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Tytuł pozycji:

FT-Raman Spectroscopy as a Tool to Study the Secondary Structures of Wheat Gliadin Proteins.

Tytuł:
FT-Raman Spectroscopy as a Tool to Study the Secondary Structures of Wheat Gliadin Proteins.
Autorzy:
Stawoska I; Institute of Biology, Pedagogical University of Krakow, Podchorążych 2, 30-084 Krakow, Poland.
Wesełucha-Birczyńska A; Faculty of Chemistry, Jagiellonian University, Gronostajowa 2, 30-387 Kraków, Poland.
Skoczowski A; Institute of Biology, Pedagogical University of Krakow, Podchorążych 2, 30-084 Krakow, Poland.; The Franciszek Górski Institute of Plant Physiology, Polish Academy of Sciences, Niezapominajek 21, 30-239 Krakow, Poland.
Dziurka M; The Franciszek Górski Institute of Plant Physiology, Polish Academy of Sciences, Niezapominajek 21, 30-239 Krakow, Poland.
Waga J; Department of Physiology, Plant Breeding and Seed Science, University of Agriculture, Podłużna 3, 30-239 Kraków, Poland.
Źródło:
Molecules (Basel, Switzerland) [Molecules] 2021 Sep 04; Vol. 26 (17). Date of Electronic Publication: 2021 Sep 04.
Typ publikacji:
Journal Article
Język:
English
Imprint Name(s):
Original Publication: Basel, Switzerland : MDPI, c1995-
MeSH Terms:
Gliadin/*chemistry
Triticum/*chemistry
Genotype ; Gliadin/genetics ; Hydrogen Bonding ; Protein Conformation, alpha-Helical ; Protein Conformation, beta-Strand ; Spectrum Analysis, Raman
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Grant Information:
POIR.04.01.04-00-0051/18 Narodowe Centrum Badań i Rozwoju
Contributed Indexing:
Keywords: Raman spectroscopy; amide I; gliadins; gluten proteins; secondary structure
Substance Nomenclature:
9007-90-3 (Gliadin)
Entry Date(s):
Date Created: 20210910 Date Completed: 20211111 Latest Revision: 20211111
Update Code:
20240105
PubMed Central ID:
PMC8434250
DOI:
10.3390/molecules26175388
PMID:
34500820
Czasopismo naukowe
Raman spectroscopy is a useful method in biological, biomedical, food, and agricultural studies, allowing the simultaneous examination of various chemical compounds and evaluation of molecular changes occurring in tested objects. The purpose of our research was to explain how the elimination of ω-fractions from the wheat gliadin complex influences the secondary structures of the remaining αβγ-gliadins. To this aim, we analyzed the endosperm of wheat kernels as well as gliadin proteins extracted from two winter wheat genotypes: wasko.gl+ (control genotype containing the full set of gliadins) and wasko.gl- (modified genotype lacking all ω-gliadins). Based on the decomposition of the amide I band, we observed a moderate increase in β-forms (sheets and turns) at the expense of α-helical and random coil structures for gliadins isolated from the flour of the wasko.gl- line. Since ω-gliadins contain no cysteine residues, they do not participate in the formation of the disulfide bridges that stabilize the protein structure. However, they can interact with other proteins via weak, low-energetic hydrogen bonds. We conclude that the elimination of ω-fractions from the gliadin complex causes minor modifications in secondary structures of the remaining gliadin proteins. In our opinion, these small, structural changes of proteins may lead to alterations in gliadin allergenicity.

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