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Research Domain: Physical & Biophysical Chemistry; Bio-nanotechnolo
Keyword: Steven G. Boxer
Research Production: Principal Research Interests
My laboratory investigates the structure and function of biological systems using many tools and methods, always with a strong physical perspective. Three interconnected themes are being pursued.

First, we have a long-standing interest in the mechanism of light-driven long-distance electron transfer in photosynthetic reaction centers, one of the fastest known reactions. This is being studied by femtosecond fluorescence and transient absorption spectroscopy, manipulation in electric fields, site-specific mutagenesis and some novel types of Stark spectroscopy we have developed and applied to many types of molecules. Related methods are also being used to probe excited state dynamics and electronic structure in variants of green fluorescent protein (GFP), widely used in cell biology.

Second, we are broadly interested in electrostatics in proteins and how electrostatics affects function. Our current work uses probes whose sensitivity to electric fields can be calibrated by Stark spectroscopy. Vibrational Stark experiments are particularly useful as they provide a calibration for mapping electrostatic fields in proteins. Probes have also been developed that can measure the time-dependent solvation of charges at different positions in proteins, a key aspect of protein-protein and protein-ligand interactions and catalysis. These approaches are also being used to investigate photosynthetic reaction centers and GFP.

Third, we use supported lipid bilayers as mimics for cell surfaces and as tools in biotechnology. A broad vision is to engineer interfaces between hard surfaces and soft materials, ultimately leading to sophisticated biocompatible interfaces that can be used to control, interrogate or organize complex living systems. We have developed methods for partitioning and manipulating the composition and organization of these unique self-assembled systems. Recent work addresses the formation of domains and protein association with these domains, interactions of DNA, proteins and cells with supported bilayers, and the mechanism of vesicle fusion, both to solid supports and mediated by proteins. This work has motivated the development of advanced optical microscopy methods for probing the interface between membranes on solid supports and cell membranes, potentially with nm vertical resolution. A novel type of imaging mass spectrometry is being applied to characterize the lateral organization and composition of bilayers and associated membranes with 50 nm resolution.
Remarks: Camille and Henry Dreyfus Professor of Chemistry (b. 1947)

B.S., 1969, Tufts University; Ph.D., 1976, University of Chicago

A.P. Sloan Fellow, 1980; Dreyfus Teacher-Scholar Fellow, 1981; Dean's Award for Distinguished Teaching, 1982; Presidential Young Investigator Award, 1984; American Society of Photobiology Award, 1992; Five College Lecturer in Chemistry, 1993; NIH Merit Award, 1994; ACS Cope Scholar Award, 1995; American Academy of Arts and Sciences, 1997

Physical, Biophysical Chemistry; Bio-nanotechnology

Title:Camille and Henry Dreyfus Professor in Chemistry
Work Phone:(650) 723-4482
Fax:(650) 723-4817
Work Address:Keck Bldg., Rm. 325
Stanford, California, 94305-5080
Email:sboxer@stanford.edu
Boxer Group 
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