Measuring proteins in H<sub>2</sub>O with 2D-IR spectroscopy

Hume, Samantha; Hithell, Gordon; Greetham, Gregory M.; Donaldson, Paul M.; Towrie, Michael; Parker, Anthony W.; Baker, Matthew J.; Hunt, Neil T.

doi:10.1039/c9sc01590f

Cited by 50 publications

(115 citation statements)

References 30 publications

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“…1c, 1d), where many absorption bands are observed which could be attributed to the proteins, such as: 2500-3500cm -1 from -OH, 2400-3200cm -1 from NH2, 1650cm -1 from the peptide bonds, and 800-1000 cm -1 from C-H [6] . However, due to the low concentration, they are mostly overlapped by the FTIR of the buffer solution PBS, which is dominated by water (0.1wt%NaCl +0.002wt%KCl +0.01wt%Na2HPO4 +0.002%wtKH2PO4 +99 + wt%H2O), such as: 2500-3500cm -1 from -OH stretching, 2250-2500cm -1 from H-O-H bending, 1650 cm -1 from -OH scissoring, and 800-1000 cm -1 from H2O liberation, which could neither be easily resolved by D2O replacement, [28,29] although absorption band at around 1630cm -1 does show some protein variation [6] . Fortunately, there exists a FTIR absorption band exclusively associated with the proteins, but not overshadowed by the solvent at 1550 cm -1 ( Fig.…”

Section: Resultsmentioning

confidence: 99%

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Wang

Zhou

et al. 2020

Preprint

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The global battle against the Covid-19 pandemic relies strongly on the human defence of antibody, which is assumed to bind the antigen’s Receptor Binding Domain with its Hypervariable Region. Due to the similarity to other viruses such as SARS, however, our understanding of the antibody-virus interaction has been largely limited to the genomic sequencing, which poses serious challenges to the containment, vaccine exploration and rapid serum testing. Based on the physical/chemical nature of the interaction, infrared spectroscopy was employed to reveal the binding disparity, when unusual temperature dependence was discovered from the 1550cm-1 absorption band, attributed to the hydrogen bonds by carboxyl/amino groups, binding the SARS-CoV-2 spike protein and closely resembled SARS-CoV-2 or SARS-CoV-1 antibodies. The infrared absorption intensity, associated with the number of hydrogen bonds, was found to increase sharply between 27°C and 31°C, with the relative absorbance matches at 37°C the hydrogen bonding numbers of the two antibody types (19 vs 12). Meanwhile the ratio of bonds at 27°C, calculated by thermodynamic exponentials rather than by the layman’s guess, produces at least 5% inaccuracy. As a result, the specificity of the SARS-CoV-2 antibody will be more conclusive beyond 31°C, instead of at the usual room temperature of 20°C - 25°C, when the vaccine research and antibody diagnosis would likely be undermined. Beyond genomic sequencing, the temperature dependence, as well as the bond number match at 37°C between relative absorbance and the hydrogen bonding numbers of the two antibody types, are not only of clinical significance in particular, but also of a sample for the physical/chemical understanding of the vaccine-antibody interactions in general.

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Section: Resultsmentioning

confidence: 99%

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Wang

Zhou

et al. 2020

Preprint

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“…Although studies of cataract samples were carried out post-mortem, a recent study has shown that 2D-IR spectroscopy could be applied to the molecular analysis of proteins in blood serum taken as part of a routine medical procedure. 42 Spectroscopic interrogation of biofluids is attractive as a label-free, minimally-invasive screening technology. 43 Biofluids, such as blood serum are generally easily obtained, with minimal patient discomfort, and they provide access to a large amount of potentially diagnostic chemical information, reporting as they do on metabolism.…”

Section: Biomedical Applicationsmentioning

confidence: 99%

“…It was demonstrated that 2D-IR spectroscopy can avoid this problem because, in contrast to IR absorption experiments, the 2D-IR amide I signature of proteins dominates that of water even at sub-millimolar protein concentrations. 42 This important result means that 2D-IR can be used to study the amide I band of protein containing samples without the need for expensive, time consuming deuteration of solvents. Equine blood serum was employed as a test system and the unique link between protein secondary structure and the 2D-IR amide I lineshape enabled differentiation of signals due to albumin and globulin protein fractions in serum and quantitative measurements of the biomedically-important albumin to globulin ratio (AGR) with an accuracy of ±4% across a clinically-relevant range.…”

Section: Biomedical Applicationsmentioning

confidence: 99%

Two-dimensional infrared spectroscopy: an emerging analytical tool?

Fritzsch

Hume

Minnes

et al. 2020

Analyst

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“…2D-IR spectra of the isotope labelled amide I band have been shown to contain sufficient constraints to solve the structure of a large peptide 7 and although such comprehensive global structural determinations are best achieved by X-ray or NMR techniques, isotope labelled amide I 2D-IR is a unique site-specic probe of equilibrium protein structure and dynamics, 8 with applications demonstrated testing ion channel lter mechanisms 9 and amyloid aggregation. 10 For 2D-IR analysis of the amide I band of unlabelled proteins, 11,12 secondary structure determination ability is comparable to ultraviolet circular dichroism 13 and there is recent evidence of utility to this end in the analysis of blood serum samples 14 and eye cataracts. 15 In this paper, 2D spectra of the amide I band of proteins are measured using alternative laser pulse sequences involving IR and Raman processes.…”

Section: Introductionmentioning

confidence: 99%

Photon echoes and two dimensional spectra of the amide I band of proteins measured by femtosecond IR – Raman spectroscopy

Donaldson

2020

Chem. Sci.

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Measuring proteins in H₂O with 2D-IR spectroscopy

Abstract: 2D-IR spectroscopy is used to measure protein amide I bands in water, avoiding the need for deuteration. We show that H/D exchange affects protein vibrational relaxation dynamics and that the ability to perform 2D-IR in water enables blood serum protein analysis.

Cited by 50 publications

References 30 publications

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Two-dimensional infrared spectroscopy: an emerging analytical tool?

Photon echoes and two dimensional spectra of the amide I band of proteins measured by femtosecond IR – Raman spectroscopy

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Measuring proteins in H2O with 2D-IR spectroscopy

Abstract: 2D-IR spectroscopy is used to measure protein amide I bands in water, avoiding the need for deuteration. We show that H/D exchange affects protein vibrational relaxation dynamics and that the ability to perform 2D-IR in water enables blood serum protein analysis.

Cited by 50 publications

References 30 publications

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Binding strength and hydrogen bond numbers between Covid-19 RBD and HVR of antibody

Two-dimensional infrared spectroscopy: an emerging analytical tool?

Photon echoes and two dimensional spectra of the amide I band of proteins measured by femtosecond IR – Raman spectroscopy

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Product

Resources

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Measuring proteins in H₂O with 2D-IR spectroscopy