Sequence-Specific Protein Secondary-Structure Assignment with Isotope Reverse-Labeled Amide I Spectroscopy

Sequence-Specific Protein Secondary-Structure Assignment with Isotope Reverse-Labeled Amide I Spectroscopy

The dramatic advances made recently by protein-structure prediction tools like AlphaFold offer an opportunity for the development of new experimental methods designed to test sequence-based predictions rather than build full atomistic structures from scratch. While atomistic methods such as X-ray cr...

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Bibliographic Details
Main Author: Jacob H. Wat (22577422) (author)
Other Authors: Tristen West (22577425) (author), Nicolas J. Pizzala (19442700) (author), Sarah Alvarez (5545145) (author), Yanbin Wang (1758400) (author), Ming Chen (115604) (author), Mike Reppert (1281084) (author)
Published: 2025
Subjects:
Biophysics
Biochemistry
Molecular Biology
Hematology
Plant Biology
Biological Sciences not elsewhere classified
Chemical Sciences not elsewhere classified
Physical Sciences not elsewhere classified
nuclear magnetic resonance
cryogenic electron microscopy
concepts experimentally using
specific structural information
new experimental approach
13 </ sup
12 </ sup
whose crystal structure
published crystal structure
low sample cost
based predictions rather
labeled protein construct
collect ftir spectra
resulting isotope reverse
labeled ftir spectroscopy
specific protein secondary
specific secondary
labeled amide
enriched spectra
approach offers
structure determination
structure content
structure assignments
structure assignment
secondary structure
traditional ftir
protein ’
enriched protein
wide variety
transform infrared
total fraction
spectroscopic methods
solubilized membranes
sheet present
routine characterization
ray crystallography
producing isotope
present contribution
often cheaper
offer insight
obtain assignments
live cells
isotope reverse
expression culture
efficient means
critical role
circular dichroism
bulk secondary
atomistic methods
amino acids
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Summary:The dramatic advances made recently by protein-structure prediction tools like AlphaFold offer an opportunity for the development of new experimental methods designed to test sequence-based predictions rather than build full atomistic structures from scratch. While atomistic methods such as X-ray crystallography, nuclear magnetic resonance (NMR) spectroscopy, and cryogenic electron microscopy (CryoEM) will always play a critical role in structure determination, their cost and stringent sample preparation requirements can be prohibitive for routine characterization. Spectroscopic methods such as circular dichroism (CD) and Fourier-transform infrared (FTIR) spectroscopy are often cheaper and faster but offer insight only into bulk secondary-structure content such as the total fraction of α-helix or β-sheet present in a protein. In the present contribution, we suggest that isotope-labeled FTIR spectroscopy has the potential to fill this gap, and we demonstrate a new experimental approach to producing isotope-enriched spectra at a low sample cost. We illustrate these concepts experimentally using the protein Top7 V48 V (whose crystal structure is known) as an example. By selectively <sup>12</sup>C-labeling individual amino acid residues in only 5 mL of <sup>13</sup>C-enriched protein-expression culture, we collect FTIR spectra of each reverse-labeled protein construct at a cost of only a few dollars of isotope-enriched material per sample. Analysis of the resulting isotope reverse-labeled FTIR spectra provides a path to secondary-structure assignments for each amino acid individually rather than only the total secondary structure estimates that are available from traditional FTIR or CD measurements. Combining these residue-specific secondary-structure assignments with knowledge of the protein’s primary sequence, we obtain assignments for the secondary structure of each stretch of amino acids in the protein that agree well with the published crystal structure of the protein. Based on these results, we suggest that this approach offers a fast and efficient means of extracting sequence-specific structural information that can be applied to proteins in a wide variety of contexts, from live cells to solubilized membranes.

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