Disulfide Isomerization After Membrane Release of Its SAR Domain Activates P1 Lysozyme

7 January 2005

journal article
other
Published by American Association for the Advancement of Science (AAAS) in Science

Vol. 307 (5706) , 113-117
https://doi.org/10.1126/science.1105143

Abstract

The P1 lysozyme Lyz is secreted to the periplasm of Escherichia coli and accumulates in an inactive membrane-tethered form. Genetic and biochemical experiments show that, when released from the bilayer, Lyz is activated by an intramolecular thiol-disulfide isomerization, which requires a cysteine in its N-terminal SAR (signal-arrest-release) domain. Crystal structures confirm the alternative disulfide linkages in the two forms of Lyz and reveal dramatic conformational differences in the catalytic domain. Thus, the exported P1 endolysin is kept inactive by three levels of control—topological, conformational, and covalent—until its release from the membrane is triggered by the P1 holin.

Keywords

This publication has 19 references indexed in Scilit:

Thiol-Based Regulatory Switches
Annual Review of Genetics, 2003
Protein Disulfide Bond Formation in Prokaryotes
Annual Review of Biochemistry, 2003
Disulfide bonds as switches for protein function
Trends in Biochemical Sciences, 2003
Holins: The Protein Clocks of Bacteriophage Infections
Annual Review of Microbiology, 2000
Phages will out: strategies of host cell lysis
Trends in Microbiology, 2000
Membrane protein biosynthesis — all sewn up?
Trends in Cell Biology, 1997
A novel methodology for assignment of disulfide bond pairings in proteins
Protein Science, 1997
A Covalent Enzyme-Substrate Intermediate with Saccharide Distortion in a Mutant T4 Lysozyme
Science, 1993
Determination of Macromolecular Structures from Anomalous Diffraction of Synchrotron Radiation
Science, 1991
Reexamination of the role of Asp20 in catalysis by bacteriophage T4 lysozyme
Biochemistry, 1991