Structural changes enhance the activity of Chainia xylanase in low urea concentrations

Ameeta R. Kumar; Subray S. Hegde; K. N. Ganesh; M. I. Khan

doi:10.1016/S1570-9639(02)00530-7

Structural changes enhance the activity of Chainia xylanase in low urea concentrations

Ameeta R. Kumar, Subray S. Hegde, K. N. Ganesh, M. I. Khan

Biochemistry

Research output: Contribution to journal › Article › peer-review

7 Scopus citations

Abstract

Low concentrations of urea (1.2 M) stimulated the activity of endo-xylanase from Chainia by 30%. Subtle structural changes in the monomeric protein were reflected in the secondary and tertiary structure of the enzyme as monitored by fluorescence and circular dichroism. Changes in λ _max of emission, the fluorescence intensity and the Stern-Volmer quenching constants for acrylamide, measured in the presence of urea, indicated changes in the microenvironment of the Trp residues, suggesting alterations in tertiary structure. The ellipticity changes at 220 nm and Selcon analysis reflected changes in the content of β-sheet while both the near- and far-UV CD spectra indicated alterations in the secondary and tertiary structure of the protein in presence of urea. The dissociation constant values (K _d) show very little change in the affinity of the enzyme for the substrate while the k_cat values suggest enhanced turnover of the substrate in presence of urea. We suggest that low urea concentrations perturb the conformational state of xylanase leading to an open and a more flexible structure, resulting in enhanced catalytic rates.

Original language	English (US)
Pages (from-to)	164-171
Number of pages	8
Journal	Biochimica et Biophysica Acta - Proteins and Proteomics
Volume	1645
Issue number	2
DOIs	https://doi.org/10.1016/S1570-9639(02)00530-7
State	Published - Feb 21 2003

Keywords

Structure
Urea
Xylanase

ASJC Scopus subject areas

Analytical Chemistry
Biophysics
Biochemistry
Molecular Biology

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10.1016/S1570-9639(02)00530-7

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title = "Structural changes enhance the activity of Chainia xylanase in low urea concentrations",

abstract = "Low concentrations of urea (1.2 M) stimulated the activity of endo-xylanase from Chainia by 30%. Subtle structural changes in the monomeric protein were reflected in the secondary and tertiary structure of the enzyme as monitored by fluorescence and circular dichroism. Changes in λ max of emission, the fluorescence intensity and the Stern-Volmer quenching constants for acrylamide, measured in the presence of urea, indicated changes in the microenvironment of the Trp residues, suggesting alterations in tertiary structure. The ellipticity changes at 220 nm and Selcon analysis reflected changes in the content of β-sheet while both the near- and far-UV CD spectra indicated alterations in the secondary and tertiary structure of the protein in presence of urea. The dissociation constant values (K d) show very little change in the affinity of the enzyme for the substrate while the kcat values suggest enhanced turnover of the substrate in presence of urea. We suggest that low urea concentrations perturb the conformational state of xylanase leading to an open and a more flexible structure, resulting in enhanced catalytic rates.",

keywords = "Structure, Urea, Xylanase",

author = "Kumar, {Ameeta R.} and Hegde, {Subray S.} and Ganesh, {K. N.} and Khan, {M. I.}",

note = "Funding Information: Financial assistance to ARK and SSH in the form of fellowships from the Council of Scientific and Industrial Research (CSIR), India, is gratefully acknowledged. This work was carried out as part of the protein engineering project of KNG and MIK, sponsored by Department of Biotechnology and CSIR, India. We also thank Dr. V. Shanker for his critical reading of the manuscript and useful suggestions.",

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AU - Hegde, Subray S.

AU - Ganesh, K. N.

AU - Khan, M. I.

N1 - Funding Information: Financial assistance to ARK and SSH in the form of fellowships from the Council of Scientific and Industrial Research (CSIR), India, is gratefully acknowledged. This work was carried out as part of the protein engineering project of KNG and MIK, sponsored by Department of Biotechnology and CSIR, India. We also thank Dr. V. Shanker for his critical reading of the manuscript and useful suggestions.

PY - 2003/2/21

Y1 - 2003/2/21

N2 - Low concentrations of urea (1.2 M) stimulated the activity of endo-xylanase from Chainia by 30%. Subtle structural changes in the monomeric protein were reflected in the secondary and tertiary structure of the enzyme as monitored by fluorescence and circular dichroism. Changes in λ max of emission, the fluorescence intensity and the Stern-Volmer quenching constants for acrylamide, measured in the presence of urea, indicated changes in the microenvironment of the Trp residues, suggesting alterations in tertiary structure. The ellipticity changes at 220 nm and Selcon analysis reflected changes in the content of β-sheet while both the near- and far-UV CD spectra indicated alterations in the secondary and tertiary structure of the protein in presence of urea. The dissociation constant values (K d) show very little change in the affinity of the enzyme for the substrate while the kcat values suggest enhanced turnover of the substrate in presence of urea. We suggest that low urea concentrations perturb the conformational state of xylanase leading to an open and a more flexible structure, resulting in enhanced catalytic rates.

AB - Low concentrations of urea (1.2 M) stimulated the activity of endo-xylanase from Chainia by 30%. Subtle structural changes in the monomeric protein were reflected in the secondary and tertiary structure of the enzyme as monitored by fluorescence and circular dichroism. Changes in λ max of emission, the fluorescence intensity and the Stern-Volmer quenching constants for acrylamide, measured in the presence of urea, indicated changes in the microenvironment of the Trp residues, suggesting alterations in tertiary structure. The ellipticity changes at 220 nm and Selcon analysis reflected changes in the content of β-sheet while both the near- and far-UV CD spectra indicated alterations in the secondary and tertiary structure of the protein in presence of urea. The dissociation constant values (K d) show very little change in the affinity of the enzyme for the substrate while the kcat values suggest enhanced turnover of the substrate in presence of urea. We suggest that low urea concentrations perturb the conformational state of xylanase leading to an open and a more flexible structure, resulting in enhanced catalytic rates.

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Structural changes enhance the activity of Chainia xylanase in low urea concentrations

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