Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin: a kinetic and specificity study

Kirsten Kastberg Møller; Fergal Patrick Rattray; Jens Christian Sørensen; Ylva Margareta Ardö

doi:10.1021/jf300557d

Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin: a kinetic and specificity study

Kirsten Kastberg Møller, Fergal Patrick Rattray, Jens Christian Sørensen, Ylva Margareta Ardö

29 Citations (Scopus)

Abstract

Bovine chymosin constitutes a traditional ingredient for enzymatic milk coagulation in cheese making, providing a strong clotting capacity and low general proteolytic activity. Recently, these properties were surpassed by camel chymosin, but the mechanistic difference behind their action is not yet clear. We used capillary electrophoresis and reversed-phase liquid chromatography-mass spectrometry to compare the first site of hydrolysis of camel and bovine chymosin on bovine κ-casein (CN) and to determine the kinetic parameters of this reaction (pH 6.5; 32 °C). The enzymes showed identical specificities, cleaving the Phe105-Met106 bond of κ-CN to produce para-κ-CN and caseinomacropeptide. Initial formation rates of both products validated Michaelis-Menten modeling of the kinetic properties of both enzymes. Camel chymosin bound κ-CN with ∼30% lower affinity (K _M) and exhibited a 60% higher turnover rate (k_cat), resulting in ∼15% higher catalytic efficiency (k_cat/K _M) as compared to bovine chymosin. A local, less dense negatively charged cluster on the surface of camel chymosin may weaken electrostatic binding to the His-Pro cluster of κ-CN to simultaneously impart reduced substrate affinity and accelerated enzyme-substrate dissociation as compared to bovine chymosin.

Original language	English
Journal	Journal of Agricultural and Food Chemistry
Volume	60
Issue number	21
Pages (from-to)	5454-5460
Number of pages	7
ISSN	0021-8561
DOIs	https://doi.org/10.1021/jf300557d
Publication status	Published - 30 May 2012

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Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin : a kinetic and specificity study. / Møller, Kirsten Kastberg; Rattray, Fergal Patrick; Sørensen, Jens Christian et al.

In: Journal of Agricultural and Food Chemistry, Vol. 60, No. 21, 30.05.2012, p. 5454-5460.

Research output: Contribution to journal › Journal article › Research › peer-review

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title = "Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin: a kinetic and specificity study",

abstract = "Bovine chymosin constitutes a traditional ingredient for enzymatic milk coagulation in cheese making, providing a strong clotting capacity and low general proteolytic activity. Recently, these properties were surpassed by camel chymosin, but the mechanistic difference behind their action is not yet clear. We used capillary electrophoresis and reversed-phase liquid chromatography-mass spectrometry to compare the first site of hydrolysis of camel and bovine chymosin on bovine κ-casein (CN) and to determine the kinetic parameters of this reaction (pH 6.5; 32 °C). The enzymes showed identical specificities, cleaving the Phe105-Met106 bond of κ-CN to produce para-κ-CN and caseinomacropeptide. Initial formation rates of both products validated Michaelis-Menten modeling of the kinetic properties of both enzymes. Camel chymosin bound κ-CN with ∼30% lower affinity (K M) and exhibited a 60% higher turnover rate (kcat), resulting in ∼15% higher catalytic efficiency (kcat/K M) as compared to bovine chymosin. A local, less dense negatively charged cluster on the surface of camel chymosin may weaken electrostatic binding to the His-Pro cluster of κ-CN to simultaneously impart reduced substrate affinity and accelerated enzyme-substrate dissociation as compared to bovine chymosin.",

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T1 - Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin

T2 - a kinetic and specificity study

AU - Møller, Kirsten Kastberg

AU - Rattray, Fergal Patrick

AU - Sørensen, Jens Christian

AU - Ardö, Ylva Margareta

PY - 2012/5/30

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N2 - Bovine chymosin constitutes a traditional ingredient for enzymatic milk coagulation in cheese making, providing a strong clotting capacity and low general proteolytic activity. Recently, these properties were surpassed by camel chymosin, but the mechanistic difference behind their action is not yet clear. We used capillary electrophoresis and reversed-phase liquid chromatography-mass spectrometry to compare the first site of hydrolysis of camel and bovine chymosin on bovine κ-casein (CN) and to determine the kinetic parameters of this reaction (pH 6.5; 32 °C). The enzymes showed identical specificities, cleaving the Phe105-Met106 bond of κ-CN to produce para-κ-CN and caseinomacropeptide. Initial formation rates of both products validated Michaelis-Menten modeling of the kinetic properties of both enzymes. Camel chymosin bound κ-CN with ∼30% lower affinity (K M) and exhibited a 60% higher turnover rate (kcat), resulting in ∼15% higher catalytic efficiency (kcat/K M) as compared to bovine chymosin. A local, less dense negatively charged cluster on the surface of camel chymosin may weaken electrostatic binding to the His-Pro cluster of κ-CN to simultaneously impart reduced substrate affinity and accelerated enzyme-substrate dissociation as compared to bovine chymosin.

AB - Bovine chymosin constitutes a traditional ingredient for enzymatic milk coagulation in cheese making, providing a strong clotting capacity and low general proteolytic activity. Recently, these properties were surpassed by camel chymosin, but the mechanistic difference behind their action is not yet clear. We used capillary electrophoresis and reversed-phase liquid chromatography-mass spectrometry to compare the first site of hydrolysis of camel and bovine chymosin on bovine κ-casein (CN) and to determine the kinetic parameters of this reaction (pH 6.5; 32 °C). The enzymes showed identical specificities, cleaving the Phe105-Met106 bond of κ-CN to produce para-κ-CN and caseinomacropeptide. Initial formation rates of both products validated Michaelis-Menten modeling of the kinetic properties of both enzymes. Camel chymosin bound κ-CN with ∼30% lower affinity (K M) and exhibited a 60% higher turnover rate (kcat), resulting in ∼15% higher catalytic efficiency (kcat/K M) as compared to bovine chymosin. A local, less dense negatively charged cluster on the surface of camel chymosin may weaken electrostatic binding to the His-Pro cluster of κ-CN to simultaneously impart reduced substrate affinity and accelerated enzyme-substrate dissociation as compared to bovine chymosin.

U2 - 10.1021/jf300557d

DO - 10.1021/jf300557d

M3 - Journal article

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VL - 60

SP - 5454

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JO - Journal of Agricultural and Food Chemistry

JF - Journal of Agricultural and Food Chemistry

IS - 21

ER -

Comparison of the hydrolysis of bovine κ-casein by camel and bovine chymosin: a kinetic and specificity study

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