Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods
The self-assembly of proteins is an essential process for a variety of cellular functions including cell respiration, mobility and division. On the other hand, protein or peptide misfolding and aggregation is related to the development of Parkinson’s disease and Alzheimer’s disease, among other aggr...
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doaj-29fec2c8b9904a7fa2d3bcbbd1feae482020-11-25T03:53:17ZengMDPI AGMolecules1420-30492020-10-01254854485410.3390/molecules25204854Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic MethodsMaría Florencia Pignataro0María Georgina Herrera1Verónica Isabel Dodero2Department of Physiology and Molecular and Cellular Biology, Institute of Biosciences, Biotechnology and Translational Biology (iB3), Faculty of Exact and Natural Sciences, University of Buenos Aires, Buenos Aires C1428EG, ArgentinaDepartment of Physiology and Molecular and Cellular Biology, Institute of Biosciences, Biotechnology and Translational Biology (iB3), Faculty of Exact and Natural Sciences, University of Buenos Aires, Buenos Aires C1428EG, ArgentinaOrganic and Bioorganic Chemistry, Department of Chemistry, Bielefeld University, 33615 Bielefeld, GermanyThe self-assembly of proteins is an essential process for a variety of cellular functions including cell respiration, mobility and division. On the other hand, protein or peptide misfolding and aggregation is related to the development of Parkinson’s disease and Alzheimer’s disease, among other aggregopathies. As a consequence, significant research efforts are directed towards the understanding of this process. In this review, we are focused on the use of UV-Visible Absorption Spectroscopy, Fluorescence Spectroscopy and Circular Dichroism to evaluate the self-organization of proteins and peptides in solution. These spectroscopic techniques are commonly available in most chemistry and biochemistry research laboratories, and together they are a powerful approach for initial as well as routine evaluation of protein and peptide self-assembly and aggregation under different environmental stimulus. Furthermore, these spectroscopic techniques are even suitable for studying complex systems like those in the food industry or pharmaceutical formulations, providing an overall idea of the folding, self-assembly, and aggregation processes, which is challenging to obtain with high-resolution methods. Here, we compiled and discussed selected examples, together with our results and those that helped us better to understand the process of protein and peptide aggregation. We put particular emphasis on the basic description of the methods as well as on the experimental considerations needed to obtain meaningful information, to help those who are just getting into this exciting area of research. Moreover, this review is particularly useful to those out of the field who would like to improve reproducibility in their cellular and biomedical experiments, especially while working with peptide and protein systems as an external stimulus. Our final aim is to show the power of these low-resolution techniques to improve our understanding of the self-assembly of peptides and proteins and translate this fundamental knowledge in biomedical research or food applications.https://www.mdpi.com/1420-3049/25/20/4854proteinspeptidesself-assemblydyesaggregationfibrils |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
María Florencia Pignataro María Georgina Herrera Verónica Isabel Dodero |
spellingShingle |
María Florencia Pignataro María Georgina Herrera Verónica Isabel Dodero Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods Molecules proteins peptides self-assembly dyes aggregation fibrils |
author_facet |
María Florencia Pignataro María Georgina Herrera Verónica Isabel Dodero |
author_sort |
María Florencia Pignataro |
title |
Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods |
title_short |
Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods |
title_full |
Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods |
title_fullStr |
Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods |
title_full_unstemmed |
Evaluation of Peptide/Protein Self-Assembly and Aggregation by Spectroscopic Methods |
title_sort |
evaluation of peptide/protein self-assembly and aggregation by spectroscopic methods |
publisher |
MDPI AG |
series |
Molecules |
issn |
1420-3049 |
publishDate |
2020-10-01 |
description |
The self-assembly of proteins is an essential process for a variety of cellular functions including cell respiration, mobility and division. On the other hand, protein or peptide misfolding and aggregation is related to the development of Parkinson’s disease and Alzheimer’s disease, among other aggregopathies. As a consequence, significant research efforts are directed towards the understanding of this process. In this review, we are focused on the use of UV-Visible Absorption Spectroscopy, Fluorescence Spectroscopy and Circular Dichroism to evaluate the self-organization of proteins and peptides in solution. These spectroscopic techniques are commonly available in most chemistry and biochemistry research laboratories, and together they are a powerful approach for initial as well as routine evaluation of protein and peptide self-assembly and aggregation under different environmental stimulus. Furthermore, these spectroscopic techniques are even suitable for studying complex systems like those in the food industry or pharmaceutical formulations, providing an overall idea of the folding, self-assembly, and aggregation processes, which is challenging to obtain with high-resolution methods. Here, we compiled and discussed selected examples, together with our results and those that helped us better to understand the process of protein and peptide aggregation. We put particular emphasis on the basic description of the methods as well as on the experimental considerations needed to obtain meaningful information, to help those who are just getting into this exciting area of research. Moreover, this review is particularly useful to those out of the field who would like to improve reproducibility in their cellular and biomedical experiments, especially while working with peptide and protein systems as an external stimulus. Our final aim is to show the power of these low-resolution techniques to improve our understanding of the self-assembly of peptides and proteins and translate this fundamental knowledge in biomedical research or food applications. |
topic |
proteins peptides self-assembly dyes aggregation fibrils |
url |
https://www.mdpi.com/1420-3049/25/20/4854 |
work_keys_str_mv |
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