Open Access
Thermal Inactivation of Glucose Oxidase
Mudeppa Devaraja Gouda
1
,
Sridevi Annapurna Singh
2
,
A. Sambasiva Rao
2
,
Munna Singh Thakur
1
,
Naikankatte Ganesh Karanth
1
1
Fermentation Technology and Bioengineering
Publication type: Journal Article
Publication date: 2003-07-01
scimago Q1
wos Q2
SJR: 1.705
CiteScore: 7.6
Impact factor: 3.9
ISSN: 00219258, 1083351X
PubMed ID:
12716878
Biochemistry
Molecular Biology
Cell Biology
Abstract
Thermal inactivation of glucose oxidase (GOD; beta-d-glucose: oxygen oxidoreductase), from Aspergillus niger, followed first order kinetics both in the absence and presence of additives. Additives such as lysozyme, NaCl, and K2SO4 increased the half-life of the enzyme by 3.5-, 33.4-, and 23.7-fold respectively, from its initial value at 60 degrees C. The activation energy increased from 60.3 kcal mol-1 to 72.9, 76.1, and 88.3 kcal mol-1, whereas the entropy of activation increased from 104 to 141, 147, and 184 cal x mol-1 x deg-1 in the presence of 7.1 x 10-5 m lysozyme, 1 m NaCl, and 0.2 m K2SO4, respectively. The thermal unfolding of GOD in the temperature range of 25-90 degrees C was studied using circular dichroism measurements at 222, 274, and 375 nm. Size exclusion chromatography was employed to follow the state of association of enzyme and dissociation of FAD from GOD. The midpoint for thermal inactivation of residual activity and the dissociation of FAD was 59 degrees C, whereas the corresponding midpoint for loss of secondary and tertiary structure was 62 degrees C. Dissociation of FAD from the holoenzyme was responsible for the thermal inactivation of GOD. The irreversible nature of inactivation was caused by a change in the state of association of apoenzyme. The dissociation of FAD resulted in the loss of secondary and tertiary structure, leading to the unfolding and nonspecific aggregation of the enzyme molecule because of hydrophobic interactions of side chains. This confirmed the critical role of FAD in structure and activity. Cysteine oxidation did not contribute to the nonspecific aggregation. The stabilization of enzyme by NaCl and lysozyme was primarily the result of charge neutralization. K2SO4 enhanced the thermal stability by primarily strengthening the hydrophobic interactions and made the holoenzyme a more compact dimeric structure.
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Total citations:
168
Citations from 2025:
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(4.17%)
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GOST
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Gouda M. D. et al. Thermal Inactivation of Glucose Oxidase // Journal of Biological Chemistry. 2003. Vol. 278. No. 27. pp. 24324-24333.
GOST all authors (up to 50)
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Gouda M. D., Singh S. A., Rao A. S., Thakur M. S., Karanth N. G. Thermal Inactivation of Glucose Oxidase // Journal of Biological Chemistry. 2003. Vol. 278. No. 27. pp. 24324-24333.
Cite this
RIS
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TY - JOUR
DO - 10.1074/jbc.M208711200
UR - https://doi.org/10.1074/jbc.M208711200
TI - Thermal Inactivation of Glucose Oxidase
T2 - Journal of Biological Chemistry
AU - Gouda, Mudeppa Devaraja
AU - Singh, Sridevi Annapurna
AU - Rao, A. Sambasiva
AU - Thakur, Munna Singh
AU - Karanth, Naikankatte Ganesh
PY - 2003
DA - 2003/07/01
PB - American Society for Biochemistry and Molecular Biology
SP - 24324-24333
IS - 27
VL - 278
PMID - 12716878
SN - 0021-9258
SN - 1083-351X
ER -
Cite this
BibTex (up to 50 authors)
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@article{2003_Gouda,
author = {Mudeppa Devaraja Gouda and Sridevi Annapurna Singh and A. Sambasiva Rao and Munna Singh Thakur and Naikankatte Ganesh Karanth},
title = {Thermal Inactivation of Glucose Oxidase},
journal = {Journal of Biological Chemistry},
year = {2003},
volume = {278},
publisher = {American Society for Biochemistry and Molecular Biology},
month = {jul},
url = {https://doi.org/10.1074/jbc.M208711200},
number = {27},
pages = {24324--24333},
doi = {10.1074/jbc.M208711200}
}
Cite this
MLA
Copy
Gouda, Mudeppa Devaraja, et al. “Thermal Inactivation of Glucose Oxidase.” Journal of Biological Chemistry, vol. 278, no. 27, Jul. 2003, pp. 24324-24333. https://doi.org/10.1074/jbc.M208711200.