of IFITM3 directly alters its biophysical properties and activity in cells to prevent virus infection.
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